Difference between revisions of "Genetic Resources"

Latest revision as of 16:08, 12 August 2021

1 Statement of Purpose
2 Contributors
3 Introduction
4 Developing Policies
- 4.1 Standard Operating Procedures (SOPs)
- 4.2 Guide to operations
5 Funding and Budgets
6 Facility Management
7 Genetic and Genomic Collections Storage
8 Operational Best Practice
9 Genetic Sample Processing
10 Inventory Control and Data Management
- 10.1 Sample labeling and tracking
- 10.2 Databasing for genetic samples
11 Use of Collections
12 Health & Safety
13 Ethical and Legal Best Practice
14 Source Material
15 Links
16 References

Statement of Purpose

This page presents standardized guidelines for the management of genetic collections associated with natural history collections. For information on procedures related to the collection of tissues, see Tissue Sample Collection. These recommended practices are informed by general standards for biorepositories and augmented by information unique to natural history collections with the goal of providing a foundation for those curating genetic samples. Information pertains to all aspects of genetic sample curation and will assist those in making decisions regarding how to collect, store, track, process, and distribute genetic specimen samples. These guidelines provide an organized method to evaluate the relative costs and benefits of various strategies and to prioritize potential improvements and minimize risks to genetic collections, which is applicable to both enhancing a single existing collection, as well as those forming a centralized repository composed of samples from multiple independent collections.

Contributors

Breda Zimkus, Linda S. Ford

Introduction

Researchers associated with natural history museums have made the collection of genetic resources a priority due to their importance in molecular studies, but often the long-term curation of these collections is difficult due to decentralized curation over multiple storage locations and lack of community best practice guidelines for their stewardship. Unlike traditional natural history specimens, the research utility of genetic samples increases with lower storage temperatures and fewer freeze–thaw events and, in addition, their use is consumptive. Collection managers must, therefore, maximize the research potential of each sample by carefully considering use on a case-by-case basis. In addition, collection personnel must always balance institutional goals with the curation needs of their respective collections. Therefore, these recommendations can be broadly or narrowly applied, depending on the mission of the institution and other factors that influence the curation of genetic samples, including budget, staffing, and space.

Developing Policies

Many natural history collections have institutional guidelines that outline how traditional specimens should be curated, but these guidelines generally are not specific enough to address the special curation needs of genetic samples. To ensure that genetic samples are curated consistently for long-term preservation and use, all genetic repositories should develop the following:

Standard Operating Procedures (SOPs)
Comprehensive guide to operations

Policies and procedures should be written by those with experience in the management of the genetic collection and should comply with all governmental and regulatory requirements. All personnel should be trained using these written guidelines to ensure accuracy and consistency of procedures when working in the repository.

Standard Operating Procedures (SOPs)

The SOP document should outline or summarize:

Tasks performed by the personnel of the repository
Scope of activities performed
How the collection satisfies the mission and goals of the institution
Access to the collection
Equipment and tools present
Acquisitions
Accessions
Cataloging procedures
Curation activities resulting from the near-exhaustive or exhaustive use of genetic samples (e.g., subsampling, deaccessioning)
Storage and organization of relevant permits and acquisition documents
Specific requirements for acceptance of genetic samples, including:

- Provisions regarding acceptable sample types

- Preservation methods

- Storage containers

- Sample organization (e.g., sample vials arranged numerically, data and vials submitted concurrently)

Minimal requirements for associated data associated (e.g., submission method, acceptable formats, Darwin Core standards)^[1]
Loans/gifts (e.g., requirements for requesting genetic samples, procedures associated with the approval, explanation of fees)
Information technology needs
Mandatory training for personnel
Health and safety programs
Personal protective equipment (PPE) required
Equipment monitoring
Maintenance activities
Backup precautions
Emergency procedures
Contact order for personnel in case of operational questions or emergencies

Guide to operations

A more comprehensive guide to operations should detail complete day-to-day collection procedures, including:

Specimen processing (e.g., accessioning, cataloging, sample transfer, sample labeling, sample tracking)
Temporary and long-term sample storage criteria
Database procedures
Detailed use of equipment (e.g., operation, calibration, certification, maintenance, repair)
Subsampling procedures
Shipment of loans/gifts
Disposal of waste (including biohazards)

Funding and Budgets

The current and future potential of a collection for researchers conducting molecular studies is highly impacted by the efficient monitoring and storage of the genetic samples. To fulfill their research mission and ensure the long-term conservation of genetic collections, repositories must function efficiently, which requires dedicated and consistent funding. For those collections that are not centralized, the cost of curating genetic samples is often included in the overall budget for the institution or department, or funds come from personal research budgets ^[2]. Comprehensive and detailed budgets allow institutions to:

Ensure that support from internal and external sources is sufficient to offset operational costs
Understand the costs of maintaining their collections
Make informed decisions regarding operations

Facility Management

Regardless of whether genetic collections are in separate locations in an institution or are housed together in a centralized repository, those curating these collections should clearly examine the storage conditions and address any issues related to the space(s). Addressing potential issues, such as restriction of access to collection rooms and/or cold-storage equipment, reorganization of equipment, improvements in lighting, upgrades to flooring, increased ventilation, and backup precautions, can ultimately improve the long-term preservation of genetic samples.

Access and security

Genetic samples have significant inherent value to research because they are often collected from remote locations as a result of costly and time-consuming collection trips. Samples should, therefore, be stored in secure locations to minimize misplacement or inadvertent loss, and their access and use should be limited to those with the appropriate training. A risk assessment should be conducted to assess both building and collection security, including current procedures and protection devices. Many genetic collections currently store samples in a room or facility that remains unlocked during the day, which is likely because many research collections are stored within college and university laboratories allowing student access ^[2]. If access to rooms where genetic resources are stored must remain unimpeded, individual freezer units can be locked with key access restricted to approved and trained users. Policies should be developed in relation to visitors to ensure that they have the appropriate training before working with collections (see OPERATIONAL BEST PRACTICE: Training). Records of training and activity in the collection areas should be maintained and archived for security, as well as health and safety requirements (see OPERATIONAL BEST PRACTICE: Records Management).

Space planning

Space planning encompasses the organization of equipment (e.g., storage units, tools), adequate workspaces, and storage for supplies, in addition to the collections themselves. Although the layout of a functioning work area might not be greatly altered for an established collection, minor changes can be made to the placement of laboratory tables, desks, shelving, biosafety cabinets, or benchtop equipment (e.g., centrifuges, electrophoresis equipment, incubators, rockers, scales, spectrophotometers, tabletop autoclaves), that can increase research efficiency or improve functioning of equipment. Understanding every procedure that will be undertaken in the space will allow more accurate organization of the space, which is essential for those designing a centralized repository, as well as those working to improve the organization of a single laboratory. The inclusion of dedicated space for working with genetic samples or hazardous chemicals (e.g., biosafety cabinet, chemical hood, designated laboratory bench, room) is recommended to protect both personnel and samples.^[3]

Open spaces must be reviewed along with dedicated storage areas to:

Ensure that mechanical refrigerator and freezer units are placed to allow for adequate airflow
Avoid obstruction of exits, access or equipment (e.g., fire extinguishers, eyewashes, safety showers) by dedicating spaces for mobile equipment (e.g., laboratory carts, dewars/cylinders of LN₂)
Consider facility and/or safety issues associated with routes traversed for specimen transport, maintenance of equipment, and delivery of dewars of LN₂, including:

- Elevators (e.g., personnel may not transport pressurized dewars in elevators if ventilation does not accommodate oxygen deficiencies)

- Steep inclines

- Floor surfaces

- Movement through populated and public areas

Lighting

Lighting in the collection space should be sufficient to allow personnel to complete small-scale tasks, including:

Examining vials for cracks
Reading hand-written or typed labels on containers
Subsampling specimens

If the light source is in close proximity to frozen samples (i.e., task lighting), a lighting unit that generates minimal heat (e.g., florescent fixtures, LEDs) should be used instead of incandescent or halogen lighting because these latter can cause samples to thaw. Emergency lighting that functions in the event of power loss should also be present to illuminate exit routes and, if needed, allow personnel to monitor cold-storage equipment (see FACILITY MANAGEMENT: Backup Precautions). Focused, portable light sources (e.g., flashlights, headlamps, battery-powered lanterns) should also be readily available within the collection in case of emergencies or if needed to examine equipment.

Flooring

Flooring used in genetic repositories should be durable enough to accommodate all activities performed in the space and be:

Washable
Able to support heavy cold-storage equipment without cracking
Level so as not to obstruct the movement of equipment, including laboratory carts and dewars (cylinders) of LN₂
Compatible with LN₂ so cracks do not occur with spills or leakage. Additional notes regarding flooring and LN₂:

-Vinyl tile and linoleum are not recommended with the use of LN₂ because they can crack and lift, presenting a hazard.

-Sealed concrete is recommended over epoxy because if LN₂ is spilled on the latter, it can break the seal between the epoxy and concrete, causing cracking

If harder surfaces, such as concrete, are selected because of their durability, anti-fatigue mats should be placed in areas where personnel stand for prolonged periods of time for potential ergonomic issues. Additionally, absorbing mats or floor grates might be needed in the front of refrigerator condensers or in the vicinity of freezers to protect personnel from slipping on occasional condensation or ice.

Ventilation

Ventilation must be adequate in all collection spaces to prevent excess heat or humidity, which cause mechanical units to overheat and create condensation that damages equipment and results in an electrical shock hazard. More importantly, ventilation must consistently maintain sufficient oxygen levels if using LN₂. Using liquid nitrogen for maintaining genetic collections requires constant monitoring of oxygen levels because nitrogen is a colorless, odorless and tasteless gas/vapor that is an asphyxiant, causing oxygen depletion. If LN₂ leaks into an enclosed space from a defective cryovat or supply dewar, oxygen levels might become depleted enough to be unsafe for occupants (see HEALTH AND SAFETY: Liquid Nitrogen Safety).

To understand potential oxygen depletion due to LN₂ use in a genetic collection, the normal evaporative losses from storage vessels and the spillage of the entire contents of a vessel should be estimated for each collection room. Potential oxygen depletion can be determined by analyzing the following:

Size of the room
Evaporation loss for each vessel (reported by the manufacturer as ‘‘volume of LN₂ lost per day’’)
Total spillage of each vessel
Number of air changes in the room per hour

If neither normal evaporation losses nor spillage cause a significant reduction of oxygen content in a room, then general exhaust ventilation or use of natural ventilation (e.g., opening doors, windows) can be considered as an option. Natural ventilation is not always possible, however, because of institutional restrictions or special designations (e.g., Biosafety Level 2 or 3) requiring that windows are sealed and/or doors shut. If risk assessment calculations of potential oxygen depletion indicate that evaporation losses and/or spillage would significantly deplete oxygen concentrations, forced-air ventilation must be installed. For accuracy in such high-risk matters, a professional engineer should be contacted and the health and safety group of the institution consulted.

Forced-air ventilation can include the following:

Extractor fans that run continually, providing 100% exhaust and assuring that none of the cycled air is returned back to the air handler
Fans that are activated manually by the user when alerted that oxygen levels are low
Fans that are activated automatically by an automatic trigger

Fans that use an automatic trigger are recommended over those with manual activation to remove need for human intervention to correct oxygen levels. Automatic activation of an extractor fan can be linked to sensors that detect room occupancy and/or oxygen levels (see FACILITY MANAGEMENT: Oxygen Monitors). Having both occupancy sensors and oxygen levels activate an extractor fan serves as a safety redundancy should one sensor fail. Regardless of the type of ventilation system chosen, exhaust systems should include forced extraction ducts that are installed at low heights close to the floor because cold nitrogen vapors are denser than ambient air and settle at floor level. Exhaust ducts should also be in close proximity to storage units for the most efficient removal. With all ventilation systems, noise exposure from fans must fall within limits recommended by the Occupational Safety and Health Administration (OSHA), and collection managers should contact their environmental health and safety group to evaluate the noise levels and attenuate the fans if needed.

Delta F Series Oxygen Monitor (electrically operated and permanent; sensor positioned close to floor level and not shown)

Oxygen monitors

Ambient air normally contains 20.9% oxygen by volume, but nitrogen gas can quickly displace the air in the event of a spill or failure of storage equipment, reducing the percent of oxygen to unsafe levels. By OSHA standards, a ‘‘hazardous atmosphere’’ can include one that is oxygen-deficient, containing less than 19.5% oxygen by volume. This type of environment exposes people to the risk o incapacitation, injury and possible death. Oxygen monitors should, therefore, be present in all rooms where LN₂ is stored or dispensed, and these monitors are essential in rooms where personnel are working with LN₂ storage equipment. Some ventilation systems using extractor fans can be automatically activated using oxygen levels; these systems can operate independently or be tied into the general room oxygen monitors (see FACILITY MANAGEMENT: Ventilation). Oxygen monitors can be either portable or permanently installed within the collection space:

Portable monitors are small, light-weight, and can be carried by individuals working in a room with LN₂ equipment
Permanent installations (i.e., battery operated, electrical units) ensure constant and consistent surveillance of oxygen levels

- Displays should be mounted approximately at eye level

- Oxygen sensors should be positioned closer to floor level but above the level of any exhaust-extraction fan located in close proximity

- Additional alarms in adjacent rooms or hallways are recommended to prevent personnel from entering an oxygen deficient areas

- Alarm notification to a remote location is a worthwhile precaution so emergency personnel and those responsible can be alerted to problems.

Regardless of whether these devices are fixed or mobile, oxygen monitors should include both audible and visual alarms. To assure that oxygen monitors comply with local regulations and function accurately, a professional engineer should be contacted and the health and safety group of the institution consulted. In addition, some electrochemical sensors used within oxygen monitors are sensitive to the surrounding environment and are subject to drift with barometric changes or can even fail if placed in extremely cold temperatures. Therefore, dedicated maintenance, periodic calibration and regular replacement of sensors is essential for all collections using LN₂.

Backup precautions

Collections that use cold-storage units to store genetic samples should include backup precautions to protect against power loss and ensure constant temperatures, thereby preventing sample loss.^[4] Backup precautions are the necessary counterpart to a monitoring program, which protects samples from loss due to specific equipment failure (see OPERATIONAL BEST PRACTICE: Manual Monitoring). Fortunately, audible or visual alarms are included in many cold-storage units, but are merely the first step in protecting genetic samples. A risk assessment should be conducted to determine the appropriate backup system given the following:

Cold-storage type (e.g., refrigerator, mechanical freezer, LN₂ cryovats)
Institutional infrastructure (e.g., available backup power sources)
Regional factors (e.g., risk of severe weather, proximity to populated areas)
Running duration of each type of backup system

Automatic systems are recommended over those that must be activated manually to ensure that collection storage equipment remains functional at all times, even when personnel are not readily available. It is also recommended that equipment alarms include both on-site and off-site notifications. Off-site alarms include 24-hour monitoring and ensure that the appropriate personnel can be contacted at any time in case of emergency. Contact information for multiple staff members trained to respond to emergencies should be included in the SOP document and posted within the collection to ensure that emergencies and alarms are addressed appropriately and immediately. Written emergency procedures should address how personnel should respond to various situations (see OPERATIONAL BEST PRACTICE: Emergency procedures).

As part of a risk assessment, collection managers should identify what equipment is essential and requires backup power in the event of power loss. Risk assessments should be conducted regularly because contents of individual cold-storage units can change, which might alter priorities for backup power. Mechanical freezers should always be connected to backup power. Managers of collections using LN₂ storage units should consider having backup power for the LN₂ cryovat controllers to ensure that cryovat units continue to receive LN₂ supply from dewars when the commercial power is not present; however, the addition of LN₂ can be done manually if needed (see GENETIC AND GENOMIC COLLECTIONS STORAGE: Liquid nitrogen cryovats). Environmental monitoring systems and safety equipment, such as oxygen sensors, specialized ventilation, and emergency lighting, should also be protected by backup measures.

If regular power is lost, an auxiliary or emergency-power system can automatically connect to emergency power. Most emergency-power systems use diesel, natural gas, or liquid propane gas-driven generators to power essential equipment in a facility. Managers evaluating emergency-power systems should consider the following:

Multiple generators might be necessary to support large collections if many mechanical freezers are present.
Enough fuel should be present to sustain power continuously for at least 48–72 hours, but there also should be an established plan for how fuel supplies can be replenished if needed. ^[5]
An uninterruptible power supply (also called uninterruptible power source, UPS) or battery/ flywheel backup can also provide short-term emergency power if commercial utility power fails. In an emergency situation, these units can provide personnel with essential time to connect to other secondary power sources, such as backup generators. In addition, some mechanical freezers require users to manually restart the unit after a power failure to protect the compressors, and an UPS would make this restart unnecessary.
Power systems should be stored in an easily accessible and dedicated storage space so collection personnel can access them when needed.
All backup power systems should be tested on a regular basis as part of the SOP to ensure that they function and can sustain the electrical load in an emergency.

Genetic and Genomic Collections Storage

The type of storage used in a genetic or genomic collection ultimately influences the potential future uses of samples in molecular research because colder temperatures reduce cellular degradation. Documentation of the number of freeze–thaw events and any chemical preservatives or buffers should also be considered because genetic sample integrity might be reduced, depending on the preparation, as well as the duration and number of freeze–thaw cycles. Collection managers should also track all storage methods utilized from the time of initial collecting and any usage events (i.e., loans/gifts).

Temperature considerations

Cryopreservation at very cold temperatures is considered the most effective technique for the long-term stabilization of genetic samples because it inhibits enzymatic and chemical activity that leads to sample degradation ^[6] ^[7] ^[8] ^[9] ^[10]When genetic sample temperatures are reduced below -137°C (the vitrification point of water), biological activity substantially slows and, at -196°C (the boiling point of liquid nitrogen), DNA degradation virtually stops because there is insufficient thermal energy for chemical reactions. Thus, the type of cold storage chosen for samples affects the long-term viability of those samples, with the most reliable form of cryogenic preservation being the storage of samples at temperatures below -137°C and improving as storage temperatures decrease below this threshold. However, collections might include genetic samples preserved in a number of ways, given size of the collection (including estimated future growth), personnel, funding, dedicated space for equipment, and ength of time the samples will be stored.

In addition to long-term storage in a collection, there must be considerations for short-term storage situations in relation to when samples are collected and transferred, such as for loans/gifts. Various methods, including freeze-drying samples or preparing them using buffers, chemical preservatives, or desiccants, are currently used for the initial preservation of genetic samples. ^[11] ^[12] ^[13] These methods, which generally allow genetic samples to be stored at room temperature, are most appropriate for short-term storage or transport and not for long-term preservation (see GENETIC SAMPLE PROCESSING: Initial preservation procedures). Long-term viability can be increased for genetic samples initially preserved using these methods if they are ultimately stored in a low-temperature environment. In general, genetic samples should be stored at the lowest temperature possible at any available time to reduce degradation and maximize future use.

Liquid nitrogen cryovats

Liquid nitrogen cryovats are cryogenic freezers that are cooled in various ways using a supply of nitrogen in the liquid phase. All methods of cryopreservation that use LN₂ are considered to be the most effective because samples are stored at temperatures below the glass-liquid transition temperature of water (-137°C). There are currently four different storage methods that use LN2:

Vapor-phase cryovat (right) with electronic controller connected to LN₂ supply dewar (left)

Vapor-phase cryovats with LN₂ present below sample racks (≤-150°C; most commonly used method by collections surveyed^[2])
Liquid-phase cryovats that allow submersion of samples in nitrogen (-196°C)
Isothermal cryovats with a specialized jacket surrounding the interior chamber and allowing nitrogen vapor to enter the freezer space via directional vents (approximately -190°C)
MVE Vario cryovats (-50°C to -150°C) that allow LN₂ to flow through a heat exchange system located in the top head of the freezer, using vaporization energy of the LN₂ to cool the unit

All four types of cryovats are available in various sizes with vial capacities that range from approximately 20,000–100,000. Use of liquid-phase cryovats are not recommended because nitrogen in a liquid state can penetrate all commercial cryogenic vials if not placed in secondary containment (e.g., polyethylene tubing), making them at risk of exploding when they expand upon warming (see GENETIC SAMPLE PROCESSING: Storage containers). In addition, cross-contamination can occur when immersing samples directly in LN₂ without securing the cryovial in secondary containment.^[14] The circulation of vapor within isothermal cryovats allows for improved visibility due to less clouding at the top of the chamber, but these cold-storage units have increased consumption of LN₂ when compared to traditional vapor-phase cryovats. MVE Vario cryovats are the newest freezer systems, having the benefit of a dry storage area, but this technology is not yet used or tested by natural history collections.^[2]

Most liquid nitrogen cryovats are equipped with electronic controllers that automatically monitor and regulate the supply of LN₂ to the unit. Liquid levels, temperature readings, and alarms are generally displayed on a controller unit panel. Cryovats with electronic controllers generally use a two-sensor system to detect LN₂ at user-defined levels. When LN₂ levels are below the low-level sensor, a solenoid valve is opened, allowing product to enter the cryovat from a nearby source (e.g., small-volume dewar, large volume bulk tank) connected via a cryogenic hose and/or vacuum-jacketed piping (see GENETIC AND GENOMIC COLLECTION STORAGE: Liquid nitrogen supply). When LN₂ levels reach the high-level sensor, the solenoid valve is closed, stopping the flow of product into the cryovat. In addition to both on-site and remote alarms, it is paramount that cryovats are checked at regular intervals and levels of LN₂ are recorded (see OPERATIONAL BEST PRACTICE: Manual monitoring). When using LN₂ cryovats, backup power for the electronic controller functions to keep a continuous supply of LN₂, although the unit itself stays cold without power (see FACILITY MANAGEMENT: Backup precautions). If a cryovat controller unit that automatically dispenses LN₂ is not connected to a backup system, readings of LN₂ levels and the addition of more product (i.e., pouring LN₂ into the cryovat) need to be done manually; LN₂ would likely need to be supplied at regular intervals to maintain ultracold temperatures if power remains off for an extended period of time. In the event of a power failure, collection procedures should detail if and when cryovat lids are opened to minimize use of LN₂ (see OPERATIONAL BEST PRACTICE: Emergency procedures).

Liquid nitrogen supply

A liquid nitrogen bulk tank at Palatine in Illinois (Joe Ravi [CC BY-SA 3.0], via Wikimedia Commons)

Liquid nitrogen to supply cryovats can be obtained and stored in three ways:

Delivery in small-volume dewars (cylinders)
Delivery to large-volume bulk tank
Self-production using an on-site LN₂ plant

Delivery in small-volume dewars (cylinders) by a commercial vendor can be done needed on a regularly scheduled basis. For most small collections, mobile dewars (up to 240 liters) are sufficient to supply cryovats. Dewars are generally placed in close proximity to the cryovats and connected with cryogenic transfer hoses, unless permanent vacuum-jacketed piping designed to transfer cryogenic liquids is installed within the repository. Dewars themselves can be purchased and refilled by a delivery vehicle, or these storage vessels can be leased so that an empty dewar is exchanged for a full one. In addition, Department of Transportation (DOT) codes regulate the specifications of liquid nitrogen delivery vessels in the USA, so collection managers should be aware if these regulations affect their delivery. LN₂ deliveries should be scheduled to minimize the amount of time that a dewar is not connected to a cryovat to ensure that a cryovat has a steady supply of LN₂.Collection managers should be aware that LN₂ evaporates at a constant rate, which can be affected by the atmospheric conditions, vessel integrity, and manufacturing tolerances.

For large collections with many cryovats, a pressurized bulk or microbulk tank should be considered. Depending on the size of the bulk vessel, the tank might need to be located outside of the building where the collection is housed. If bulk tanks are placed indoors, itmight be possible for external wall boxes to be installed to allow bulk tanks to be filled without having to enter the building. Costly vacuum-jacketed cryogenic pipes are needed to deliver the LN₂ from the tank to the point of use, so for cost efficiency, bulk tanks should be located as close to the cryovats as possible. In many areas, bulk tank storage is regulated by city or state ordinances; oxygen monitors are also essential if these storage units are placed indoors (see FACILITY MANAGEMENT: Oxygen monitors).

In smaller collections that are located in remote locations where LN₂ cannot be easily delivered, collection managers might consider the use of LN₂ plants, which generate nitrogen by separating it out from the ambient air. The plant-generated LN₂ is stored in a tank that then can be moved and connected to a cryovat.

Mechanical freezers and refrigerators

Storage methods used by genetic resource collections surveyed by in 45 independent collections at 39 different institutions for all collections surveyed (dark grey) and centralized repositories (light grey).^[2]

Mechanical freezers and refrigerators offer a large range of storage temperatures, including ultracold freezers (-50°– -86°C), general-purpose or laboratory freezers (-12°– -30°C for manual defrost models; automatic defrost models allow temperatures to fluctuate more broadly), and general-purpose refrigerators (1°– 12°C). As previously discussed, cryogenic storage at extremely low temperatures is considered the most effective method for the long-term stabilization of genetic samples. However, refrigeration is sometimes considered for short- or long-term storage if certain buffers or chemicals were used in sample preservation, and these additives only require that genetic samples be kept below ambient temperature. Collection managers must record all chemical additions and preservatives used with their genetic samples to ensure that the samples are stored at the appropriate temperature recommended by the manufacturer. If multiple cold-storage methods are used within a collection, the SOP should clearly outline the criteria for storing samples at the different temperatures.

Freezers and refrigerators are available in a variety of sizes, styles, and voltages, including upright or chest configurations. Many models are available with locks for additional security (see FACILITY MANAGEMENT: Access and security). Collection managers should ensure that each electrical unit has a dedicated circuit so power is not overloaded, and that units are positioned to allow for sufficient airflow around them (see FACILITY MANAGEMENT: Space planning). Heat released from cold-storage equipment should be monitored and counter-balanced by an HVAC or cooling system when needed. Those collection managers purchasing new equipment should consider freezer units that have increased energy efficiency, which generally ensures that less heat is emitted to the surrounding air. Compressors can also be placed outside of the building for some freezer units, removing the need for HVAC or cooling in the collection space where the mechanical freezer is located. Fortunately, compressor systems on newer cold-storage units include those being cooled by water, whereby valves connected to local water sources automatically control the flow needed to maintain cooler compressor temperatures, which enhance the stability and reliability of the unit. Because cold- storage units are integral to the functioning of a genetic or genomic collection, the SOP should outline specific protocols for regular preventative maintenance and emergency repair of all mechanical units (see OPERATIONAL BEST PRACTICE: Equipment preventative maintenance, repair, and replacement).

Mechanical freezers and refrigerators require less dedicated time in their day-to-day operation when compared to LN₂ cryovats, but collections have an increased risk of loss in the event of mechanical breakdown or power disruption. Even a short power outage can be detrimental to samples being stored in a mechanical cold-storage unit. Battery backup systems or an UPS are needed to maintain units in the event of a short power outage or until power can be switched over to a robust backup system for longer term emergencies (see FACILITY MANAGEMENT: Backup precautions). Internal and, if possible, remote monitoring should be present to prevent sample loss due to mechanical failure of units (see OPERATIONAL BEST PRACTICES: Manual monitoring). To safeguard against all possible risks, including power outage and mechanical failure, both monitoring procedures and backup precautions should be clearly outlined in the collection SOP.

Operational Best Practice

Genetic and genomic collections are more equipment- and personnel-dependent than traditional natural history specimens, with more catastrophic consequences if storage equipment fails or samples are handled improperly. In addition, genetic samples are consumable resources, so they become more limited with each use for research.

Facility functions and services provided

Genetic resource collections can provide many key services to fulfill institutional missions and assist internal and external researchers in achieving project goals. How broadly and consistently these key services can be addressed is related to how genetic collections are set up at an institution (i.e., separate locations or centralized facility). The main functions of most centralized genetic resource facilities associated with natural history museums include ^[2]:

Sample storage
Sample tracking
Sub-sampling and/or processing of loans/gifts

A small percentage of repositories provide additional genetic laboratory functions, including DNA/RNA extraction, polymerase chain reaction (PCR), and sequencing.^[2]

Besides genetic sample maintenance, additional research services could potentially be provided by genetic resource collections, including assistance with project planning or proposal submissions, sample collecting, assistance with sample transportation from the field, sample quality assessment using spectrophotometry or other methods, and student or intern training.^[15] Collections could also provide or lend supply materials for those researchers who will be depositing samples in the biorepository, including sample vials, sample boxes, reagents, LN₂ dewars, dry shippers, LN₂, or dry ice. To ensure that sufficient equipment, supplies, trained personnel,and funding to maintain high-quality specimens are available, and to potentially offer additional services, collection managers should clearly outline priorities, as well as the molecular laboratory tasks performed by collection staff (e.g., DNA/RNA extractions, fluorometric/spectrophotometric quantification of DNA, DNA barcoding to identify or confirm identifications) in the SOP document.

Personnel

Genetic and genomic resource collections must be managed properly and continuously to ensure that samples are properly stored and maintained. Depending on the size of the collection and institution type, personnel might include a single manager or numerous employees. A recent survey of genetic resource collections associated with natural history museums found that the vast majority had curators/professors with higher academic degrees or collection managers with higher degrees maintaining the collections ^[2]. Other personnel working with genetic resources included:

Collection managers without higher degrees
Staff or technical assistants
Paid and unpaid student assistants
Volunteers

At minimum, collections staff should include a dedicated manager who is trained to manage the day-to-day activities within the collection and can ensure that all procedures are completed as instructed in SOP documents. A collection manager also prevents unauthorized access to storage areas, thus protecting samples from misplacement, accidental thawing, or contamination^[16]. Duties and reporting relationships for each staff member should be clearly outlined in a written job description. Collection managers should ensure that all personnel working in the collection have the appropriate training to undertake the duties assigned in their particular job description, especially with regard to health and safety issues. Proper maintenance of genetic resource also requires assistance from additional departments outside of those working directly with the collection, including building maintenance and operations, environmental health and safety, information technology, and security.

Training

All genetic collection staff must receive adequate training to ensure that they can perform all aspects of their job description and follow all policies and regulations, including those mandated by international, national, regional, and local statutes. All new personnel, including staff, students, interns, and volunteers, should be trained by authorized staff to understand the details and justification for the SOP documents and comprehensive protocols. Policies should also be developed in relation to both short-term and long-term visiting researchers to ensure that they have the appropriate training before working with collections. Training should include the following:

Best practice for working with genetic resources (see GENETIC SAMPLE PROCESSING: Sample transfer; USE OF COLLECTIONS: Aliquoting samples)
Database usage and the proper storage of samples in accordance with corresponding database records (see INVENTORY CONTROL AND DATA MANAGEMENT: Databasing for genetic samples)
Safety and security, including the appropriate use of tools and equipment, proper personal protective equipment, and risks of working with chemicals and biospecimens

Internal records should be kept of all approved personnel and dates of their various training events, especially because some training requires mandatory updates at regular intervals. All training programs should be regularly assessed to make sure that information is up to date, and it is recommended that training be done in collaboration with the health and safety group at the institution.

Manual monitoring

The viability of genetic samples is dependent on storage equipment operating at optimum efficiency. Collection procedures should clearly outline how to monitor and check collection equipment, how often it should be done, and how to maintain documentation. Diligent and consistent monitoring of the following equipment should be completed:

Cold-storage equipment

- Personnel should visually inspect and record the temperature of the equipment on a regular basis (e.g., daily, multiple times per week).

- Levels in liquid nitrogen cryovats should be measured manually on a regular basis to confirm that the measured levels match the control displays

- Temperature and nitrogen-level data should be tracked on a regular basis to identify problematic trends

Transportable pressurized vessels, including dewars (cylinders) of LN₂, should be examined upon receipt from outside vendors

- Dewars should be checked to ensure that pressurization is compatible with the cold-storage equipment

- Dewars should have no be visible damage or leakage

- When in use, these vessels should be closely monitored to estimate rate of use and ensure that valves are functioning properly

Equipment preventative maintenance, repair, and replacement

Proper functioning of cold-storage equipment is essential for the long-term stability of genetic material. All equipment should have regular routine maintenance in accordance with the recommendations of the manufacturer. Preventative maintenance of mechanical freezers should include:

Comparing the temperature set-point versus the actual temperature (see OPERATIONAL BEST PRACTICE: Manual monitoring)
Testing backup batteries
Ensuring that gaskets and seals are intact without tears
Routine cleaning of freezer coils and condenser filters
Regular defrosting

In addition to increased dependability, regular maintenance of cold-storage equipment, such as mechanical freezers, is associated with significant energy savings.
Liquid nitrogen cryovats should have routine maintenance to ensure:

Internal temperature sensors function properly
LN₂ readings are accurate
Fill valves operate normally
Alarms activate under the defined conditions
Insulating materials (e.g., polystyrene foam) do not have cracks or built-up frost
No ice or frost build is present in sensor tubes

Biosafety cabinets and chemical fume hoods should be tested and certified routinely to ensure that they are functioning appropriately and in compliance with both local regulations and any requirements associated with biosafety level status. Oxygen monitors also need regular maintenance and/or calibration as life safety equipment (see FACILITY MANAGEMENT: Oxygen monitors). All safety equipment, including eyewashes, safety showers, fire detection units, and fire suppression systems, should be tested regularly to ensure reliability, which is generally best accomplished in collaboration with the health and safety group of the institution. Managers should keep records of all routine and special maintenance, including dates, description of the issues (e.g., alarms, incident reports), tests performed, and actions taken to resolve any problems. The SOP should provide plans, including instructions and schedules for preventative maintenance, calibration, repair, and replacement of equipment.

Regular assessments of equipment should be made by collection managers to help establish a timeline for replacement. Mechanical freezers generally last from 5 to 15+ years with manufacturers reporting a range of 8–12 years, whereas liquid nitrogen cryovats generally last longer, functioning for 10–35 years ^[17]. Collection managers should track the ages of all equipment and know the manufacturer’s expected lifespan for each. Based on the age and performance of the equipment, long-range plans for replacement can be anticipated and replacement funding can be ensured. If a cold-storage unit should fail, written procedures should be in place to identify how to transfer the samples from the failed unit to their emergency storage location (see OPERATIONAL BEST PRACTICES: Emergency procedures).

Records management

Collection managers should maintain records that detail collection, processing, storage and use of samples. Copies of all relevant permits and acquisition documents, which detail the legal attainment of all genetic samples either alone or associated with traditional voucher specimens, must be maintained for both legal obligation and assessment of the sample history and quality. Up-to-date records should be available that document personnel training, equipment activity (e.g., monitoring, preventative maintenance, repairs), safety inspections, and legal compliance (e.g., active permits) as outlined in the SOP.

Genetic sample data can be recorded as part of an institutional database, which potentially tracks both the original voucher specimen and any subsequent associated genetic or genomic derivatives, or a stand-alone tracking system that is used only for genetic samples (see INVENTORY CONTROL AND DATA MANAGEMENT: Databasing for genetic samples). Documentation of genetic sample locations in cold-storage units should be as precise as possible so that samples can be located quickly (see INVENTORY CONTROL AND DATA MANAGEMENT: Sample labeling and tracking). Dates can be easily confused because their format differs throughout the world; thus, recorded dates should be formatted consistently and in an unambiguous manner. Security for electronic records should include password protection and automatic time-outs on computers and online databases, as well as scheduled backups for all data. Large collections should have electronic records backed up daily on a network or remote secure server, whereas small collections might consider doing local backups on a weekly basis.

Emergency procedures

Collections should have emergency procedures, including evacuation procedures and detailed disaster plans, outlined in their SOP to address how personnel should respond to various situations, ranging from laboratory incidents to natural disasters^[18] ^[19]. Generally, emergency procedures and disaster preparedness should be developed to address incidents at various levels of involvement, including:

Issues confined to the genetic collection (e.g., clean-up of chemical spills, transfer of genetic samples from a failed cold-storage unit)
Building-wide or institution-wide events (e.g., flood or water damage as a result of plumbing issue or roofing leak)
Local issues (e.g., city-wide power outage)
Regional events (e.g., earthquake, hurricane, tornado, tsunami)

Because emergencies with genetic resources can become disasters if immediate action is not taken, it is recommended that a risk assessment is conducted and personnel have regular reviews and drills to ensure their familiarity with emergency procedures and backup plans for every conceivable situation (see FACILITY MANAGEMENT: Backup precautions). It is also essential that personnel are familiar with the locations of all equipment and tools needed to quickly and efficiently perform their responsibilities during each type of emergency, ranging from how and where to transfer samples from a failed unit to how to turn on backup power during a power outage. Contact information for personnel responsible in case of emergency in the order that they should be contacted, facilities managers, and outside contacts for emergencies (e.g., power companies, fuel supply companies, important contractors) should be included in the SOP document, provided to those responding to off-site alarms, and clearly posted in the collection. Contact information should be regularly reviewed to ensure that it remains current.

Genetic Sample Processing

Genetic samples require specialized storage to maintain their viability, but the manner by which they are initially preserved when collected and any subsequent changes made prior to their deposition in a collection also greatly affects their utility in research. In addition, procedures used by collection personnel to prepare the samples for deposition in long-term storage can have detrimental consequences if not completed properly.

Initial preservation procedures

The methods currently used to preserve genetic material during initial sampling vary widely owing to the sampling location, tissue type, and intended research use. A comprehensive treatise of methods to preserve genetic samples is discussed in Nagy (2010)^[20]. Of all the methods examined, flash-freezing using liquid nitrogen or a mixture of dry ice and ethanol is considered to be the one of the best ways to preserve samples because the speed by which the sample is frozen prevents large ice crystals from forming and no preservative is needed, which maximizes the research potential of the sample. Some chemical agents or buffers (e.g., glycerol, dimethyl sulfoxide [DMSO]) are used to protect macromolecules and/or tissue integrity from damage caused by ice formation during cryopreservation techniques. Buffers, chemical preservatives, and alcohols, especially ethanol, do not require immediate refrigeration and are frequently used for the initial preservation of samples because it circumvents the complicated logistics involved with flash-freezing samples in the field or keeping them cold during transport. All preservation techniques have caveats to their use, however, and genetic resource collections must be fully aware of both the benefits and limitations to make informed decisions.

Methods and preservatives used in the initial preservation of genetic samples in surveyed collections^[2]. Responses in the “Other (F)” category included lysis buffers, buccal swabs, silica gel dessicants, and FTA paper®.

In a recent survey of genetic resource collections associated with natural history museums, samples were found to be initially preserved in a variety of different ways ^[2]:

Flash-frozen
Preserved with ≥ 95% ethanol (zoological samples)
Buffers and chemical preservatives

- DMSO (in many different aqueous solutions; one of the most commonly used formulations is a salt-saturated solution of DMSO (20% DMSO, 0.25 M ethylenedi- aminetetraacetic acid [EDTA], sodium chloride [NaCl] saturated, pH 7.5^[20])

- RNAlater (Ambion, Austin, TX)

- Allprotect Tissue Reagent

- Lysis buffers

Buccal swabs
Whatman FTA (GE Healthcare Bio-Sciences, Pittsburgh, PA) filter paper

Desiccation methods, commonly used to preserve botanical samples, use either physical processes or chemical agents to dehydrate samples. These methods can be very effective in preserving samples if they are maintained in a humidity-controlled environment after the desiccation process. Physical processes that lead to desiccation include:

Sun-drying
Air-drying
Flash-drying
Oven-drying
Vacuum-drying
Freeze- drying

Substances that induce natural desiccation include:

Rice
Sodium chloride (NaCl)
Calcium sulphate (CaSO4, commonly known as drierite^[20])
Sodium silicate (obtainable in powder, crystal or gel form).

Freeze-drying (lyophilization or cryodesiccation) is the controllable dehydration of samples by vacuum desiccation. This method involves the conversion of water within the sample into ice, crystallization of the sample, sublimation of ice under a vacuum, and subsequent evaporation of remaining water from the crystallized sample^[21]. Silica gel beads are commonly used by botanical collectors as a desiccant with the advantage that whole samples can be stored at room temperature as long as the material is stored in tightly sealed containers and are regularly checked for dryness^[22].

Chemical desiccation, which involves adding a chemical to extract moisture from samples, can be completed using a number of different substances, including:

Amyl acetate
Hexamethyl-disilazane
Xylene (which is the chemical Dimethylbenzene),
Methyl cellosolve/cellusolve (also known as ethylene glycol monomethyl ether)
Calcium oxide (CaO, commonly called lime)
Sulphuric acid (H₂SO₄)

Each of these chemical methods has certain considerations for the samples and personnel that should be closely examined before working with them^[23]). Regardless of the method of desiccation, moisture content must be continuously controlled or samples quickly degrade. In addition, samples preserved in this manner are more sensitive to thermal decay at higher temperatures due to their reduced water content and should be stored in a low-temperature environment as soon as possible to ensure that samples remainviable.

Collection staff often does not have control of how genetic samples are originally preserved, and most genetic resource collections associated with natural history museums accept samples that are preserved using numerous different methods^[2]. As more information is discovered about preservation methods themselves, it is becoming more important to know how samples were preserved and handled. Collection managers should make every effort to record the initial preservation methods used and any subsequent changes to storage for their samples, including media or containers. Both media and temperature can affect the ways that samples can be used for future molecular analysis; thus, all curation data for genetic samples should be made available to researchers before their selection and use. Research advancements are constant in molecular studies, and future technological developments might allow for the stabilization and storage of biological samples at room temperature, which could eventually eliminate the need for low-temperature storage environments for newly collected samples. To determine if these new emerging technologies will be effective for existing genetic collections, the detailed curation history regarding how each individual sample was preserved, stored, and utilized will become increasingly important.

Storage containers

Genetic resources can be stored in a variety of ways, depending on the tissue type, sample size, and cold-storage methods used in a collection. Primary storage containers of the samples themselves can include plastic bags, paper envelopes, reaction plates, or vials. When primary storage containers are accessioned into a collection, they must be examined to determine if they are appropriate for the type of cold storage being used in the collection. The SOP should clearly define acceptable storage containers and encourage their in-house researchers to use them because any variation could involve material and staff costs to rectify. For all types of cold storage, the most commonly used sizes of vials are between 1.2 and 2.0 ml, which is the size and configuration that maximizes storage capacity while retaining ease of handling ^[2].

One area of immense variability is with the number of vial types used in natural history collections ^[2]. Potential vial issues are the same for both mechanical freezers and cryovats, although more extreme for cryovats because of their colder temperatures and quicker temperature change. Samples stored using LN₂ must have vials that are rated for use with cryogenic temperatures, which are most often made of polypropylene and include screw-top caps. Some additional useful information about vials include:

Vials used during initial collection (dark grey) and final storage (light grey) of genetic samples in surveyed collections^[2]. Variation in the types of vials included location of the threads internally or externally on the vial opening, and vials caps with or without gaskets.

Glass vials are not recommended because of their fragility when handling and vulnerability to cracking when stressed.
Microcentrifuge vials with pop-off lids are not recommended because liquid nitrogen can enter them and cause them to open or explode.
Self-standing vials (flat-bottom or skirted) may be useful to curatorial staff.
Vials that allow for locking into a rack for one-handed operation may allow curatorial staff to process samples more quickly.
Vials can have threads located internally or externally on the vial opening.

- Externally-threaded closures promote more sterile conditions because internal threading can allow contaminants to enter if the cap is placed on an unclean surface when removed.

- Externally-threaded vials can be susceptible to cracks and loss of air-tightness, which can lead to sample dessication or oxidation ^[24]^[25].

- Internally-threaded vials might allow increased storage capacity, depending on the vial selected, but users also suggest that material can be trapped within the threads of this vial type^[26].

Some manufacturers suggest that vial caps that incorporate a silicone gasket or O-ring (internally or externally threaded) are ideal for vapor-phase LN₂ freezing because the seal is enhanced, but care must be taken if the vial cap is over-tightened because the gasket can become distended. In addition, the presence of gaskets or O-ring might improve the initial performance of seals but can be problematic when used with some alcohols (e.g., ethanol) because some gasket material, such as silicone, is vapor permeable.
Vial manufacturers recommend that samples not be immersed in LN₂ unless they have secondary containment because the accidental entrapment of liquefied nitrogen inside the vial leads to pressure build up and, upon removal, rapid vaporization of the liquid can result in leakage or even explosion (see HEALTH AND SAFETY: Liquid nitrogen safety). Heat-sealing vials into flexible polyethylene tubing is recommended for safe storage in the liquid-phase environment.

Depending on the size of the samples and their primary storage method in the collection, various secondary and tertiary storage containers (e.g., boxes, cassettes, sample storage canes for immersion in LN₂, racks) can be used to organize samples and maximize space. The majority of natural history museums recently surveyed organizes their collections with a vial box and rack system^[2]. The box-and-rack system is a simple but effective way to maximize space within a cold-storage unit and reduce the amount of time needed to search for a specific box. The overall cost of box-and-rack systems depends on the style and number of both the boxes and racks purchased. The use of racks also decreases potential risks to the collection when personnel are retrieving samples. Collections without racks often stack boxes on top of one another within cold-storage units, forcing personnel to remove or displace boxes to access those underneath or behind. In addition, the movement of individual boxes to retrieve samples requires more time, increases the possibility that samples will thaw, and decreases the chance that boxes will be put back in their original location. Lastly, racks allow samples to be quickly moved to other freezers in the event of a freezer failure and decrease the possibility that samples are misplaced while in a temporary storage location.

Racks systems made from aluminum or stainless steel can house most standard-sized boxes and can be oriented horizontally or vertically to fit in mechanical upright or chest freezers, as well as LN₂ cryovats. Aluminum might be chosen for racks in collections that need precise and controlled freezing of samples because this metal is a better energy conductor than stainless steel. Stainless steel racks are more durable and, because the steel does not oxidize, they remain clean. Racks most often come with a locking rod that runs through the front of the shelves, ensuring that boxes are held in place when the rack is moved. Racks also can have spring clips instead of locking rods, which allow quicker access to boxes, but can be problematic if the racks are bumped or dropped. Identifiers can be added by riveting or etching onto racks, or by labels (e.g., unique locating identifiers, barcodes) that can be affixed to the tops of racks and rack shelves (see INVENTORY CONTROL AND DATA MANAGEMENT: Sample labeling and tracking).

A number of different types of vial storage boxes can be used, such as cardboard, chipboard (paperboard), fiberboard, metal, polycarbonate, or polypropylene. It is recommended that moisture-proof boxes be used even though they are more costly, because water repellency increases their long-term durability. When purchasing new boxes, care should be taken to ensure that they are compatible with both the existing rack system and the cold-storage equipment. Collection managers should be aware that polypropylene boxes with hinged lids, which are often used in the field because they are shatter-resistant and have attached lids, might not fit in standard-sized racks. In addition, personnel in collections using either the liquid or vapor phase of nitrogen should use boxes with holes or slots present on the underside of the box to allow the LN₂ to drain. Collections using cryovats should confirm that particles of cardboard, chipboard (paperboard), or fiberboard will not prevent equipment from functioning properly if boxes begin to degrade; otherwise, a more durable type of box should be used. Aspects of ordinary use are another important consideration for storage boxes in a collection. Collection managers should be aware that boxes that have numbered, gridded inserts inside might be difficult to read after being removed from cold temperatures because of frost. In contrast, boxes with grid numbering present on the lid, rather than the box itself, can have frost easily wiped off; however, finding the correct vial may be difficult once the lid is removed because care must be taken to keep the lid numbering aligned with the internal grid.

Sample transfer

When samples are received by collection staff, they might need to be transferred into new primary storage containers, especially if they are stored in a manner that is incompatible with the cold-storage system or if initially preserved in sub-optimal conditions for long-term storage (e.g., preservatives need to be removed). Collection personnel should ensure that contact between different specimens is avoided and all instruments used in the tissue transfer process are handled in such a way that ensures that biological contaminants are destroyed. Disposable equipment (e.g., single-use blades, disposable forceps) replaced after on use greatly reduces the chances of sample contamination, but this practice can become too costly for many collections. Several methods (e.g., heat/flame, chemical agents, steam sterilization in an autoclave) can be used to prevent contamination between genetic samples, but collection managers must be sure that their particular procedures denature or destroy all contaminating genetic material. Some practices, such as cleaning instruments using detergent and water, render instruments and surfaces safe to touch, but these methods do not protect samples from cross-contamination. Disinfection of work surfaces, decontamination of equipment, and sterilization procedures are all needed to ensure safe operations for both staff and genetic samples, and these techniques can vary depending on the task at hand.

Comprehensive procedures should clearly outline which handling methods are appropriate for the various tasks when working with samples. Some techniques, such as autoclaving and use of UV light, destroy all biological matter but require a longer time to accomplish, and thus are better utilized before and after processing a batch of samples. Alternatively, other methods, such as heat/flame or hydrogen peroxide, could be used to immediately decontaminate subsampling tools and ensure no cross-contamination while working through a batch of samples, because ease and speed of use is important. If a chemical agent such as hydrogen peroxide or bleach is used to clean equipment or surfaces, procedures should ensure that those agents do not contaminate samples because these techniques destroy biological matter (e.g., dry instruments thoroughly before manipulating samples). Personnel should also be careful not to inadvertently contaminate the samples by touching their own body or clothes, or allowing hair to come in contact with samples. In addition, they should always wear the proper PPE to protect genetic samples and for their own personal safety (see HEALTH AND SAFETY: Personal protective equipment).

Inventory Control and Data Management

The ability to find a specimen is essential for the curation of any natural history collection. The manner by which the physical locations of genetic samples are tracked is particularly important in their curation because it is virtually impossible for personnel to search the entire collection if a particular sample is missing. In addition, proper inventory and data management allows collection managers to maximize the capacity of their cold- storage units while reducing the amount of time needed to locate samples, which is crucial given that the quality of some genetic material can be reduced with each freeze–thaw event.

Sample labeling and tracking

Proper sample tracking is key to ensuring that cold-storage equipment does not have to remain open for long periods, or samples are not repeatedly exposed to temperatures that initiate thawing. An appropriate tracking system could include:

Sample labeling
Multiple levels of container labeling
Use of a database to record sample location data
Using a convention for numbering that assigns unique locating identifiers (e.g., barcodes) to all levels of sample storage (e.g., primary, secondary, and tertiary containers)

It is recommended that for maximum efficiency, sample vials stored within LN₂ cryovats or mechanical freezers should have unique locating identifiers assigned to the cryogenic vials, as well as unique locating identifiers assigned to the associated boxes, shelves within racks, racks in their entirety, and individual cold-storage units. Each sample vial can then be located in the collection by a unique location number combination. Any labels placed on vials or storage containers should be typewritten or computer-generated; hand-written identifiers might be difficult to read due to the handwriting or decomposition of the ink as a result of cold temperatures or mechanical friction. Upon arrival to a collection, samples might need further curation to meet collection standards, including the addition of typewritten or computer-generated labels to vials or the transfer of samples into the appropriate type of vials. Extreme care must be taken because most genetic samples are initially labeled using reference numbers written on the vial by the researcher. All label placements should be tested under projected environmental conditions to ensure that ink, adhesive, and the label itself withstands the cold-storage temperatures. On secondary containers, such as boxes or racks, labels should be placed in areas where friction is minimal to reduce the risk that the label face is worn down by repeated scratching or rubbing.

Barcodes labels rated for cryogenic conditions or vials manufactured with barcodes are commonly used by genetic resource collections to facilitate sample tracking, including for primary and other hierarchies of containers ^[2]. Preprinted or self-printed barcode labels that are mostly transparentand wrap completely around vials, allow information hand-written on the vials to be viewed when positioned over the writing. Vials manufactured with barcodes on the side or bottom are less commonly used, most likely because these vials rarely have an area where researchers can include hand-written information. Barcodes inserted into vial caps do facilitate he barcoding process because they require less handling time when compared to vial-wrapping labels, but there are added risks that inserts could fall out or a cap could become disassociated from the vial itself. Radio frequency identification (RFID) tags transmit unique locating identifiers associated with tagged objects and, unlike traditional barcodes, these tags do not need to be within the line of sight of the reader. RFID technology is currently being used only to track secondary and tertiary containers (e.g., boxes, racks) within the natural history community, but this method could potentially be used to track primary containers when the tag size and associated costs decrease ^[2].

Databasing for genetic samples

By their nature, genetic resource collections generate and track a large amount of data associated with their samples. A computer-based inventory system, such as a stand-alone database, internal spreadsheet, or networked database, is essential so that all sample metadata can be tracked^[27]. The system should have the capacity to assign a unique identifier to each genetic sample entered in the database and associate all derived genetic samplings and derivatives with the original specimen, which might be the original genetic sample itself or a traditional voucher specimen. It is essential that a tissue sample or genetic extract can be readily linked to the traditional voucher specimen. Changes/updates to data, including taxonomic identification, should be made to all preparation types, even if data are tracked separately for the traditional voucher specimen and genetic sample, The chosen database should accommodate for museum-wide variables given that traditional voucher specimens are likely housed apart from their associated genetic samples due to their different storage and conservation needs and, in addition, personnel curating these two collections are likely different. Regardless of the chosen database, data standards are also critical to ensure that the format of the information, syntax and punctuation are consistent, allowing databases to function as research and curation tools when used in basic queries, enhances the exchange of data among research and informatics partners, and facilitates the utilization of data with data aggregators (e.g., Global Biodiversity Information Facility [GBIF], iDigBio, VertNet).

Those curating genetic resource collections associated with natural history museums are currently using a number of different platforms to track data, including^[2]:

Free-access database application systems developed for museums (e.g., Arctos, Specify)
Commercial database application systems (e.g., FileMaker Pro, Microsoft Access, FreezerPro)
Web delivery through data aggregators (e.g., GBIF, HerpNET, ORNIS)
Internally written applications

All of the systems currently being used have benefits and drawbacks; before selecting a system, collection managers should evaluate the size of their genetic resource collection and internal computing resources, and determine how to integrate o link data associated with genetic samples and traditional voucher specimens. Free database application systems developed for natural history collections can easily associate specimen parts, but these systems might need to be customized to include data fields specific to genetic samples, such as changes to preservation, freeze–thaw events, and remaining volume. Some commercial systems (e.g., KE EMu) can accommodate genetic sample data, but some collection managers might find annual license fees too costly to maintain. Also, some specialized systems (e.g., FreezerProH) can prioritize sample location data, which is important for a larger genetic collection, but disassociates traditional voucher specimen data from genetic samples. The use of a web-based data aggregator (e.g., Global Genome Biodiversity Network [GGBN^[28]], GBIF) can allow external users to access data, but an internal platform is still necessary to allow collection personnel to track genetic sample metadata. Internally written applications might seem ideal because they can be tailored, but they require personnel dedicated to their development and maintenance, and who have an understanding of how to build the system with the flexibility and scalability needed for data and metadata growth.

Use of Collections

Most natural history museums have active loan/gift programs, but the consumptive nature of genetic resources requires collections to develop specific policies to address the demand on this unique type of collection. Genetic collections must also ensure that the manner by which genetic samples are processed and transported preserves the integrity of the original sample and all subsequent subsamples.

Loan policies

In the context of natural history museums, a loan is a temporary transfer of a single specimen or lot of specimens, generally for research, for a specified period of time. Most loan policies for traditional natural history specimens are applicable to genetic samples but, owing to the consumptive nature of this resource and unique issues related to custodianship, clear policies should be developed in relation to the distribution of genetic samples. Baker and Hafner (1984) suggested that the term ‘‘loan’’ be replaced with ‘‘gift’’ or ‘‘donation’’ when discussing transfer of genetic samples between collections and researchers because the specimens are not returned; however, Zimkus and Ford (2014)^[2] found that some genetic collections do request unused samples to be sent back. Loan/gift policies should be explicit how custodianship issues, as well as permissions to approve the transfer of genetic material, are made, especially for institutions with a centralized repository. Unlike traditional natural history specimens within an institution, genetic samples might be part of a voucher specimen that was accessioned by another collection before the sample itself was deposited in the genetic collection.

Because genetic collections are consumptive, loan/gift policies should clearly outline the required information that should be submitted in sample requests to justify that a material transfer is warranted. The following information is recommended for inclusion in loan/gift requests:

Objectives of the proposed research and its scientific merit
Taxa and total number of genetic samples requested
Experimental protocol to be employed
Amount of genetic material requested per sample
Desired method of transport (e.g., room temperature in preservative, frozen on dry ice)
Plans for the dissemination of knowledge gained from the proposed research with the originating institution and scientific community, including:

- Publications resulting from use of the samples

- Online publication of sequence data

Loan/gift policies should also clearly state the allowable use of genetic samples and associated metadata. Policies should stipulate that loans/gifts may not be transferred from one institution to another without the written permission of the originating institution. This also ensures that those receiving samples do not patent or otherwise profit from the use of specimens (as outlined in the Convention on Biological Diversity). Researchers might also be obliged to acknowledge the institution in all publications resulting from use of their loan/ gift material and make available citations or reprints of such publications.

Loan/gift policies for genetic resources differ from those of other types of natural history specimens because genetic sequence data is generated from their consumptive use. The majority of genetic resource collections surveyed request that researchers submit genetic sequence data to a public genetic sequence database, such as NCBI GenBank (http://www.ncbi.nlm.nih.gov/)^[2]. This requirement is important for consumable collections because it ensures that sequence data is available to other researchers, unnecessary work is not duplicated, and originating institutions comply with granting agreements to make data accessible. Whenever possible, collections should link the end products of research (e.g., genetic sequences) captured in communal databases to the original genetic samples and/or voucher specimen records found in the originating institution’s database. To ensure compliance, it is recommended that collection managers should follow up with researchers annually and consider loans/gifts ‘‘closed’’ only when all policy requirements are met.

If the institution provides the appropriate amount of material, the genetic samples loaned/gifted should be completely consumed by the researcher (see USE OF COLLECTIONS: Aliquoting Samples). If a portion of a genetic sample remains unused after the project, however, researchers might be unclear about what to do with the remaining samples. In a recent collection survey, institutions requested that researchers address leftover samples in various ways, including destroying the remaining samples, returning samples to the originating institution for destruction or reuse, or accessioning samples into the researcher’s personal or institutional collection ^[2]. The loan/gift policy should clearly outline the requirements of researchers in regards to any unused genetic material. It is recommended that subsamples that are returned to loaning collections for potential future reuse be maintained separately from the original samples in case the returning sample’s integrity was compromised (e.g., contaminated, mislabeled, improperly stored) while on loan. The use history of each sample is important to track, especially for returned material, because this allows personnel to inventory and use only returned samples if all other portions have been consumed (see [[#Databasing for genetic samples|INVENTORY CONTROL AND DATA MANAGEMENT: Databasing for genetic samples). When returned samples are reused, tracking also allows collection manager to inform researchers of the chain of custody of the returned sample, so that future researchers can evaluate the risks of use of such samples.

Aliquoting samples

To maximize their use and research potential, genetic resources should not be sent in their entirety; rather genetic samples should be aliquoted for internal or external use (see USE OF COLLECTIONS: Loan policies). Regardless of the end user, subsampling methods should be employed that maximize collection utility by minimally handling samples, effectively removing the smallest sampling amount, and reducing freeze–thaw events while manipulating samples. Implementing efficient organizational methods, from storage containers to database management systems, minimizes the amount of time required to locate samples. At any one time, only a manageable number of samples should be retrieved, so that cold-storage units do not remain open and the time that storage containers are kept outside of these units is minimized. During the subsampling process, samples should be kept as close to their normal storage temperature as possible. Depending on the temperature from which the samples were taken, liquid nitrogen, dry ice, or wet ice can be used to help keep samples cold during processing.

The amount of a genetic sample provided to a researcher should be scaled to their individual request to ensure long-term availability of the original sample for other researchers. The SOP should provide baseline standards to guide the amount of genetic material sent as a loan/gift, including considerations for the type of preparation requested (e.g., tissue subsample, aliquot of extraction, PCR product) and the experimental protocol to be implemented. In a recent collection survey, collections were found to set these sampling criteria in various ways ^[2]. Over one-third of the surveyed collections provided the approximate amount of tissue needed for two to three DNA extractions; fewer collections quantified the amount of a sample sent (i.e., ranging from 1 mm² to 6 mm² in size, weighing from 10 mg to 2 g), likely because measuring or weighing individual samples is a time-consuming process that most collections cannot afford. Collection managers should also consider whether to extract DNA, rather than send tissue samples, especially when rare samples or those with low remaining volumes are requested. Regardless of the general criteria, personnel working with genetic samples should be knowledgeable of the sample amounts needed for methods commonly conducted (e.g., DNA extraction, RNA extraction, PCR, cloning).

Packaging and shipping loans/gifts

As with traditional natural history specimens, loan/gift shipments of genetic samples should include loan paperwork on institutional letterhead that documents the contents, handling requirements, and policies of use (see USE OF COLLECTIONS: Loan policies). Before any loans/gifts are processed, collection personnel must:

Determine all the national or international laws and regulations pertaining to the genetic samples and the shipment
Include copies of all permits and certificates with the shipment in a location that is easily accessible on the outside of the package
Include invoice that can be signed and returned by the researcher upon receipt of the samples
Determine if special permits or requirements are necessary, including:^[29]

- US Department of Agriculture (USDA)

- International Treaty on Plant Genetic Resources for Food and Agriculture (PGRFA)^[30]

- Convention on International Trade in Endangered Species of Wild Fauna and Flora (CITES)^[31] ^[32], and various US domestic laws, including the Endangered Species Act (ESA)^[33]

- Lacey Act^[33]

- Migratory Bird Treaty Act (MBTA)

As the legal landscape evolves, collection personnel must receive the appropriate training, with applicable updates, in both national and international regulations, including the shipment of biological samples and dangerous goods (e.g., DOT, International Air Transport Association [IATA] Special Provision A180), and the recent ratification of the Convention on Biological Diversity Nagoya Protocol on Access and Benefit-Sharing. See Shipping and Handling of Dangerous Goods for additional information.

Loans/gifts of genetic samples can be shipped using various methods and, depending on the sample type and ultimate use, material transfers might require special means of shipping to preserve specimen integrity and quality. Cold or frozen material should be shipped in a manner that will maintain the appropriate temperature for the duration of the shipment with allowance for delay in arrival time. Refrigerant should last an additional 24−72 hours, depending on whether the shipment is domestic or international, especially because customs will be involved for the latter^[17]. It is advised that refrigerated or frozen shipments are not sent on days that require transit over a weekend or holiday period, so as to avoid delays and ensure that recipients are available for immediate receipt of the samples. The coordination of shipping and receiving samples is important for all parties, so to avoid mishaps, both the shipper and recipient should track the package while in transit. Collection personnel should contact the recipient before sending the shipment to confirm that they are present to receive the package as scheduled and, again, contact the researcher to notify them when the shipment is specifically scheduled to arrive.

When packing, genetic samples should be positioned in the package so that they are surrounded by refrigerant on all sides, rather than having samples placed on top of or underneath refrigerant. Any empty space between samples and refrigerant should be filled with dunnage material (e.g., loosefill non-biodegradable peanuts, padding material). Specimens that are sensitive to humidity (e.g., botanical samples) should be shipped in sealed bags with desiccant to ensure that humidity levels are controlled in transit. The following are typical temperature conditions required for shipment of genetic samples, including the insulation and/or refrigerant that can be used to maintain the desired temperature (modified^[17]).

UN 1845 label for shipments including dry ice.

Ambient (20°–30°C): insulated packaging with a minimum of 4-cm-thick walls to protect from fluctuations in ambient temperature; chemical preservative might or might not be necessary, depending on sample type.
Refrigerated (2°–8°C): insulated packaging with a minimum of 4-cm-thick walls with wet ice or gel packs; chemical preservative might or might not be necessary, depending on sample type.
Frozen (-20°C): insulated packaging with a minimum of 4-cm-thick walls with gel packs designed for frozen temperatures.
Frozen (-70°C): insulated packaging with a minimum of 4-cm-thick walls with dry ice pellets, sheets, or blocks. Note: dry ice (solid CO₂) is considered a hazardous material.
Frozen (at or below -150°C): LN₂ dry shipper. Dry nitrogen shippers are insulated containers that contain LN₂ that is fully absorbed in a porous material within the walls and, therefore, considered a non-dangerous product by DOT and IATA regulations.

Recently surveyed genetic resource collections were found to most frequently ship samples frozen using dry ice, or at ambient temperature using ethanol or DMSO as a preservative.^[2] Shipping methods among collections likely differed due to overall cost, shipping restrictions, ease of shipment, and the intended use of the samples. With increasing regulations on shipments and shipping training for personnel, expenses have become prohibitive for many institutions and, as a result, many collections are either requesting or requiring that researchers offset the associated costs.

Health & Safety

Health and safety policies are essential because they protect personnel who are working with genetic resource collections, but these policies also ultimately protect the collection itself because they promote proper and efficient practices. All health and safety policies should be reviewed with the appropriate health and safety group at the institution and fully outlined in the SOP of the genetic collection.

General laboratory practices

Good laboratory practices should be implemented in genetic resource collections to protect staff from exposure to various hazards (e.g., potential pathogens, chemicals, sharps). For staff safety, certain activities should be prohibited in the laboratory or collection space, including:

Eating
Drinking
Storing food
Smoking
Applying cosmetics
Handling contact lenses
Mouth pipetting

For collections harvesting genetic samples from traditional voucher specimens, collection managers must ensure that any biosafety waste is processed in accordance with institutional regulations and any pertinent local, state, or national guidelines. Policies should be instituted for the safe handling and disposal of sharps (e.g., needles, razor blades, scalpels). Lastly, good laboratory practice includes washing hands at the end of preparation work, after gloves are removed, and prior to leaving the laboratory.

Personal protective equipment

All personnel, including visitors, should wear appropriate and approved clothing (e.g., buttoned lab coats, long pants, shoes that completely cover the feet) when working in a laboratory environment, such as a genetic collection.^[34] Shorts, skirts and open-toe shoes are not appropriate, especially in labs that require a Biosafety Level 2 designation. In addition, long hair and dangling jewelry should be secured. Depending on the laboratory application, personnel should wear the appropriate gloves; this includes latex or nitrile gloves when handling chemicals or biological samples, cryogenic gloves to protect against frostbite when working with ultracold equipment or samples, and heat-resistant gloves when using autoclaves or other equipment that reach high temperatures. Eyes should always be protected from exposure to chemicals and biohazards by using safety glasses, goggles or face shields; eye and face protection devices should comply with American National Standards Institute recommendations (i.e., ANSI Z87.1) when used with chemicals.

Liquid nitrogen safety

Cryogenic apron, cryogenic gloves and face shield. (Photograph by B. Zimkus.)

Those collections that use LN₂ storage equipment require additional safety precautions and equipment specifically rated for cryogenic conditions. Specialized ventilation and oxygen monitors might be needed to protect personnel from the risk of oxygen depletion and possible asphyxiation (see FACILITY MANAGEMENT: Ventilation; FACILITY MANAGEMENT: Oxygen monitors). When working with LN₂, appropriate PPE is recommended:

Cryogenic gloves, which are water-resistant insulated gloves rated for cryogenic temperatures, to protect the hands from cold temperatures and nitrogen vapor
Cryogenic aprons to protect the body when using the liquid phase of nitrogen
Eye protection (e.g., safety glasses) when working with samples that have been stored in the liquid phase of nitrogen because sample vials can burst without warning if LN₂ enters them through minute cracks
Goggles and/or a face shield when dispensing LN₂ to additionally protect the face and eyes from possible splashing
Closed-toe shoes (not canvas) that can be quickly removed (e.g., few laces, buckles, zippers)
Lab coats
Pants without cuffs; pants should not be tucked into shoes or boots because LN₂ can become trapped if spilled

If nitrogen in the liquid form contacts the skin or eyes, the tissue should be immediately flooded or soaked with tepid or warm water (105°F –115°F [41°C–46°C]). Hot water (above 46°C) should never be used because this can cause additional damage to the skin. In addition, the skin must not be rubbed because this can damage the tissue; thus, any contact should involve only gentle patting or dabbing. If LN₂ comes in contact with the eyes, contact lenses should be removed immediately and the eyes flushed with tepid or warm water for at least 15 minutes, and the upper and lower eyelids should be lifted occasionally during the flushing process. If any injury occurs from a cryogenic burn, medical attention should be sought as soon as possible.

Cryogenic fluids must be handled and stored only in containers specifically designed for these products. Unapproved materials can become brittle and shatter or become over-pressurized, causing risks of explosion. All cryogenic vessels must be equipped with pressure-relief devices (e.g., relief valve, venting lid/stopper) to prevent excessive pressure build-up. A tremendous amount of force can be generated if liquid nitrogen rapidly vaporizes, so pressure-relief devices on LN₂ equipment should be monitored to ensure that they are functioning properly. Transfer operations involving open cryogenic containers, such as dewars, should be conducted slowly to minimize boiling, splashing, and thermal shock to the receiving vessel. A phase separator (i.e., fitting that attaches to end of a transfer hose that separates gas from liquid)can also be used to control the vapor path while dispensing. When dispensing or pouring LN₂, receiving vessels should be placed as close as possible to the source; a table or other sturdy surface can be used to position the vessel in the proper location. Funnels should not be used to channel LN₂ because they can freeze, creating a splash hazard, or be propelled upwards if the container is overfilled.

Dry ice safety

Use of dry ice (i.e., solid phase of CO₂) is regulated and requires specialized training for use in shipments. When dry ice is used, collection managers should ensure that there is adequate ventilation because CO₂ can displace oxygen, causing loss of consciousness or even asphyxiation. All confined areas should be closely monitored when dry ice is in use. Walk-in freezers should be kept free of dry ice because carbon dioxide can rapidly build up without regular air exchange; owing to this inherent danger, proper signage should be posted outside walk-in freezers to prevent staff from placing dry ice into walk-in freezers.

Biosafety

Collection managers should consult all federal biosafety and biocontainment regulations relevant to the activities conducted that involve potentially hazardous biological materials within the collection. Policies should incorporate all regulations hat outline standard and special practices, safety equipment, and facility requirements to minimize potential hazards to laboratory personnel and the environment. USDA permits could be needed for work with some specific taxa, such as birds, some mammals, and plants. Depending on the biosafety level required for the collection as determined by the USDA, certain requirements might need to be met, including:

Training in handling pathogenic agents
Restrictions to collection access when work is being conducted
Conduction of particular work in a biological safety cabinet

A biosafety cabinet (BSC), also known as a biological or microbiological safety cabinet, is an enclosed, ventilated workspace for handling materials potentially contaminated with pathogens (e.g., Exotic Newcastle Disease, Foot-and-Mouth Disease, Hantavirus, Highly Pathogenic Avian Influenza). BSCs differ from fume hoods because BSC exhaust air is HEPA-filtered as it exits. BSCs are classified as one of three classes by their level of protection provided to personnel and the environment (i.e., Class I, II, III). Class II Type A2 BSC, which includes a minimum inflow velocity of 100 ft/min (30.5 m/min), is the most commonly used BSC providing protection for personnel, the environment, and the samples. Collection managers should be aware that gas lines should not be installed into BSCs because air is contained within, rather than being exhausted from the cabinet, leading to the potential build up of flammable materials. Additionally, open flames, such as those generated by Bunsen burners, can detrimentally affect airflow in a BSC, disrupting the pattern of HEPA-filtered air supplied to the work surface. To provide adequate protection, BSCs require proper use, monitoring, and regular maintenance. SOP documents must outline these approved activities, including appropriate height of the sash opening to minimize airflow, methods used to decontaminate surfaces, as well as testing and certification protocols for the unit itself (see OPERATIONAL BEST PRACTICE: Equipment preventative maintenance, repair, and replacement).

Chemical safety

Genetic resource collections should maintain an inventory of all chemicals used and access to Safety Data Sheets (SDS) for every chemical used within the collection. A chemical hygiene plan should also be included in SOP documents, which outlines the appropriate use of chemicals in the collection, as well as their containment and procedures for clean-up if spills occur. Personnel should have the appropriate training for all procedures related to chemical safety, which frequently involves training by institutional groups, such as health and safety and the fire group (see OPERATIONAL BEST PRACTICE: Training).

Fire safety

Collection personnel must comply with all local fire and building codes. Automatic fire detection units and suppression systems, including appropriate hand-held fire extinguishers and sprinkler systems, are recommended. The SOP should include information regarding major fire hazards and potential ignition sources, as well as what working materials are flammable hazards (e.g., ethanol). Personnel should be trained in fire prevention and emergency procedures relating to evacuation if a fire occurs (see OPERATIONAL BEST PRACTICE: Training). All fire detection systems and suppression systems should be tested on a regular basis and frequently involve health and safety, fire, and building facility personnel at the institution (see OPERATIONAL BEST PRACTICE: Equipment preventative maintenance, repair, and replacement).

Ethical and Legal Best Practice

The accumulation and use of genetic samples involve numerous ethical and legal issues. Most natural history museums have institutional policies that address legal compliance and ethical standards, but many times, genetic samples are present in individual laboratories or stand-alone collections whose activities might not be specifically addressed in the broader institutional policies. In these instances, dedicated policies might not be in place to govern broad aspects of legal and ethical issues associated with the initial collection, transport, and use of genetic samples. Genetic resource collections are subject to the same regulations, laws, and consequences as traditional natural history collections. As such, they must have accessioning practices that ensure and document that all samples are legally collected, transported, and acquired by the collection. Copies of all necessary permits, including collecting permits, relevant Material Transfer Agreements, export permits from the country of origin, and import permits into the country of the genetic collection, must be on file within the institution or genetic resource collection. The accession process should also ensure and document that all animals collected were done so in a manner consistent with pertinent guidelines, such as Institutional Animal Care and Use Committee (IACUC) regulations.

Unlike most traditional natural history collections, genetic resource collections make samples available to researchers for molecular analyses with the understanding that derivatives and even possible genetic modifications of the original sample will be produced. It is a legal responsibility that collections personnel, therefore, act as custodians to ensure that genetic samples are used in accordance with all laws and governing policies,including the original collecting or acquisition agreements and pertinent international conventions^[35] ^[33]. Collection managers should be aware that countries or other governing entities might have restrictions in relation to the commercial use of genetic samples, whereas educational or research use is permitted. In addition, entities that retain ownership (e.g., US National Park Service) can have specific regulations in relation to exportation, importation, or use of samples.

To document compliance and provide responsible stewardship for consumptive genetic resources, collection personnel should track the use history of all genetic samples and their derivatives, and link this information to the available metadata (e.g., NCBI GenBank; see INVENTORY CONTROL AND DATA MANAGEMENT: Databasing for genetic samples). Loan/gift policy must, therefore, be explicit in the approved uses of genetic samples and associated metadata, as well as expectations for what the researcher should do with any samples remaining after the completion of the research (see USE OF COLLECTIONS: Loan policies). Policy should also clearly outline requirements resulting from use of the genetic material. Research users and collection managers should both make a dedicated effort to ensure that collections are formally acknowledged for use of their samples and collections are notified of published studies that result from the use of their material. Knowledge of sample use is ital to genetic resource collections, because they must justify their significance in research to both their institution and outside funding bodies. Lastly, copyright and intellectual property rights in relation to genetic sample metadata provided to researchers or presented on public websites should be accompanied by policy that outlines the terms and conditions of its use, including the requirements to share results from the research.

Source Material

Zimkus, B.M. and L.S. Ford. 2014. Best Practices for Genetic Resources Associated with Natural History Collections Recommendations for Practical Implementation. Collection Forum 28(1-2), pp. 77-112.

Links

References

↑ Wieczorek, J., D. Bloom, R. Guralnick, S. Blum, M. Doring, R. Gionvanni, T. Robertson, and D. Vieglais. 2012. Darwin core: An evolving community-developed biodiversity data standard. PLoS ONE 7(1): e29715.
↑ ^2.00 ^2.01 ^2.02 ^2.03 ^2.04 ^2.05 ^2.06 ^2.07 ^2.08 ^2.09 ^2.10 ^2.11 ^2.12 ^2.13 ^2.14 ^2.15 ^2.16 ^2.17 ^2.18 ^2.19 ^2.20 ^2.21 ^2.22 Zimkus, B.M. and L.S. Ford. 2014. Genetic resource collections associated with natural history museums: A survey and analysis to establish a benchmark of standards. Pp. 9–44 in DNA Banking for the 21st Century. Proceedings of the U.S. Workshop on DNA Banking (W.L. Applequist and L. Campbell, eds.). William L. Brown Center, St. Louis, Missouri. 187 pp.
↑ Savolainen, V., M.P. Powell, K. Davies, A. Corthals, and G. Reeves (eds). 2006. DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice and Uses. Kew Publishing, Royal Botanic Garden, Kew, England. 151 pp.
↑ Hanner, R., A. Corthals, and H.C. Dessauer. 2005. Salvage of genetically valuable tissues following a freezer failure. Molecular Phylogenetics and Evolution 34:452–455.
↑ International Society for Biological and Environmental Repositories. 2012. 2012 Best practices for repositories: Collection, storage, retrieval, and distribution of biological materials for research. Biopreservation and Biobanking 10:79–161.
↑ Engstrom, M.D., R.W. Murphy, and O. Haddrath. 1990. Sampling vertebrate collections for molecular research: Practice and policies. Pp. 315–330 in Managing the Modern Herbarium (D.A. Metsger and S.C. Byers, eds.). Granville Island Publising, Vancouver, Canada. 384 pp.
↑ Karlsson, J.O. and M. Toner. 1996. Long-term storage of tissues by cryopreservation: Critical issues. Biomaterials 17:243–256.
↑ Kilpatrick, C.W. 2002. Noncryogenic preservation of mammalian tissues for DNA extraction: An assessment of storage methods. Biochemical Genetics 40:53–62.
↑ Mutter, G.L., D. Zahrieh, C. Liu, D. Neuberg, D. Finkelstein, H.E. Baker, and J.A. Warrington. 2004. Comparison of frozen and RNALater solid tissue storage methods for use in RNA expression microarrays. BMC Genomics 5:88.
↑ Corthals, A. and R. DeSalle. 2005. An application of tissue and DNA banking for genomics and conservation: The Ambrose Monell Cryo-Collection (AMCC). Systematic Biology 54:819–823.
↑ Gemeinholzer, B., I. Rey, K. Weising, M. Grundmann, A.N. Müllner, H. Zetsche, G. Droege, O. Seberg, G. Petersen, D.M. Rawson, and L.A. Weigt. 2010. Chapter 7—Organizing specimen and tissue preservation techniques in the field for subsequent molecular analyses. Pp. 129–157 in Manual on Field Recording Techniques and Protocols for All Taxa Biodiversity Inventories (J. Eymann, J. Degreef, C. Ha¨ user, J.C. Monje, Y. Samyn, and D. VandenSpiegel, eds.). Belgian National Focal Point to the Global Taxonomy Initiative, Brussels, Belgium. 653 pp.
↑ Nagy, Z.T. 2010. A hands-on overview of tissue preservation methods for molecular genetic analyses. Organisms Diversity & Evolution 10:91–105.
↑ Buś, M. and M. Allen. 2014. Collecting and preserving biological samples from challenging environments for DNA analysis. Biopreservation and Biobanking 12:17–22.
↑ Clark, G.N. 1999. Sperm cryopreservation: Is there a significant risk of cross-contamination. Human Reproduction 14:2941–2943.
↑ Hanner, R., A. Corthals, and H.C. Dessauer. 2005. Salvage of genetically valuable tissues following a freezer failure. Molecular Phylogenetics and Evolution 34:452–455.
↑ Savolainen, V., M.P. Powell, K. Davies, A. Corthals, and G. Reeves (eds). 2006. DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice and Uses. Kew Publishing, Royal Botanic Garden, Kew, England. 151 pp.
↑ ^17.0 ^17.1 ^17.2 [ISBER] International Society for Biological and Environmental Repositories. 2012. 2012 Best practices for repositories: Collection, storage, retrieval, and distribution of biological materials for research. Biopreservation and Biobanking 10:79–161.
↑ [ICOM] International Council of Museums. 1993. Guidelines for Disaster Preparedness in Museums. http://icom.museum/fileadmin/user_upload/pdf/Guidelines/guidelinesdisasters_eng.pdf (1 January 2014). (Off-print from Museums Security and Protection: A Handbook for Cultural Heritage Institutions [D. Listen, ed.] ICOM in conjunction with Routledge, London, New York. 319 pp.)
↑ Dorge, V. and S.L. Jones. 1999. Building an Emergency Plan: A Guide for Museums and Other Cultural Institutions. Getty Conservation Institute, Los Angeles. 272 pp.
↑ ^20.0 ^20.1 ^20.2 Nagy, Z.T. 2010. A hands-on overview of tissue preservation methods for molecular genetic analyses. Organisms Diversity & Evolution 10:91–105.
↑ Adams, G. 2007. The principles of freeze-drying. Methods in Molecular Biology 368:15–38.
↑ Chase, M.W. and H.G. Hills. 1991. Silica gel: An ideal material for field preservation of leaf samples for DNA studies. Taxon 40:215–220.
↑ Nagy, Z.T. 2010. A hands-on overview of tissue preservation methods for molecular genetic analyses. Organisms Diversity & Evolution 10:91–105.
↑ Corthals, A. 2006. The Ambrose Monell Cryo-Collection: A museum-based molecular collection. Pp. 107–113 in DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice and Uses (V. Savolainen, M.P. Powell, K. Davis, G. Reeves, and A. Corthals, eds.). Kew Publishing, Royal Botanic Garden, Kew,England. 151 pp.
↑ Corthals, A. and R. DeSalle. 2005. An application of tissue and DNA banking for genomics and conservation: The Ambrose Monell Cryo-Collection (AMCC). Systematic Biology 54:819–823.
↑ Johnson, B. 1999. Frozen in time: Ultra low freezers, dewars, and tubes. The Scientist 13(1):19.
↑ Cable, S. and T.K. Fulcher. 2006. Databasing and information technology. Pp. 61–65 in DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice and Uses (V. Savolainen, M.P. Powell, K. Davis, G. Reeves, and A. Corthals, eds.). Kew Publishing, Royal Botanic Garden, Kew, England. 151 pp.
↑ Coddington, J., K. Barker, G. Droege, J.J. Astrin, P. Bartels, C. Butler, D. Cantrill, F. Forest, B. Gemeinholzer, D. Hobern, J. Mackenzie-Dodds, E.O. Tuama, G. Petersen, O. Sanjur, D. Schindel, and O. Seberg. 2014. GGBN: Making genomic collections discoverable for research through a networked community of biodiversity repositories. Pp. 165–168 in DNA Banking for the 21st Century. Proceedings of the U.S. Workshop on DNA Banking (W.L. Applequist and L. Campbell, eds.). William L. Brown Center, St. Louis, Missouri. 187 pp.
↑ Renner, S.C., D. Neumann, M. Burkart, U. Feit, P. Giere, A. Gröger, A. Paulsch, C. Paulsch, M. Sterz and K. Vohland. 2012. Import and export of biological samples from tropical countries — Considerations and guidelines for research teams. Organisms Diversity & Evolution 12:81–98.
↑ Moore, G.K. and W. Tymowski. 2005. Explanatory guide to the International Treaty on Plant Genetic Resources for Food and Agriculture. IUCN Environmental Policy and Law Paper No. 57. IUCN, Gland, Switzerland. 212 pp.
↑ Davis, K., C. Williams, M. Wolfson, and J. Donaldson. 2006. Practical implementation of the CBD and CITES. Pp. 36–46 in DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice and Uses (V. Savolainen, M.P. Powell, K. Davis, G. Reeves,and A. Corthals, eds.). Kew Publishing, Royal Botanic Garden, Kew, England. 151 pp.
↑ Donaldson, J. 2006. CITES and DNA banking. Pp. 30–35 in DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice and Uses (V. Savolainen, M.P. Powell, K. Davis, G. Reeves, and A. Corthals, eds.). Kew Publishing, Royal Botanic Garden, Kew, England. 151 pp.
↑ ^33.0 ^33.1 ^33.2 Applequist, W. 2014. Legal and ethical issues related to DNA banking. Pp. 137–146 in DNA Banking for the 21st Century. Proceedings of the U.S. Workshop on DNA Banking (W.L. Applequist and L. Campbell, eds.). William L. Brown Center, St. Louis, Missouri. 187 pp.
↑ Kapinos, E. and S. Graham. 2006. DNA banking and health, safety and security. Pp. 52–60 in DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice and Uses (V. Savolainen, M.P. Powell, K. Davis, G. Reeves, and A. Corthals, eds.). Kew Publishing, Royal Botanic Garden, Kew, England. 151 pp.
↑ Secretariat of the Convention on Biological Diversity. 2011. Nagoya Protocol on Access to Genetic Resources and the Fair and Equitable Sharing of Benefits Arising from Their Utilization to the Convention on Biological Diversity. Secretariat of the Convention on Biological Diversity, Montreal, Canada. 25 pp. http://www.cbd.int/abs/doc/protocol/nagoya-protocol-en.pdf (1 November 2014).

[1] Wieczorek, J., D. Bloom, R. Guralnick, S. Blum, M. Doring, R. Gionvanni, T. Robertson, and D. Vieglais. 2012. Darwin core: An evolving community-developed biodiversity data standard. PLoS ONE 7(1): e29715.

[ZimkusFord2014-2] 2.00 ^2.01 ^2.02 ^2.03 ^2.04 ^2.05 ^2.06 ^2.07 ^2.08 ^2.09 ^2.10 ^2.11 ^2.12 ^2.13 ^2.14 ^2.15 ^2.16 ^2.17 ^2.18 ^2.19 ^2.20 ^2.21 ^2.22 Zimkus, B.M. and L.S. Ford. 2014. Genetic resource collections associated with natural history museums: A survey and analysis to establish a benchmark of standards. Pp. 9–44 in DNA Banking for the 21st Century. Proceedings of the U.S. Workshop on DNA Banking (W.L. Applequist and L. Campbell, eds.). William L. Brown Center, St. Louis, Missouri. 187 pp.

[3] Savolainen, V., M.P. Powell, K. Davies, A. Corthals, and G. Reeves (eds). 2006. DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice and Uses. Kew Publishing, Royal Botanic Garden, Kew, England. 151 pp.

[4] Hanner, R., A. Corthals, and H.C. Dessauer. 2005. Salvage of genetically valuable tissues following a freezer failure. Molecular Phylogenetics and Evolution 34:452–455.

[5] International Society for Biological and Environmental Repositories. 2012. 2012 Best practices for repositories: Collection, storage, retrieval, and distribution of biological materials for research. Biopreservation and Biobanking 10:79–161.

[6] Engstrom, M.D., R.W. Murphy, and O. Haddrath. 1990. Sampling vertebrate collections for molecular research: Practice and policies. Pp. 315–330 in Managing the Modern Herbarium (D.A. Metsger and S.C. Byers, eds.). Granville Island Publising, Vancouver, Canada. 384 pp.

[7] Karlsson, J.O. and M. Toner. 1996. Long-term storage of tissues by cryopreservation: Critical issues. Biomaterials 17:243–256.

[8] Kilpatrick, C.W. 2002. Noncryogenic preservation of mammalian tissues for DNA extraction: An assessment of storage methods. Biochemical Genetics 40:53–62.

[9] Mutter, G.L., D. Zahrieh, C. Liu, D. Neuberg, D. Finkelstein, H.E. Baker, and J.A. Warrington. 2004. Comparison of frozen and RNALater solid tissue storage methods for use in RNA expression microarrays. BMC Genomics 5:88.

[10] Corthals, A. and R. DeSalle. 2005. An application of tissue and DNA banking for genomics and conservation: The Ambrose Monell Cryo-Collection (AMCC). Systematic Biology 54:819–823.

[11] Gemeinholzer, B., I. Rey, K. Weising, M. Grundmann, A.N. Müllner, H. Zetsche, G. Droege, O. Seberg, G. Petersen, D.M. Rawson, and L.A. Weigt. 2010. Chapter 7—Organizing specimen and tissue preservation techniques in the field for subsequent molecular analyses. Pp. 129–157 in Manual on Field Recording Techniques and Protocols for All Taxa Biodiversity Inventories (J. Eymann, J. Degreef, C. Ha¨ user, J.C. Monje, Y. Samyn, and D. VandenSpiegel, eds.). Belgian National Focal Point to the Global Taxonomy Initiative, Brussels, Belgium. 653 pp.

[12] Nagy, Z.T. 2010. A hands-on overview of tissue preservation methods for molecular genetic analyses. Organisms Diversity & Evolution 10:91–105.

[13] Buś, M. and M. Allen. 2014. Collecting and preserving biological samples from challenging environments for DNA analysis. Biopreservation and Biobanking 12:17–22.

[14] Clark, G.N. 1999. Sperm cryopreservation: Is there a significant risk of cross-contamination. Human Reproduction 14:2941–2943.

[15] Hanner, R., A. Corthals, and H.C. Dessauer. 2005. Salvage of genetically valuable tissues following a freezer failure. Molecular Phylogenetics and Evolution 34:452–455.

[16] Savolainen, V., M.P. Powell, K. Davies, A. Corthals, and G. Reeves (eds). 2006. DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice and Uses. Kew Publishing, Royal Botanic Garden, Kew, England. 151 pp.

[ISBER-17] 17.0 ^17.1 ^17.2 [ISBER] International Society for Biological and Environmental Repositories. 2012. 2012 Best practices for repositories: Collection, storage, retrieval, and distribution of biological materials for research. Biopreservation and Biobanking 10:79–161.

[18] [ICOM] International Council of Museums. 1993. Guidelines for Disaster Preparedness in Museums. http://icom.museum/fileadmin/user_upload/pdf/Guidelines/guidelinesdisasters_eng.pdf (1 January 2014). (Off-print from Museums Security and Protection: A Handbook for Cultural Heritage Institutions [D. Listen, ed.] ICOM in conjunction with Routledge, London, New York. 319 pp.)

[19] Dorge, V. and S.L. Jones. 1999. Building an Emergency Plan: A Guide for Museums and Other Cultural Institutions. Getty Conservation Institute, Los Angeles. 272 pp.

[Nagy2010-20] 20.0 ^20.1 ^20.2 Nagy, Z.T. 2010. A hands-on overview of tissue preservation methods for molecular genetic analyses. Organisms Diversity & Evolution 10:91–105.

[21] Adams, G. 2007. The principles of freeze-drying. Methods in Molecular Biology 368:15–38.

[22] Chase, M.W. and H.G. Hills. 1991. Silica gel: An ideal material for field preservation of leaf samples for DNA studies. Taxon 40:215–220.

[23] Nagy, Z.T. 2010. A hands-on overview of tissue preservation methods for molecular genetic analyses. Organisms Diversity & Evolution 10:91–105.

[24] Corthals, A. 2006. The Ambrose Monell Cryo-Collection: A museum-based molecular collection. Pp. 107–113 in DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice and Uses (V. Savolainen, M.P. Powell, K. Davis, G. Reeves, and A. Corthals, eds.). Kew Publishing, Royal Botanic Garden, Kew,England. 151 pp.

[25] Corthals, A. and R. DeSalle. 2005. An application of tissue and DNA banking for genomics and conservation: The Ambrose Monell Cryo-Collection (AMCC). Systematic Biology 54:819–823.

[26] Johnson, B. 1999. Frozen in time: Ultra low freezers, dewars, and tubes. The Scientist 13(1):19.

[27] Cable, S. and T.K. Fulcher. 2006. Databasing and information technology. Pp. 61–65 in DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice and Uses (V. Savolainen, M.P. Powell, K. Davis, G. Reeves, and A. Corthals, eds.). Kew Publishing, Royal Botanic Garden, Kew, England. 151 pp.

[28] Coddington, J., K. Barker, G. Droege, J.J. Astrin, P. Bartels, C. Butler, D. Cantrill, F. Forest, B. Gemeinholzer, D. Hobern, J. Mackenzie-Dodds, E.O. Tuama, G. Petersen, O. Sanjur, D. Schindel, and O. Seberg. 2014. GGBN: Making genomic collections discoverable for research through a networked community of biodiversity repositories. Pp. 165–168 in DNA Banking for the 21st Century. Proceedings of the U.S. Workshop on DNA Banking (W.L. Applequist and L. Campbell, eds.). William L. Brown Center, St. Louis, Missouri. 187 pp.

[29] Renner, S.C., D. Neumann, M. Burkart, U. Feit, P. Giere, A. Gröger, A. Paulsch, C. Paulsch, M. Sterz and K. Vohland. 2012. Import and export of biological samples from tropical countries — Considerations and guidelines for research teams. Organisms Diversity & Evolution 12:81–98.

[30] Moore, G.K. and W. Tymowski. 2005. Explanatory guide to the International Treaty on Plant Genetic Resources for Food and Agriculture. IUCN Environmental Policy and Law Paper No. 57. IUCN, Gland, Switzerland. 212 pp.

[31] Davis, K., C. Williams, M. Wolfson, and J. Donaldson. 2006. Practical implementation of the CBD and CITES. Pp. 36–46 in DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice and Uses (V. Savolainen, M.P. Powell, K. Davis, G. Reeves,and A. Corthals, eds.). Kew Publishing, Royal Botanic Garden, Kew, England. 151 pp.

[32] Donaldson, J. 2006. CITES and DNA banking. Pp. 30–35 in DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice and Uses (V. Savolainen, M.P. Powell, K. Davis, G. Reeves, and A. Corthals, eds.). Kew Publishing, Royal Botanic Garden, Kew, England. 151 pp.

[Applequist-33] 33.0 ^33.1 ^33.2 Applequist, W. 2014. Legal and ethical issues related to DNA banking. Pp. 137–146 in DNA Banking for the 21st Century. Proceedings of the U.S. Workshop on DNA Banking (W.L. Applequist and L. Campbell, eds.). William L. Brown Center, St. Louis, Missouri. 187 pp.

[34] Kapinos, E. and S. Graham. 2006. DNA banking and health, safety and security. Pp. 52–60 in DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice and Uses (V. Savolainen, M.P. Powell, K. Davis, G. Reeves, and A. Corthals, eds.). Kew Publishing, Royal Botanic Garden, Kew, England. 151 pp.

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@@ Line 1: / Line 1: @@
 == Statement of Purpose ==
-Researchers  associated  with  natural history museums have made the collection of genetic resources a priority due to  their  importance in molecular  studies, but often the long-term curation  of these collections is difficult due to decentralized curation over multiple storage locations and lack of community best practice guidelines for their stewardship. Unlike traditional natural history specimens, the research utility of genetic samples increases with lower storage temperatures and fewer freeze–thaw events and, in addition, their use is consumptive. Collection managers must, therefore, maximize the research potential of each sample by carefully considering use on a case-by-case basis. This page presents standardized guidelines for the management of genetic collections associated with natural history collections. These recommended  practices are informed  by general  standards for biorepositories and augmented by information unique to natural history collections with the goal of providing a foundation for those curating genetic samples. Information pertains  to all aspects of genetic sample curation and will assist those in making decisions regarding how to collect, store, track, process, and distribute  genetic specimen samples. These guidelines also will allow users to make informed decisions regarding how to apply and improve the curation of their collection given their institution’s goals and available resources.
+This page presents standardized guidelines for the management of genetic collections associated with natural history collections. For information on procedures related to the collection of tissues, see [[Tissue Sample Collection]]. These recommended  practices are informed  by general  standards for biorepositories and augmented by information unique to natural history collections with the goal of providing a foundation for those curating genetic samples. Information pertains to all aspects of genetic sample curation and will assist those in making decisions regarding how to collect, store, track, process, and distribute  genetic specimen samples. These guidelines provide an organized method to evaluate the relative costs and benefits of various strategies and to prioritize potential improvements and minimize risks to genetic collections, which is applicable to both enhancing a single existing collection, as well as those forming a centralized repository composed of samples from multiple independent collections.
+==Contributors==
+[[User:BredaZimkus|Breda Zimkus]], Linda S. Ford
 ==Introduction==
+Researchers  associated  with  natural history museums have made the collection of genetic resources a priority due to  their  importance in molecular  studies, but often the long-term curation  of these collections is difficult due to decentralized curation over multiple storage locations and lack of community best practice guidelines for their stewardship. Unlike traditional natural history specimens, the research utility of genetic samples increases with lower storage temperatures and fewer freeze–thaw events and, in addition, their use is consumptive. Collection managers must, therefore, maximize the research potential of each sample by carefully considering use on a case-by-case basis. In addition, collection personnel must always balance institutional goals with the curation needs of their respective collections. Therefore, these recommendations can be broadly or narrowly applied, depending on the mission of the institution and other factors that influence the curation of genetic samples, including budget, staffing, and space.
 ==Developing Policies==
-Many natural history collections have institutional guidelines that outline how traditional specimens should be curated,  but these guidelines generally are not specific enough to address the special curation needs of genetic samples. To ensure that genetic samples are curated consistently for long-term preservation and use, all genetic repositories should develop the following:
+Many natural history collections have institutional guidelines that outline how traditional specimens should be curated, but these guidelines generally are not specific enough to address the special curation needs of genetic samples. To ensure that genetic samples are curated consistently for long-term preservation and use, all genetic repositories should develop the following:
-# Dedicated written policies
 # Standard Operating Procedures (SOPs)
 # Comprehensive guide to operations
+Policies and procedures should be written by those with experience in the management of the genetic collection and should comply with all governmental and regulatory requirements. All personnel should be trained using these written guidelines to ensure accuracy and consistency of procedures when working in the repository.
-==== Policy ====
-Policy should govern all aspects of the use and storage of materials housed in the collection, including:
-* Acquisitions - Collection managers should ensure that all genetic samples, even those without associated traditional voucher specimens, were acquired and transported legally
-* Accessions
-* Cataloging procedures
-* Active care and use (i.e., loan, gift,  material transfer) of the genetic samples
-* Curation activities resulting from the near-exhaustive or exhaustive use of genetic samples (e.g., subsampling, deaccessioning)
-* Storage and organization of all relevant permits and acquisition documents
-* Minimal requirements for associated data associated (e.g., submission method, acceptable formats, Darwin Core standards)<ref>Wieczorek, J., D. Bloom, R. Guralnick, S. Blum, M. Doring, R. Gionvanni, T. Robertson, and D. Vieglais. 2012. Darwin  core: An evolving community-developed biodiversity data standard. PLoS ONE 7(1): e29715. </ref>
-* Loans/gifts - including the requirements for requesting genetic samples, internal procedures associated with the approval or authorization of loans/gifts, and an explanation of any fees associated with material transfers.
-<br>
 ==== Standard Operating Procedures (SOPs) ====
@@ Line 26: / Line 18: @@
 * Tasks performed by the personnel of the repository
 * Scope of activities performed
-* How the collection satisfies the mission and goals of the institution.
+* How the collection satisfies the mission and goals of the institution
 * Access to the collection
 * Equipment and tools present
+* Acquisitions
+* Accessions
+* Cataloging procedures
+* Curation activities resulting from the near-exhaustive or exhaustive use of genetic samples (e.g., subsampling, deaccessioning)
+* Storage and organization of relevant permits and acquisition documents
+* Specific requirements for acceptance of genetic samples, including:
+::- Provisions regarding acceptable sample types
+::- Preservation methods
+::- Storage containers
+::- Sample organization (e.g., sample vials arranged numerically, data and vials submitted concurrently)
+* Minimal requirements for associated data associated (e.g., submission method, acceptable formats, Darwin Core standards)<ref>Wieczorek, J., D. Bloom, R. Guralnick, S. Blum, M. Doring, R. Gionvanni, T. Robertson, and D. Vieglais. 2012. Darwin  core: An evolving community-developed biodiversity data standard. PLoS ONE 7(1): e29715. </ref>
+* Loans/gifts (e.g., requirements for requesting genetic samples, procedures associated with the approval, explanation of fees)
 * Information technology needs
 * Mandatory training for personnel
 * Health and safety programs
-* Personal protective equipment (PPE) required,
+* Personal protective equipment (PPE) required
 * Equipment monitoring
 * Maintenance activities
 * Backup precautions
 * Emergency procedures
-* Specific requirements for acceptance of genetic samples including:
+* Contact order for personnel in case of operational questions or emergencies<br>
-::provisions regarding acceptable sample types
-::preservation methods
-::storage containers
-::sample organization (e.g., sample vials arranged numerically, data and vials submitted concurrently)
-* Contact order for personnel in case of operational questions or emergencies (this information should also be clearly posted in the collection)
-<br>
 ==== Guide to operations ====
-A more comprehensive guide to operations should detail complete day-to-day collection procedures including:
+A more comprehensive guide to operations should detail complete day-to-day collection procedures, including:
 * Specimen processing (e.g., accessioning, cataloging, sample transfer, sample labeling, sample tracking)
 * Temporary and long-term sample storage criteria
@@ Line 54: / Line 52: @@
 * Shipment of loans/gifts
 * Disposal of waste (including biohazards)
-Policies and procedures should be written by those with experience in the management of the genetic collection and should comply with all governmental and regulatory  requirements. All personnel should be trained using these written guidelines to ensure accuracy and consistency of procedures when working in the repository.
 ==Funding and Budgets==
-The current  and future potential  of a collection for researchers  conducting  molecular studies is highly impacted by the efficient monitoring and storage of the genetic samples. A malfunction  in simple equipment,  such as a freezer, can render  a genetic or genomic collection  useless. To  fulfill their  research  mission  and  ensure  the  long-term conservation of genetic collections, repositories  must function efficiently, which requires dedicated   and   consistent   funding.
+The current  and future potential of a collection for researchers  conducting  molecular studies is highly impacted by the efficient monitoring and storage of the genetic samples. To  fulfill their research mission and ensure the  long-term conservation of genetic collections, repositories must function efficiently, which requires dedicated and consistent funding. For those collections that  are not centralized, the cost of curating genetic samples is often included in the overall budget for the institution or department, or funds come from personal research budgets <ref name=ZimkusFord2014>Zimkus,  B.M.  and  L.S. Ford.  2014. Genetic  resource  collections  associated  with natural  history  museums:  A survey and analysis to establish a benchmark of standards. Pp. 9–44 in DNA Banking for the 21st  Century. Proceedings of the U.S. Workshop on DNA Banking (W.L. Applequist  and L. Campbell,  eds.). William L. Brown Center,  St. Louis, Missouri.  187 pp.</ref>. Comprehensive and detailed budgets allow institutions to:
-* The   successful   operation  of   genetic   resource collections  is complex,  and  detailed  budgets  are  needed  to  ensure  that  support  from internal  and  external  sources  is sufficient  to  offset  operational costs.
+* Ensure that support from internal and external sources is sufficient to offset operational costs
-* Comprehensive budgets  allow institutions to track  spending  associated  with curating  genetic resources so  that   they  understand  the  costs  of  maintaining   their  collections  and  can  make informed  decisions.
+* Understand the costs of maintaining their collections
-* For  those  collections that  are not  centralized,  the cost of curating genetic samples is often included in the overall budget for the institution or department, or  funds  come from  personal  research  budgets <ref name=ZimkusFord2014>Zimkus,  B.M.  and  L.S. Ford.  2014. Genetic  resource  collections  associated  with natural  history  museums:  A survey and analysis to establish a benchmark of standards. Pp. 9–44 in DNA Banking for the 21st  Century. Proceedings of the U.S. Workshop on DNA Banking (W.L. Applequist  and L. Campbell,  eds.). William L. Brown Center,  St. Louis, Missouri.  187 pp.</ref>.
+* Make informed decisions regarding operations
 ==Facility Management==
@@ Line 67: / Line 63: @@
 <br>
 ===Access and security===
-Genetic  samples  have  significant  inherent  value  to  research because they are often collected from remote locations as a result of costly and time-consuming collection trips. Samples should, therefore, be stored in secure locations to minimize misplacement or inadvertent loss, and their access and use should be limited to those with the appropriate training.  A risk assessment should be conducted to assess both building and collection security, including current procedures and protection devices. In addition to aspects of health and safety, training should encompass best practice techniques for handling genetic samples and the appropriate use of cold-storage equipment (see [[#Training|OPERATIONAL BEST PRACTICE: Training]]). Many genetic collections currently store samples in a room or facility that remains unlocked during the day, which is likely because many research collections are stored within college and university laboratories allowing student access <ref name=ZimkusFord2014/>. If access to rooms where genetic resources are stored must remain unimpeded, individual freezer units can be locked with key access restricted to approved and trained users. Policies should be developed in relation to visitors to ensure that they have the appropriate training before working with collections (see [[#Training|OPERATIONAL BEST PRACTICE: Training]]). Records of training and activity in the collection areas should be maintained  and archived for security, as well as health and safety requirements  (see [[#Records management|OPERATIONAL BEST PRACTICE: Records Management]]).
+Genetic  samples  have  significant  inherent  value  to  research because they are often collected from remote locations as a result of costly and time-consuming collection trips. Samples should, therefore, be stored in secure locations to minimize misplacement or inadvertent loss, and their access and use should be limited to those with the appropriate training. A risk assessment should be conducted to assess both building and collection security, including current procedures and protection devices. Many genetic collections currently store samples in a room or facility that remains unlocked during the day, which is likely because many research collections are stored within college and university laboratories allowing student access <ref name=ZimkusFord2014/>. If access to rooms where genetic resources are stored must remain unimpeded, individual freezer units can be locked with key access restricted to approved and trained users. Policies should be developed in relation to visitors to ensure that they have the appropriate training before working with collections (see [[#Training|OPERATIONAL BEST PRACTICE: Training]]). Records of training and activity in the collection areas should be maintained  and archived for security, as well as health and safety requirements  (see [[#Records management|OPERATIONAL BEST PRACTICE: Records Management]]).
 <br>
 ===Space planning===
-Space planning encompasses the organization of equipment (e.g.,
+Space planning encompasses the organization of equipment (e.g., storage units, tools), adequate workspaces, and storage for supplies, in addition to the collections themselves. Although the layout of a functioning work area might not be greatly altered for an established collection, minor changes can be made to the placement of laboratory tables, desks, shelving, biosafety cabinets, or benchtop equipment (e.g., centrifuges, electrophoresis equipment, incubators, rockers, scales, spectrophotometers, tabletop autoclaves), that can increase research efficiency or improve functioning of equipment. Understanding every procedure that will be undertaken in the space will allow more accurate organization of the space, which is essential for those designing a centralized repository, as well as those working to improve the organization of a single laboratory. The inclusion of dedicated space for working with genetic samples or hazardous chemicals (e.g., biosafety cabinet, chemical hood, designated laboratory bench, room) is recommended to protect both personnel and samples.<ref>Savolainen,  V., M.P.  Powell, K. Davies, A. Corthals,  and G. Reeves (eds). 2006. DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice  and Uses. Kew Publishing, Royal  Botanic  Garden, Kew, England. 151 pp.</ref>
-storage units, tools), adequate workspaces, and storage for supplies, in addition to the collections themselves.  Although the layout of a functioning work area might not be greatly altered for an established collection, minor changes can be made to the placement of  laboratory tables, desks, shelving, biosafety cabinets, or benchtop equipment (including centrifuges, electrophoresis equipment, incubators, rockers, scales, spectro- photometers, and tabletop autoclaves), that  can increase research efficiency or improve functioning  of equipment.  Understanding every procedure that will be undertaken in the space will allow more accurate organization of the space, which is essential  for  those designing a centralized repository,  as well as those working to improve the organization of a single laboratory. The inclusion of dedicated space for working with genetic samples or hazardous chemicals (e.g., biosafety cabinet, chemical hood, designated  laboratory bench, or room) is recommended  to protect both personnel and samples.<ref>Savolainen,  V., M.P.  Powell, K. Davies, A. Corthals,  and G. Reeves (eds). 2006. DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice  and Uses. Kew Publishing,  Royal  Botanic  Garden,  Kew, England.  151 pp.</ref> An essential, efficiency-improving addition might be a dedicated cold-storage unit for specimens being actively processed, either prior to permanent storage, or while being subsampled or aliquoted for a loan/gift.  Cold-storage  units  should  be  selected  and organized based on their work purpose, because the type of storage might differ between those  used for  temporary storage (e.g., refrigerator units,  freezer units) and those for long-term (e.g., mechanical  freezer units, liquid nitrogen cryovats).
 <br>
 <Br>
-In a genetic resource collection, open spaces must be reviewed along with dedicated storage areas.  Efforts  should  be made to ensure that  mechanical  refrigerator and freezer units are placed with sufficient space around  them to allow for adequate  airflow because compressors can  overheat  if units  are  placed  too  close to  other  units  or  walls. Moveable  or  mobile equipment,  including laboratory carts or dewars (cylinders) of liquid nitrogen (LN2), should have dedicated resting places so as to not obstruct exits, access, or equipment, including fire extinguishers, eyewashes, or safety  showers.  In  addition, routes  traversed for specimen transport, maintenance of equipment, and delivery of dewars of LN2, should be reviewed to consider facility and/or safety issues, such as elevators (e.g., personnel may not transport pressurized dewars in elevators if ventilation does not accommodate oxygen deficiencies), steep inclines, floor surfaces, and movement through  populated and public areas.
+Open spaces must be reviewed along with dedicated storage areas to:
-<br>
+* Ensure that mechanical refrigerator and freezer units are placed to allow for adequate airflow
+* Avoid obstruction of exits, access or equipment (e.g., fire extinguishers, eyewashes, safety showers) by dedicating spaces for mobile equipment (e.g., laboratory carts, dewars/cylinders of LN<sub>2</sub>)
+* Consider facility and/or safety issues associated with routes traversed for specimen transport, maintenance of equipment, and delivery of dewars of LN<sub>2</sub>, including:
+::- Elevators (e.g., personnel may not transport pressurized dewars in elevators if ventilation does not accommodate oxygen deficiencies)
+::- Steep inclines
+::- Floor surfaces
+::- Movement through populated and public areas
 ===Lighting===
-Lighting in the collection space should be sufficient to allow personnel to complete small-scale tasks, including examining vials for cracks, reading hand-written or typed labels on containers or subsampling specimens.  If  the light source is in  close proximity to frozen  samples (i.e., task  lighting),  a lighting unit  that  generates  minimal heat (e.g., florescent fixtures, LEDs) should be used instead of incandescent or halogen lighting because these latter can cause samples to thaw. Emergency lighting that functions in the event of power loss should also be present to illuminate exit routes and, if needed, allow personnel to monitor  cold-storage  equipment  (see [[#Backup precautions|FACILITY  MANAGEMENT: Backup Precautions]]).  Focused, portable   light  sources (e.g., flashlights, headlamps, battery-powered lanterns) should  also  be  readily  available  within  the  collection in case of emergencies or if needed to examine equipment.
+Lighting in the collection space should be sufficient to allow personnel to complete small-scale tasks, including:
+*Examining vials for cracks
+*Reading hand-written or typed labels on containers
+*Subsampling specimens<br>
+If the light source is in close proximity to frozen samples (i.e., task  lighting), a lighting unit that generates minimal heat (e.g., florescent fixtures, LEDs) should be used instead of incandescent or halogen lighting because these latter can cause samples to thaw. Emergency lighting that functions in the event of power loss should also be present to illuminate exit routes and, if needed, allow personnel to monitor cold-storage equipment  (see [[#Backup precautions|FACILITY  MANAGEMENT: Backup Precautions]]).  Focused, portable  light sources (e.g., flashlights, headlamps, battery-powered lanterns) should  also be readily available within the collection in case of emergencies or if needed to examine equipment.
 <br>
 === Flooring ===
-Flooring  used in  genetic repositories should be durable enough to accommodate all activities performed in the space. Flooring surfaces should be washable, able to support heavy cold-storage equipment without cracking, and level so as not to obstruct the movement of equipment, including laboratory carts and dewars (cylinders) of LN2.  If  LN2 is being used, the flooring  should  not  crack  if spills or leaks occur. Flooring surfaces, such as vinyl tile and linoleum, are not recommended  because they can crack and lift, presenting a hazard.  Sealed concrete is recommended over epoxy because if LN2 is spilled on the latter, it can break the seal between the epoxy and concrete, causing cracking.  If harder  surfaces,  such as concrete, are selected because  of their  durability, anti-fatigue mats should be placed in areas where personnel  stand  for prolonged periods of time for potential ergonomic issues. Additionally, absorbing  mats or floor grates might be needed in the front  of refrigerator condensers  or in the vicinity of freezers to protect personnel  from slipping on occasional  condensation or ice.
+Flooring used in genetic repositories should be durable enough to accommodate all activities performed in the space and be:
+*Washable
+*Able to support heavy cold-storage equipment without cracking
+*Level so as not to obstruct the movement of equipment, including laboratory carts and dewars (cylinders) of LN<sub>2</sub>
+*Compatible with LN<sub>2</sub> so cracks do not occur with spills or leakage. Additional notes regarding flooring and LN<sub>2</sub>:
+::-Vinyl tile and linoleum are not recommended with the use of LN<sub>2</sub> because they can crack and lift, presenting a hazard.
+::-Sealed concrete is recommended over epoxy because if LN<sub>2</sub> is spilled on the latter, it can break the seal between the epoxy and concrete, causing cracking <br>
+If harder surfaces, such as concrete, are selected because of their durability, anti-fatigue mats should be placed in areas where personnel stand for prolonged periods of time for potential ergonomic issues. Additionally, absorbing mats or floor grates might be needed in the front of refrigerator condensers or in the vicinity of freezers to protect personnel from slipping on occasional condensation or ice.
 <br>
 === Ventilation ===
-Ventilation must be adequate in all collection spaces to prevent excess heat or humidity and, more importantly if using LN2,
+Ventilation must be adequate in all collection spaces to prevent excess heat or humidity, which cause mechanical units to overheat and create condensation that damages equipment and results in an electrical shock hazard. More importantly, ventilation must consistently maintain sufficient oxygen levels if using LN<sub>2</sub>. Using liquid nitrogen for maintaining genetic collections requires constant monitoring of oxygen levels because nitrogen is a colorless, odorless and tasteless gas/vapor that is an asphyxiant, causing oxygen depletion. If LN<sub>2</sub> leaks into an enclosed space from a defective cryovat or supply dewar, oxygen levels might become depleted enough to be unsafe for occupants (see [[#Liquid nitrogen safety|HEALTH AND SAFETY: Liquid Nitrogen Safety]]).
-it  must consistently maintain sufficient oxygen levels. Excess heat  and  humidity  within  collections  cause mechanical units to overheat and create condensation, which can damage equipment  and result in an electrical shock hazard.  Using liquid nitrogen for maintaining genetic collections requires constant monitoring of oxygen levels because  nitrogen   is  a  colorless, odorless and tasteless gas/vapor that is an asphyxiant, causing oxygen depletion. If LN2 leaks into an enclosed space from a defective cryovat or supply dewar, oxygen levels might become depleted enough to be unsafe for occupants (see [[#Liquid nitrogen safety|HEALTH AND SAFETY: Liquid Nitrogen Safety]]). To understand potential oxygen depletion due to LN2 use in a genetic collection, the normal evaporative losses from storage vessels and the spillage of the entire contents of a vessel should be estimated for each collection room. Potential  oxygen depletion can be  determined   by  analyzing  the  size of the  room,  evaporation loss for each vessel (reported  by the manufacturer as ‘‘volume of LN2 lost per day’’), total spillage of each vessel, and the number of air changes in the room per hour. If neither normal evaporation losses nor spillage cause a significant reduction  of oxygen content in a room, then general exhaust ventilation or use of natural ventilation (e.g., opening doors, windows) can be considered as an option to maintain safe oxygen levels. Natural ventilation is not always possible, however, because some laboratories might have institutional restrictions or special designations (e.g., Biosafety Level 2 or 3) requiring that windows are sealed and doors shut during operation. If risk assessment calculations of potential  oxygen depletion indicate that evaporation losses and/or spillage would significantly deplete oxygen concentrations, forced-air  ventilation  must  be installed.  For accuracy in such high-risk matters, a professional  engineer should be contacted  and the health and safety group of the institution consulted.
 <br>
-<Br>
+To understand potential oxygen depletion due to LN<sub>2</sub> use in a genetic collection, the normal evaporative losses from storage vessels and the spillage of the entire contents of a vessel should be estimated for each collection room. Potential  oxygen depletion can be determined by analyzing the following:
-Forced-air ventilation can include extractor  fans that  run continually, or fans that  are either activated manually or automatically. An extractor fan that runs continually provides 100% exhaust and assures that none of the cycled air is returned  back to the air handler. A noncontinuous extractor fan is a ventilation system activated in one of two ways: manually by the user when alerted that oxygen levels are low or, preferably, by an automatic trigger because this option removes the need for human intervention to rectify the issue. Automatic activation  of an extractor fan can be linked to sensors that detect room occupancy and/or oxygen levels (see [[#Oxygen monitors|FACILITY MANAGEMENT: Oxygen Monitors]]). Using oxygen levels to activate an extractor  using a predetermined set point has the advantage  that it can remove built-up nitrogen that results from slow leakage when a room is not occupied. Having both occupancy sensors and oxygen levels  activate an extractor fan serves as a safety redundancy should one sensor fail. Regardless  of the type of ventilation system chosen, exhaust systems should include forced extraction  ducts that  are installed at low heights close to the floor because cold nitrogen vapors are denser than ambient air and settle at floor level. Exhaust  ducts should also be in close proximity to storage units for the most efficient removal. With all ventilation  systems, noise exposure from fans must fall within limits recommended  by the Occupational Safety and Health  Administration (OSHA), and collection managers  should contact  their environmental health and safety group to evaluate the noise levels and attenuate the fans if needed.
+*Size of the room
+*Evaporation loss for each vessel (reported  by the manufacturer as ‘‘volume of LN<sub>2</sub> lost per day’’)
+*Total spillage of each vessel
+*Number of air changes in the room per hour<br>
+If neither normal evaporation losses nor spillage cause a significant reduction of oxygen content in a room, then general exhaust ventilation or use of natural ventilation (e.g., opening doors, windows) can be considered as an option. Natural ventilation is not always possible, however, because of institutional restrictions or special designations (e.g., Biosafety Level 2 or 3) requiring that windows are sealed and/or doors shut. If risk assessment calculations of potential oxygen depletion indicate that evaporation losses and/or spillage would significantly deplete oxygen concentrations, forced-air ventilation must be installed. For accuracy in such high-risk matters, a professional  engineer should be contacted  and the health and safety group of the institution consulted. <br>
 <br>
+Forced-air ventilation can include the following:
+*Extractor fans that run continually, providing 100% exhaust and assuring that none of the cycled air is returned back to the air handler
+*Fans that are activated manually by the user when alerted that oxygen levels are low
+*Fans that are activated automatically by an automatic trigger
+Fans that use an automatic trigger are recommended over those with manual activation to remove need for human intervention to correct oxygen levels. Automatic activation of an extractor fan can be linked to sensors that detect room occupancy and/or oxygen levels (see [[#Oxygen monitors|FACILITY MANAGEMENT: Oxygen Monitors]]). Having both occupancy sensors and oxygen levels  activate an extractor fan serves as a safety redundancy should one sensor fail. Regardless of the type of ventilation system chosen, exhaust systems should include forced extraction ducts that are installed at low heights close to the floor because cold nitrogen vapors are denser than ambient air and settle at floor level. Exhaust ducts should also be in close proximity to storage units for the most efficient removal. With all ventilation systems, noise exposure from fans must fall within limits recommended by the Occupational Safety and Health  Administration (OSHA), and collection managers should contact their environmental health and safety group to evaluate the noise levels and attenuate the fans if needed.
+<br>
+[[File:Oxygen_monitor.png|thumb|right|Delta F Series Oxygen Monitor (electrically operated and permanent; sensor positioned close to floor level and not shown)]]
 === Oxygen monitors ===
-Ambient  air  normally contains 20.9% oxygen by volume, but nitrogen gas can quickly displace the air in the event of a spill or failure of storage equipment, reducing the percent of oxygen to unsafe levels.  By OSHA standards, a ‘‘hazardous atmosphere’’ can include one that is oxygen-deficient, containing  less than 19.5% oxygen by volume. This type of environment exposes people to the risk of incapacitation, impairment of ability to self-rescue (i.e., escape the area  unaided), injury, acute illness, or possible death. Oxygen monitors should, therefore, be present in all rooms where LN2 is stored or dispensed, and these monitors are essential in rooms where personnel are working with LN2 storage equipment.  Some ventilation systems using extractor fans can be automatically activated using oxygen levels; these systems can operate  independently or be tied into the general room oxygen monitors ([[#Ventilation|see FACILITY MANAGEMENT: Ventilation]]).
+Ambient air normally contains 20.9% oxygen by volume, but nitrogen gas can quickly displace the air in the event of a spill or failure of storage equipment, reducing the percent of oxygen to unsafe levels.  By OSHA standards, a ‘‘hazardous atmosphere’’ can include one that is oxygen-deficient, containing  less than 19.5% oxygen by volume. This type of environment exposes people to the risk o incapacitation, injury and possible death. Oxygen monitors should, therefore, be present in all rooms where LN<sub>2</sub> is stored or dispensed, and these monitors are essential in rooms where personnel are working with LN<sub>2</sub> storage equipment.  Some ventilation systems using extractor fans can be automatically activated using oxygen levels; these systems can operate  independently or be tied into the general room oxygen monitors (see [[#Ventilation|FACILITY MANAGEMENT: Ventilation]]). Oxygen monitors can be either portable or permanently installed within the collection space:
-<br>
+*Portable monitors are small, light-weight, and can be carried by individuals working in a room with LN<sub>2</sub> equipment
-<Br>
+*Permanent installations (i.e., battery operated, electrical units) ensure constant and consistent surveillance of oxygen levels
-Oxygen monitors can be either portable or permanently installed within the collection space; their placement might be regulated by local authorities. Portable monitors are small, light-weight, and can be carried by individuals working in a room  with LN2 equipment. Permanent installations, which are either battery  operated  or electrical units mounted to the  walls, are recommended over portable units to ensure constant and consistent surveillance  of oxygen levels. Displays  that  continuously indicate the oxygen level and include alarms should be mounted approximately at eye level; however, sensors should be positioned closer to floor level but above the level of any exhaust-extraction fan located in close  proximity.  To assure that oxygen monitors  comply with local regulations and function accurately, a professional engineer should be contacted and the health and safety group of the institution consulted. Regardless of whether these devices are fixed or mobile, oxygen monitors should  include both audible and visual alarms.  Additional alarms in adjacent rooms or  hallways  are recommended to prevent personnel from potentially entering a room  with deficient oxygen. Alarm  notification  to a remote location is also a worthwhile precaution, because  emergency personnel and those responsible for  the collection can be alerted  to problems. Unfortunately, some electrochemical sensors used within oxygen monitors are sensitive to the surrounding environment and are subject to drift with barometric changes or can even fail if placed in extremely cold temperatures. In addition, the sensors used within some oxygen monitors can become saturated over time, so they must be replaced at regular intervals. Dedicated maintenance  and periodic calibration of the monitoring  devices is therefore essential for all collections using LN2. Both the SOP document and comprehensive guide to operation should contain the information needed to properly  maintain  and regularly test oxygen-monitoring equipment.
+::- Displays should be mounted approximately at eye level
+::- Oxygen sensors should be positioned closer to floor level but above the level of any exhaust-extraction fan located in close proximity
+::- Additional alarms in adjacent rooms or hallways are recommended to prevent personnel from entering an oxygen deficient areas
+::- Alarm notification to a remote location is a worthwhile precaution so emergency personnel and those responsible can be alerted to problems.<br>
+Regardless of whether these devices are fixed or mobile, oxygen monitors should include both audible and visual alarms. To assure that oxygen monitors comply with local regulations and function accurately, a professional engineer should be contacted and the health and safety group of the institution consulted. In addition, some electrochemical sensors used within oxygen monitors are sensitive to the surrounding environment and are subject to drift with barometric changes or can even fail if placed in extremely cold temperatures. Therefore, dedicated maintenance, periodic calibration and regular replacement of sensors is essential for all collections using LN<sub>2</sub>.
 <br>
 === Backup precautions ===
-Collections that use cold-storage units to store genetic samples should include backup precautions to protect against power loss and ensure constant temperatures, thereby preventing sample loss.<ref>Hanner, R., A. Corthals, and H.C. Dessauer. 2005. Salvage of genetically valuable tissues following a freezer failure. Molecular Phylogenetics and Evolution 34:452–455.</ref>  Backup  precautions are the necessary counterpart to a monitoring program, which protects samples from loss due to specific equipment failure (see OPERATIONAL BEST  PRACTICE: Manual  Monitoring). Fortunately, audible or visual alarms are included in many cold-storage  units,  but  are merely the first step in protecting genetic samples. A risk assessment should be conducted to determine   the   appropriate backup system given the cold-storage type (e.g., refrigerator, mechanical freezer, LN2 cryovats),    institutional infrastructure (e.g., available backup  power sources), regional factors (e.g., risk of severe weather, proximity to populated areas), and the running duration of each type of backup  system. Automatic systems are recommended  over  those  that  must  be activated manually to ensure that collection storage equipment remains functional at all times, even when personnel are not readily available. It is also recommended  that equipment alarms include both on-site and off-site notifications. Off-site alarms include 24-hour monitoring and ensure that the appropriate personnel can be contacted  at any time in case of emergency. Contact information for  multiple  staff members trained to respond to  emergencies  should  be included in the SOP document and posted within the collection to ensure that emergencies and alarms are addressed appropriately and immediately. Written emergency procedures should address how personnel should respond to various situations (see OPERATIONAL BEST  PRACTICE: Emergency Procedures).
+Collections that use cold-storage units to store genetic samples should include backup precautions to protect against power loss and ensure constant temperatures, thereby preventing sample loss.<ref>Hanner, R., A. Corthals, and H.C. Dessauer. 2005. Salvage of genetically valuable tissues following a freezer failure. Molecular Phylogenetics and Evolution 34:452–455.</ref>  Backup  precautions are the necessary counterpart to a monitoring program, which protects samples from loss due to specific equipment failure ([[#Manual Monitoring|see OPERATIONAL BEST  PRACTICE: Manual  Monitoring]]). Fortunately, audible or visual alarms are included in many cold-storage  units,  but  are merely the first step in protecting genetic samples. A risk assessment should be conducted to determine the appropriate backup system given the following:
+*Cold-storage type (e.g., refrigerator, mechanical freezer, LN<sub>2</sub> cryovats)
+*Institutional infrastructure (e.g., available backup  power sources)
+*Regional factors (e.g., risk of severe weather, proximity to populated areas)
+*Running duration of each type of backup system
+Automatic systems are recommended over those that must be activated manually to ensure that collection storage equipment remains functional at all times, even when personnel are not readily available. It is also recommended  that equipment alarms include both on-site and off-site notifications. Off-site alarms include 24-hour monitoring and ensure that the appropriate personnel can be contacted at any time in case of emergency. Contact information for multiple staff members trained to respond to  emergencies should  be included in the SOP document and posted within the collection to ensure that emergencies and alarms are addressed appropriately and immediately. Written emergency procedures should address how personnel should respond to various situations ([[#Emergency procedures|see OPERATIONAL BEST  PRACTICE: Emergency procedures]]).
 <br>
 <Br>
-As part of a risk assessment, collection managers should identify what equipment is essential and requires backup power in the event of power loss. Risk assessments should be conducted regularly because contents of individual cold-storage units  can change, which might alter priorities for backup power. Mechanical freezers should always be connected to backup power.  Managers of collections using LN2 storage units should consider having  backup  power for the LN2 cryovat controllers  to ensure that cryovat units continue to receive LN2 supply from dewars when the commercial power is not present; however, the addition of LN2 can be done manually if needed (see GENETIC AND GENOMIC COLLECTION STORAGE: Liquid Nitrogen Cryovats).  Environmental monitoring systems and safety equipment, such as oxygen sensors, specialized ventilation, and emergency lighting, should also be protected by backup measures.
+As part of a risk assessment, collection managers should identify what equipment is essential and requires backup power in the event of power loss. Risk assessments should be conducted regularly because contents of individual cold-storage units  can change, which might alter priorities for backup power. Mechanical freezers should always be connected to backup power. Managers of collections using LN<sub>2</sub> storage units should consider having backup power for the LN<sub>2</sub> cryovat controllers to ensure that cryovat units continue to receive LN<sub>2</sub> supply from dewars when the commercial power is not present; however, the addition of LN<sub>2</sub> can be done manually if needed ([[#Liquid nitrogen cryovats|see GENETIC AND GENOMIC COLLECTIONS STORAGE: Liquid nitrogen cryovats]]).  Environmental monitoring systems and safety equipment, such as oxygen sensors, specialized ventilation, and emergency lighting, should also be protected by backup measures.
 <br>
 <Br>
-If regular power is lost, an auxiliary or emergency-power system generally uses an automatic transfer   switch  to  connect  to emergency power. Most emergency-power systems  use diesel, natural  gas, or liquid propane gas-driven generators  to  power the identified essential equipment in a facility. Multiple generators might be necessary to support large collections if many mechanical freezers are present. Enough fuel should be present to sustain power continuously for at least 48 to 72 hours, but there also should be an established plan for how fuel supplies can be replenished if needed. <ref>International Society for Biological and Environmental Repositories. 2012. 2012 Best practices for repositories: Collection, storage, retrieval, and distribution of biological materials for research. Biopreservation and Biobanking 10:79–161.</ref>  An uninterruptible power supply (also called uninterruptible power source, UPS) or battery/ flywheel  backup can also provide  short-term emergency  power  if commercial  utility power fails. UPS units are designed as a steady, continuous power source during interim breaks in power and generally only function for relatively short periods of time. In an emergency situation,  these units can provide personnel with essential time to connect to other secondary power sources, such as backup generators.  In addition, some mechanical freezers require users to manually restart the unit after a power failure to protect the compressors, and an UPS would make this restart unnecessary. Power systems should be stored in an easily accessible and  dedicated storage  space so collection  personnel can access them when needed. All backup power systems should be tested on a regular basis as part of the SOP to ensure that they function and can sustain the electrical load in an emergency (see POLICY BEST  PRACTICE).
+If regular power is lost, an auxiliary or emergency-power system can automatically connect to emergency power. Most emergency-power systems use diesel, natural  gas, or liquid propane gas-driven generators to power essential equipment in a facility. Managers evaluating emergency-power systems should consider the following:
+*Multiple generators might be necessary to support large collections if many mechanical freezers are present.
+*Enough fuel should be present to sustain power continuously for at least 48–72 hours, but there also should be an established plan for how fuel supplies can be replenished if needed. <ref>International Society for Biological and Environmental Repositories. 2012. 2012 Best practices for repositories: Collection, storage, retrieval, and distribution of biological materials for research. Biopreservation and Biobanking 10:79–161.</ref>
+*An uninterruptible power supply (also called uninterruptible power source, UPS) or battery/ flywheel  backup can also provide short-term emergency power if commercial utility power fails. In an emergency situation, these units can provide personnel with essential time to connect to other secondary power sources, such as backup generators. In addition, some mechanical freezers require users to manually restart the unit after a power failure to protect the compressors, and an UPS would make this restart unnecessary.
+*Power systems should be stored in an easily accessible and dedicated storage space so collection personnel can access them when needed.
+*All backup power systems should be tested on a regular basis as part of the SOP to ensure that they function and can sustain the electrical load in an emergency.
 ==Genetic and Genomic Collections Storage==
-The type of storage used in a genetic or genomic collection ultimately influences the potential  future uses of samples in molecular research because colder temperatures reduce cellular degradation. Documentation of the  number of  freeze–thaw  events and any chemical preservatives or buffers should also be considered because genetic sample integrity might be reduced, depending  on the preparation,as well as the duration and number of freeze–thaw  cycles. Collection managers  must, therefore, track  all storage methods utilized and usage events for their genetic samples from the time of initial collecting until their use for research.
+The type of storage used in a genetic or genomic collection ultimately influences the potential future uses of samples in molecular research because colder temperatures reduce cellular degradation. Documentation of the number of  freeze–thaw events and any chemical preservatives or buffers should also be considered because genetic sample integrity might be reduced, depending on the preparation, as well as the duration and number of freeze–thaw cycles. Collection managers should also track all storage methods utilized from the time of initial collecting and any usage events (i.e., loans/gifts).
 <br>
 ===Temperature considerations===
-Collections  might include genetic samples preserved in a number of ways, depending  on the size of the collection  (including  estimated  future growth), personnel, funding, dedicated space for equipment, and length of  time the samples will be stored. Cryopreservation at very cold temperatures is considered the most effective technique for the long-term stabilization  of genetic samples because it inhibits enzymatic and chemical activity that leads to sample degradation <ref>Engstrom,  M.D., R.W. Murphy, and O. Haddrath. 1990. Sampling vertebrate  collections for molecular research: Practice and policies. Pp. 315–330 in Managing the Modern Herbarium (D.A. Metsger and S.C. Byers, eds.). Granville  Island  Publising, Vancouver,  Canada. 384 pp.</ref> <ref>Karlsson,   J.O.   and   M.   Toner.   1996.  Long-term   storage   of  tissues  by  cryopreservation:  Critical   issues. Biomaterials  17:243–256.</ref> <ref>Kilpatrick, C.W. 2002. Noncryogenic  preservation  of mammalian  tissues for DNA  extraction:  An assessment of storage  methods.  Biochemical Genetics 40:53–62.</ref> <ref>Mutter,   G.L.,  D.  Zahrieh,   C.  Liu,  D.  Neuberg,   D.  Finkelstein,   H.E.  Baker,  and  J.A.  Warrington.  2004. Comparison of frozen and RNALater solid tissue storage methods for use in RNA expression microarrays. BMC Genomics  5:88.</ref> <ref>Corthals,  A. and R. DeSalle. 2005. An application of tissue and DNA  banking  for genomics and conservation: The Ambrose  Monell Cryo-Collection (AMCC).  Systematic Biology 54:819–823.</ref>( When  genetic sample temperatures are reduced below -137°C (the vitrification point of water), biological activity substantially slows and, at -196°C (the boiling point of liquid nitrogen), DNA degradation virtually stops because there is insufficient thermal energy for chemical reactions. Thus, the type of cold storage chosen for samples affects the long-term  viability of those samples, with the most reliable form of cryogenic preservation being the storage of samples at temperatures below -137°C and improving as storage temperatures decrease below this threshold.
+Cryopreservation at very cold temperatures is considered the most effective technique for the long-term stabilization of genetic samples because it inhibits enzymatic and chemical activity that leads to sample degradation <ref>Engstrom,  M.D., R.W. Murphy, and O. Haddrath. 1990. Sampling vertebrate  collections for molecular research: Practice and policies. Pp. 315–330 in Managing the Modern Herbarium (D.A. Metsger and S.C. Byers, eds.). Granville  Island  Publising, Vancouver,  Canada. 384 pp.</ref> <ref>Karlsson,  J.O.  and  M. Toner. 1996.  Long-term   storage   of  tissues  by  cryopreservation:  Critical   issues. Biomaterials  17:243–256.</ref> <ref>Kilpatrick, C.W. 2002. Noncryogenic  preservation  of mammalian  tissues for DNA  extraction:  An assessment of storage  methods. Biochemical Genetics 40:53–62.</ref> <ref>Mutter,   G.L.,  D.  Zahrieh,   C.  Liu,  D.  Neuberg,   D.  Finkelstein,   H.E.  Baker,  and  J.A.  Warrington.  2004. Comparison of frozen and RNALater solid tissue storage methods for use in RNA expression microarrays. BMC Genomics  5:88.</ref> <ref>Corthals,  A. and R. DeSalle. 2005. An application of tissue and DNA  banking  for genomics and conservation: The Ambrose  Monell Cryo-Collection (AMCC).  Systematic Biology 54:819–823.</ref>When genetic sample temperatures are reduced below -137°C (the vitrification point of water), biological activity substantially slows and, at -196°C (the boiling point of liquid nitrogen), DNA degradation virtually stops because there is insufficient thermal energy for chemical reactions. Thus, the type of cold storage chosen for samples affects the long-term viability of those samples, with the most reliable form of cryogenic preservation being the storage of samples at temperatures below -137°C and improving as storage temperatures decrease below this threshold. However, collections might include genetic samples preserved in a number of ways, given size of the collection (including  estimated  future growth), personnel, funding, dedicated space for equipment, and ength of time the samples will be stored.
 <br>
-In addition  to long-term storage in a collection, there must be considerations for short- term storage situations  in relation to when samples are collected and transferred, such as for loans/gifts. Various methods, including freeze-drying samples or preparing  them using buffers, chemical preservatives, or desiccants, are currently used for the initial preservation of genetic samples. <ref>Gemeinholzer,  B., I. Rey, K. Weising, M. Grundmann, A.N.  Mu¨ llner, H. Zetsche,  G. Droege,  O. Seberg, G. Petersen, D.M.  Rawson,  and L.A. Weigt. 2010. Chapter  7—Organizing  specimen and tissue preservation techniques  in  the  field for  subsequent  molecular  analyses.  Pp.  129–157 in  Manual  on Field Recording Techniques and Protocols  for All Taxa  Biodiversity Inventories (J. Eymann,  J. Degreef,  C. Ha¨ user,  J.C. Monje,  Y. Samyn,  and  D. VandenSpiegel,  eds.). Belgian National Focal  Point  to the Global  Taxonomy Initiative,  Brussels, Belgium. 653 pp.</ref> <ref>Nagy, Z.T. 2010. A hands-on  overview of tissue preservation  methods for molecular genetic analyses. Organisms Diversity & Evolution  10:91–105.</ref> <ref>Bus´, M. and  M. Allen. 2014. Collecting  and  preserving  biological  samples from  challenging  environments  for DNA  analysis. Biopreservation and Biobanking  12:17–22.</ref> These methods, which generally allow genetic samples to be stored at room temperature, are most appropriate for short-term storage or transport and not for long-term preservation (see GENETIC SAMPLE PROCESSING: Initial Preservation Procedures). Long-term viability can be increased for genetic samples initially preserved using these methods if they are ultimately stored in a low-temperature environment. In general, genetic samples should be stored at the lowest temperature possible at any available time to reduce degradation and maximize future use.
+In addition  to long-term storage in a collection, there must be considerations for short-term storage situations in relation to when samples are collected and transferred, such as for loans/gifts. Various methods, including freeze-drying samples or preparing  them using buffers, chemical preservatives, or desiccants, are currently used for the initial preservation of genetic samples. <ref>Gemeinholzer,  B., I. Rey, K. Weising, M. Grundmann, A.N.  Müllner, H. Zetsche,  G. Droege,  O. Seberg, G. Petersen, D.M.  Rawson,  and L.A. Weigt. 2010. Chapter  7—Organizing  specimen and tissue preservation techniques  in  the  field for  subsequent  molecular  analyses.  Pp.  129–157 in  Manual  on Field Recording Techniques and Protocols  for All Taxa  Biodiversity Inventories (J. Eymann,  J. Degreef,  C. Ha¨ user,  J.C. Monje,  Y. Samyn,  and  D. VandenSpiegel,  eds.). Belgian National Focal  Point  to the Global  Taxonomy Initiative,  Brussels, Belgium. 653 pp.</ref> <ref>Nagy, Z.T. 2010. A hands-on  overview of tissue preservation  methods for molecular genetic analyses. Organisms Diversity & Evolution  10:91–105.</ref> <ref>Buś, M. and  M. Allen. 2014. Collecting  and  preserving  biological  samples from  challenging  environments  for DNA  analysis. Biopreservation and Biobanking  12:17–22.</ref> These methods, which generally allow genetic samples to be stored at room temperature, are most appropriate for short-term storage or transport and not for long-term preservation ([[#Initial preservation procedures|see GENETIC SAMPLE PROCESSING: Initial preservation procedures]]). Long-term viability can be increased for genetic samples initially preserved using these methods if they are ultimately stored in a low-temperature environment. In general, genetic samples should be stored at the lowest temperature possible at any available time to reduce degradation and maximize future use.
 <br>
 ===Liquid nitrogen cryovats===
-Liquid  nitrogen  cryovats  are cryogenic freezers that are cooled in various ways using a supply of nitrogen in the liquid phase. All methods of cryopreservation that use LN2 are considered to be the most effective because samples are stored at temperatures below the glass-liquid transition temperature of water (-137°C). There are currently four different storage methods that use LN2:
+Liquid  nitrogen  cryovats  are cryogenic freezers that are cooled in various ways using a supply of nitrogen in the liquid phase. All methods of cryopreservation that use LN<sub>2</sub> are considered to be the most effective because samples are stored at temperatures below the glass-liquid transition temperature of water (-137°C). There are currently four different storage methods that use LN2:
-#vapor-phase cryovats that include a standing level of LN2 present below a rotating carousel that houses sample racks (≤-150°C), which was the most commonly used method by collections surveyed by Zimkus and Ford <ref name=ZimkusFord2014/>
+[[File:Cryovat_dewar.png|thumb|right|Vapor-phase cryovat (right) with electronic controller connected to LN<sub>2</sub> supply dewar (left)]]
-#liquid-phase cryovats that allow submersion of samples in nitrogen (-196°C)
+#Vapor-phase cryovats with LN<sub>2</sub> present below sample racks (≤-150°C; most commonly used method by collections surveyed<ref name=ZimkusFord2014/>)
-#isothermal  cryovats  with a specialized  jacket  surrounding the interior chamber and allowing nitrogen vapor to enter the freezer space via directional vents (approximately -190°C)
+#Liquid-phase cryovats that allow submersion of samples in nitrogen (-196°C)
-#MVE Vario cryovats (-50°C to -150°C) that allow LN2 to flow through a heat exchange system located in the top head of the freezer, using vaporization energy of the  LN2 to cool the unit.
+#Isothermal cryovats with a specialized  jacket  surrounding the interior chamber and allowing nitrogen vapor to enter the freezer space via directional vents (approximately -190°C)
-All four types of cryovats are available in various sizes with vial capacities that range from approximately 20,000 to almost 100,000. Use of liquid-phase cryovats are not recommended because nitrogen in a liquid state can penetrate all commercial cryogenic vials if not placed in secondary containment (e.g., polyethylene tubing), making them at risk of exploding when they expand upon warming (see GENETIC SAMPLE PROCESSING: Storage Containers). In addition, cross-contamination can occur when immersing  samples  directly in LN2 without  securing the cryovial in secondary containment.<ref>Clark, G.N. 1999. Sperm   cryopreservation: Is there a significant risk of cross-contamination. Human Reproduction 14:2941–2943.</ref> The circulation of vapor within isothermal cryovats allows for improved visibility due to less clouding at the top of the chamber, but these cold-storage  units have  increased consumption of LN2 when compared to traditional vapor-phase cryovats. MVE Vario TM cryovats are the newest freezer systems, having the benefit of a dry storage area, but this technology is not yet used or tested by natural history collections.<ref name=ZimkusFord2014/>
+#MVE Vario cryovats (-50°C to -150°C) that allow LN<sub>2</sub> to flow through a heat exchange system located in the top head of the freezer, using vaporization energy of the LN<sub>2</sub> to cool the unit
+All four types of cryovats are available in various sizes with vial capacities that range from approximately 20,000–100,000. Use of liquid-phase cryovats are not recommended because nitrogen in a liquid state can penetrate all commercial cryogenic vials if not placed in secondary containment (e.g., polyethylene tubing), making them at risk of exploding when they expand upon warming (see [[#Storage containers|GENETIC SAMPLE PROCESSING: Storage containers]]). In addition, cross-contamination can occur when immersing  samples  directly in LN<sub>2</sub> without  securing the cryovial in secondary containment.<ref>Clark, G.N. 1999. Sperm cryopreservation: Is there a significant risk of cross-contamination. Human Reproduction 14:2941–2943.</ref> The circulation of vapor within isothermal cryovats allows for improved visibility due to less clouding at the top of the chamber, but these cold-storage units have increased consumption of LN<sub>2</sub> when compared to traditional vapor-phase cryovats. MVE Vario cryovats are the newest freezer systems, having the benefit of a dry storage area, but this technology is not yet used or tested by natural history collections.<ref name=ZimkusFord2014/>
 <br>
-Most liquid nitrogen cryovats are equipped with electronic controllers that automatically monitor  and regulate the supply of LN2 to the unit. Liquid levels, temperature readings, and alarms are generally displayed on a controller unit panel. Cryovats with electronic controllers  generally use a two-sensor system to detect LN2 at user-defined levels. When LN2 levels are below the low-level sensor, a solenoid valve is opened, allowing LN2 to enter the cryovat from a nearby source (e.g., small-volume dewar, large volume bulk tank) connected via a cryogenic hose and/or vacuum-jacketed piping (see GENETIC AND  GENOMIC COLLECTION  STORAGE: Liquid Nitrogen  Supply). When LN2 levels reach the high-level sensor, the solenoid valve is closed, stopping  the flow of LN2 into the cryovat. Liquid nitrogen cryovats (i.e., liquid-phase, vapor-phase, isothermal) can  maintain ultracold temperatures for periods of time if they are not opened but, ultimately, they must have LN2 to  maintain  their cold temperatures. In addition to both on-site and remote alarms, it is paramount that cryovats are checked at regular intervals and levels of LN2 are recorded (see OPERATIONAL BEST PRACTICE: Manual Monitoring).  When using LN2 cryovats, backup power for the electronic controller  functions  to keep a continuous supply of  LN2, although the unit itself  stays  cold  without power (see  FACILITY MANAGEMENT:  Backup  Precautions). If a cryovat controller unit  that automatically dispenses  LN2 is not connected to a backup  system, readings of LN2 levels and the addition of more product (i.e., pouring LN2 into the cryovat) need to be done manually. For those cryovats that store samples in the vapor phase (i.e., vapor-phase, isothermal), LN2 would likely need to be supplied at regular intervals to maintain ultracold temperatures if power remains off for an extended period of time and there is no backup connection.  In the event of a power  failure,  collection  procedures  should  detail  if and when cryovat lids are opened to minimize use of LN2 (see OPERATIONAL BEST  PRACTICE: Emergency Procedures).
+Most liquid nitrogen cryovats are equipped with electronic controllers that automatically monitor and regulate the supply of LN<sub>2</sub> to the unit. Liquid levels, temperature readings, and alarms are generally displayed on a controller unit panel. Cryovats with electronic controllers  generally use a two-sensor system to detect LN<sub>2</sub> at user-defined levels. When LN<sub>2</sub> levels are below the low-level sensor, a solenoid valve is opened, allowing product to enter the cryovat from a nearby source (e.g., small-volume dewar, large volume bulk tank) connected via a cryogenic hose and/or vacuum-jacketed piping (see [[#Liquid nitrogen supply|GENETIC AND  GENOMIC COLLECTION  STORAGE: Liquid nitrogen supply]]). When LN<sub>2</sub> levels reach the high-level sensor, the solenoid valve is closed, stopping the flow of product into the cryovat. In addition to both on-site and remote alarms, it is paramount that cryovats are checked at regular intervals and levels of LN<sub>2</sub> are recorded (see [[#Manual monitoring|OPERATIONAL BEST PRACTICE: Manual monitoring]]).  When using LN<sub>2</sub> cryovats, backup power for the electronic controller functions to keep a continuous supply of LN<sub>2</sub>, although the unit itself stays cold without power (see [[#Backup precautions|FACILITY MANAGEMENT: Backup precautions]]). If a cryovat controller unit that automatically dispenses LN<sub>2</sub> is not connected to a backup  system, readings of LN<sub>2</sub> levels and the addition of more product (i.e., pouring LN<sub>2</sub> into the cryovat) need to be done manually; LN<sub>2</sub> would likely need to be supplied at regular intervals to maintain ultracold temperatures if power remains off for an extended period of time. In the event of a power  failure,  collection  procedures  should  detail  if and when cryovat lids are opened to minimize use of LN<sub>2</sub> (see [[#Emergency procedures|OPERATIONAL BEST  PRACTICE: Emergency procedures]]).
 <br>
 ===Liquid nitrogen supply===
-Liquid  nitrogen  to  supply  cryovats  can  be  obtained  and stored in three ways:
+[[File:Cryogenic Liquid Nitrogen Tank.jpg|thumb|right|A liquid nitrogen bulk tank at Palatine in Illinois (Joe Ravi [CC BY-SA 3.0], via Wikimedia Commons)]]
-#delivery in small-volume dewars (cylinders)
-#delivery to large- volume bulk tanks
+Liquid  nitrogen  to  supply  cryovats  can  be  obtained  and stored in three ways:
-#self-production using an on-site LN2  plant.
+#Delivery in small-volume dewars (cylinders)
-If a commercial vendor  is present in the area,  LN2 can be delivered as needed on a regularly scheduled basis. For most small collections, mobile dewars, generally up to 240 liters, are sufficient to supply cryovats. These dewars are generally placed in close proximity  to the cryovats and connected with cryogenic transfer hoses, unless permanent vacuum-jacketed piping designed  to  transfer  cryogenic  liquids is installed  within the repository.  The dewars themselves can be purchased and refilled by a delivery vehicle, or these storage vessels can be leased so that an empty dewar is exchanged for a full one. In addition,  Department of Transportation (DOT) codes regulate the specifications of liquid nitrogen delivery vessels in the  USA,  so  collection  managers  should  be aware if these regulations affect their delivery. LN2 deliveries should be scheduled to minimize the amount  of time that a dewar is not connected to a cryovat to ensure that a cryovat has a  steady  supply  of  LN2. Collection managers should be aware that  LN2 evaporates at a constant rate, which can be affected by the atmospheric conditions, vessel integrity, and manufacturing tolerances. For large collections with many cryovats, a pressurized bulk or microbulk tank should be considered. Depending  on the size of the bulk vessel, the tank might need to be located outside of the building where the collection is housed. If bulk tanks are placed indoors, itmight be possible for external wall boxes to be installed to allow bulk tanks to be filled without having to enter the building. Costly vacuum-jacketed cryogenic pipes are needed to deliver the LN2 from the tank to the point of use, so for cost efficiency, bulk tanks should be located as close to the cryovats as possible. In many areas, bulk tank storage is regulated  by city or state ordinances;  oxygen monitors  are also essential if these storage units are placed indoors (see FACILITY MANAGEMENT: Oxygen Monitors). In smaller collections that are located in remote locations where LN2 cannot be easily delivered, collection managers might consider the use of LN2 plants, which generate nitrogen by separating it out from the ambient  air. The plant-generated LN2 is stored in a tank  that then can be moved and connected to a cryovat. Regardless of how nitrogen is obtained, personnel must balance  multiple competing factors, including product stock versus available space and over-supply  stock versus both cost and leakage, to ensure cryovats have a constant supply. To manage this balance, collection managers should track the amount  of LN2 used to estimate an efficient timeline for when more supply is needed (see OPERATIONAL BEST PRACTICE: Manual  Monitoring).
+#Delivery to large-volume bulk tank
+#Self-production using an on-site LN<sub>2</sub> plant
+Delivery in small-volume dewars (cylinders) by a commercial vendor can be done needed on a regularly scheduled basis. For most small collections, mobile dewars (up to 240 liters) are sufficient to supply cryovats. Dewars are generally placed in close proximity to the cryovats and connected with cryogenic transfer hoses, unless permanent vacuum-jacketed piping designed  to  transfer  cryogenic  liquids is installed  within the repository.  Dewars themselves can be purchased and refilled by a delivery vehicle, or these storage vessels can be leased so that an empty dewar is exchanged for a full one. In addition,  Department of Transportation (DOT) codes regulate the specifications of liquid nitrogen delivery vessels in the  USA,  so  collection  managers  should  be aware if these regulations affect their delivery. LN<sub>2</sub> deliveries should be scheduled to minimize the amount of time that a dewar is not connected to a cryovat to ensure that a cryovat has a steady supply of LN<sub>2</sub>.Collection managers should be aware that LN<sub>2</sub> evaporates at a constant rate, which can be affected by the atmospheric conditions, vessel integrity, and manufacturing tolerances.
+<br>
+For large collections with many cryovats, a pressurized bulk or microbulk tank should be considered. Depending  on the size of the bulk vessel, the tank might need to be located outside of the building where the collection is housed. If bulk tanks are placed indoors, itmight be possible for external wall boxes to be installed to allow bulk tanks to be filled without having to enter the building. Costly vacuum-jacketed cryogenic pipes are needed to deliver the LN<sub>2</sub> from the tank to the point of use, so for cost efficiency, bulk tanks should be located as close to the cryovats as possible. In many areas, bulk tank storage is regulated by city or state ordinances; oxygen monitors are also essential if these storage units are placed indoors (see [[#Oxygen monitors|FACILITY MANAGEMENT: Oxygen monitors]]).
+<br>
+In smaller collections that are located in remote locations where LN<sub>2</sub> cannot be easily delivered, collection managers might consider the use of LN<sub>2</sub> plants, which generate nitrogen by separating it out from the ambient  air. The plant-generated LN<sub>2</sub> is stored in a tank that then can be moved and connected to a cryovat.
+<Br>
 ===Mechanical freezers and refrigerators===
-Mechanical freezers and refrigerators offer a large range of storage temperatures, including ultracold freezers that can sustain temperatures between -50° and -86°C, general-purpose or laboratory freezers that normally operate between -12° and  -30°C for manual defrost models (automatic defrost models allow temperatures to fluctuate more broadly), and general-purpose refrigerators that maintain temperatures between 1° and 12°C. As previously discussed, cryogenic storage at extremely low temperatures is considered the most effective method for the long-term  stabilization of genetic samples. However,  refrigeration is sometimes considered for short- or long-term storage if certain buffers or chemicals were used in sample preservation, and these additives only require that genetic samples be kept below ambient temperature. Collection managers  must record all chemical additions  and preservatives used with their genetic samples to ensure that the samples are stored at the appropriate temperature recommended  by the manufacturer. If multiple cold-storage methods are used within a  collection, the SOP should clearly outline the criteria for storing samples at the different temperatures.
+[[File:Zimkus_Ford_Fig_5_NEW.tif |thumb|right|Storage methods used by genetic resource collections surveyed by in 45 independent collections at 39 different institutions for all collections surveyed (dark grey) and centralized repositories (light grey).<ref name=ZimkusFord2014>Zimkus,  B.M.  and  L.S. Ford.  2014. Genetic  resource  collections  associated  with natural  history  museums:  A survey and analysis to establish a benchmark of standards. Pp. 9–44 in DNA Banking for the 21st  Century. Proceedings of the U.S. Workshop on DNA Banking (W.L. Applequist  and L. Campbell,  eds.). William L. Brown Center,  St. Louis, Missouri.  187 pp.</ref>]]
+Mechanical freezers and refrigerators offer a large range of storage temperatures, including ultracold freezers (-50°– -86°C), general-purpose or laboratory freezers (-12°– -30°C for manual defrost models; automatic defrost models allow temperatures to fluctuate more broadly), and general-purpose refrigerators (1°– 12°C). As previously discussed, cryogenic storage at extremely low temperatures is considered the most effective method for the long-term  stabilization of genetic samples. However, refrigeration is sometimes considered for short- or long-term storage if certain buffers or chemicals were used in sample preservation, and these additives only require that genetic samples be kept below ambient temperature. Collection managers must record all chemical additions and preservatives used with their genetic samples to ensure that the samples are stored at the appropriate temperature recommended  by the manufacturer. If multiple cold-storage methods are used within a  collection, the SOP should clearly outline the criteria for storing samples at the different temperatures.
 <br>
 <Br>
-Freezers and refrigerators are available in a variety of sizes, styles, and  voltages, including  upright or chest  configurations. Many models are available with locks for additional  security (see  FACILITY MANAGEMENT: Access and   Security). Collection managers should ensure that each electrical unit has a dedicated circuit so power is not overloaded,  and that units are positioned to allow for sufficient airflow around them (see FACILITY  MANAGEMENT: Space Planning).  Heat  released from cold-storage equipment should be monitored and counter-balanced by an HVAC or cooling system when needed. Those collection managers purchasing  new equipment should consider freezer units that have increased energy efficiency, which generally ensures that less heat is emitted to the surrounding air. Compressors can also be placed outside of the building for some freezer units, removing the need for HVAC or cooling in the collection space where the mechanical freezer is located.  Fortunately, compressor systems on newer cold-storage units include  those being cooled by water, whereby valves connected to local water sources automatically control the flow needed  to  maintain cooler compressor temperatures, which enhance the stability and reliability of the unit. Because  cold- storage units are integral to the functioning of a genetic or genomic collection, the SOP should  outline specific protocols for regular preventative maintenance and emergency repair of all mechanical units (see OPERATIONAL BEST PRACTICE: Equipment Preventative Maintenance, Repair, and Replacement).
+Freezers and refrigerators are available in a variety of sizes, styles, and voltages, including  upright or chest  configurations. Many models are available with locks for additional  security (see [[#Access and security|FACILITY MANAGEMENT: Access and security]]). Collection managers should ensure that each electrical unit has a dedicated circuit so power is not overloaded, and that units are positioned to allow for sufficient airflow around them (see [[#Space planning|FACILITY MANAGEMENT: Space planning]]). Heat  released from cold-storage equipment should be monitored and counter-balanced by an HVAC or cooling system when needed. Those collection managers purchasing new equipment should consider freezer units that have increased energy efficiency, which generally ensures that less heat is emitted to the surrounding air. Compressors can also be placed outside of the building for some freezer units, removing the need for HVAC or cooling in the collection space where the mechanical freezer is located.  Fortunately, compressor systems on newer cold-storage units include those being cooled by water, whereby valves connected to local water sources automatically control the flow needed to maintain cooler compressor temperatures, which enhance the stability and reliability of the unit. Because cold- storage units are integral to the functioning of a genetic or genomic collection, the SOP should outline specific protocols for regular preventative maintenance and emergency repair of all mechanical units (see [[#Equipment preventative maintenance, repair, and replacement|OPERATIONAL BEST PRACTICE: Equipment preventative maintenance, repair, and replacement]]).
 <br>
 <Br>
-Mechanical freezers and refrigerators require less dedicated time in their day-to-day operation when compared to LN2 cryovats, but collections have an increased risk of loss in the event of mechanical  breakdown or power disruption. Even a short  power outage can be detrimental to samples being stored in a mechanical cold-storage  unit. Battery backup  systems or an UPS are needed to maintain units in the event of a short power outage or until power can be switched over to a robust backup system for longer term emergencies (see FACILITY  MANAGEMENT: Backup Precautions). Internal and, if possible, remote monitoring should be present to prevent sample loss due to mechanical failure of units (see OPERATIONAL  BEST   PRACTICE: Manual Monitoring).  To safeguard against all possible risks, including power outage and  mechanical failure, both monitoring procedures and backup  precautions should be clearly outlined in the collection SOP.
+Mechanical freezers and refrigerators require less dedicated time in their day-to-day operation when compared to LN<sub>2</sub> cryovats, but collections have an increased risk of loss in the event of mechanical  breakdown or power disruption. Even a short  power outage can be detrimental to samples being stored in a mechanical cold-storage  unit. Battery backup  systems or an UPS are needed to maintain units in the event of a short power outage or until power can be switched over to a robust backup system for longer term emergencies (see [[#Backup precaution|FACILITY  MANAGEMENT: Backup precautions]]). Internal and, if possible, remote monitoring should be present to prevent sample loss due to mechanical failure of units (see [[#Manual monitoring|OPERATIONAL BEST  PRACTICES: Manual monitoring]]).  To safeguard against all possible risks, including power outage and  mechanical failure, both monitoring procedures and backup  precautions should be clearly outlined in the collection SOP.
-==Operational Best Practices==
+==Operational Best Practice==
 Genetic and genomic collections are more equipment- and personnel-dependent than traditional natural history specimens, with more catastrophic consequences if storage equipment fails or samples are handled improperly. In addition, genetic samples are consumable resources, so they become more limited with each use for research.
 <Br>
 ===Facility functions and services provided===
-Genetic  resource  collections  can  provide many key services to fulfill institutional missions and assist internal and  external researchers  in achieving project  goals. How broadly and consistently these key services can be addressed is related  to how genetic collections  are set up at an institution (i.e., separate locations or centralized facility). The main functions of most centralized genetic resource facilities  associated with  natural history  museums  include sample  storage, sample tracking, and tissue sub-sampling and/or processing of loans/gifts.<ref name=ZimkusFord2014/> A small percentage of repositories provide additional genetic laboratory functions, including DNA/RNA extraction, polymerase chain reaction (PCR), and sequencing. Although most institutions are moving toward the centralization of genetic resources,  institutions that have  maintained genetic samples within multiple locations have prioritized accessibility to collections for internal researchers; collections are generally stored within the laboratories of the principle investigators  conducting  research using those particular genetic samples, and it is unclear how accessible these samples are to the scientific community.<ref name=ZimkusFord2014/>
+Genetic  resource  collections  can  provide many key services to fulfill institutional missions and assist internal and  external researchers in achieving project goals. How broadly and consistently these key services can be addressed is related  to how genetic collections  are set up at an institution (i.e., separate locations or centralized facility). The main functions of most centralized genetic resource facilities associated with natural history museums  include <ref name=ZimkusFord2014/>:
-<Br>
+*Sample storage
+*Sample tracking
+*Sub-sampling and/or processing of loans/gifts
+A small percentage of repositories provide additional genetic laboratory functions, including DNA/RNA extraction, polymerase chain reaction (PCR), and sequencing.<ref name=ZimkusFord2014/>
 <Br>
-Besides genetic sample maintenance, additional research services could potentially  be provided by genetic resource collections, although  this would be more easily achieved in a centralized facility, including assistance with project planning or proposal submissions, sample collecting, assistance with sample transportation from the field, sample quality assessment  using spectrophotometry or other methods, and student or intern training.<ref>Hanner,  R., A. Corthals,  and  H.C.  Dessauer.  2005. Salvage of genetically valuable  tissues following a freezer failure. Molecular  Phylogenetics and Evolution  34:452–455.</ref> Collections  could also provide or lend supply materials for those researchers who will be depositing samples in the biorepository, including sample vials, sample boxes, reagents, LN2 dewars, dry  shippers, LN2, or dry ice. To ensure that sufficient equipment, supplies, trained personnel,and funding to maintain high-quality specimens are available, and to potentially  offer additional services, collection managers should clearly outline priorities, as well as the molecular laboratory tasks performed by collection staff (e.g., DNA/RNA extractions, fluorometric/spectrophotometric quantification of DNA, DNA  barcoding to identify or confirm identifications), in the SOP document. Policy should include standards for the receipt of  genetic material to the collection, defining how samples and  metadata must  be stored (i.e., acceptable  sample storage vessel sizes and types), labeled, and organized, so personnel can easily incorporate new samples into the collection.
+Besides genetic sample maintenance, additional research services could potentially be provided by genetic resource collections, including assistance with project planning or proposal submissions, sample collecting, assistance with sample transportation from the field, sample quality assessment using spectrophotometry or other methods, and student or intern training.<ref>Hanner,  R., A. Corthals,  and  H.C.  Dessauer.  2005. Salvage of genetically valuable  tissues following a freezer failure. Molecular  Phylogenetics and Evolution  34:452–455.</ref> Collections could also provide or lend supply materials for those researchers who will be depositing samples in the biorepository, including sample vials, sample boxes, reagents, LN<sub>2</sub> dewars, dry  shippers, LN<sub>2</sub>, or dry ice. To ensure that sufficient equipment, supplies, trained personnel,and funding to maintain high-quality specimens are available, and to potentially  offer additional services, collection managers should clearly outline priorities, as well as the molecular laboratory tasks performed by collection staff (e.g., DNA/RNA extractions, fluorometric/spectrophotometric quantification of DNA, DNA  barcoding to identify or confirm identifications) in the SOP document.
 <br>
 ===Personnel===
-Genetic and genomic resource collections must be managed properly and continuously to ensure that samples are properly  stored and maintained,and remain available for use in research. Depending on the size of the collection and institution type, personnel might include a single manager or numerous employees. A recent survey of genetic resource collections associated  with natural history museums found that the vast majority had curators/professors with higher academic  degrees or  collection managers with higher degrees maintaining the collections (Zimkus and Ford 2014). Other personnel working with genetic resources included collection managers without higher degrees, staff or technical assistants, paid and unpaid student assistants, and volunteers. At minimum, collections staff should include a dedicated manager who is trained to manage the day-to- day activities within the collection and can ensure that all procedures are completed as instructed in SOP documents. A collection manager also prevents unauthorized access to storage areas, thus protecting samples from misplacement, accidental thawing, or contamination (Savolainen et al. 2006). Duties and reporting relationships for each staff member should be clearly outlined in a written job description. Collection managers should ensure that all personnel working in the collection have the appropriate training to undertake the duties assigned in their particular job description, especially with regard to health and safety issues. Although it is ideal to hire personnel that have previous experience, it is understandable that many collections must function with the assistance of students, interns, or volunteers owing to limited budgets or their nature as educational institutions. Therefore, adequate training and  oversight by managers is crucial to guarantee that all policies are implemented and the genetic material is protected  for long- term availability. Proper maintenance of genetic resource also requires assistance from additional departments outside of those working directly with the collection, including building maintenance and operations, environmental health and safety, information technology, and security.
+Genetic and genomic resource collections must be managed properly and continuously to ensure that samples are properly stored and maintained. Depending on the size of the collection and institution type, personnel might include a single manager or numerous employees. A recent survey of genetic resource collections associated  with natural history museums found that the vast majority had curators/professors with higher academic degrees or collection managers with higher degrees maintaining the collections <ref name=ZimkusFord2014>Zimkus,  B.M.  and  L.S. Ford.  2014. Genetic  resource  collections  associated  with natural  history  museums:  A survey and analysis to establish a benchmark of standards. Pp. 9–44 in DNA Banking for the 21st  Century. Proceedings of the U.S. Workshop on DNA Banking (W.L. Applequist  and L. Campbell,  eds.). William L. Brown Center,  St. Louis, Missouri.  187 pp.</ref>. Other personnel working with genetic resources included:
+*Collection managers without higher degrees
+*Staff or technical assistants
+*Paid and unpaid student assistants
+*Volunteers
+At minimum, collections staff should include a dedicated manager who is trained to manage the day-to-day activities within the collection and can ensure that all procedures are completed as instructed in SOP documents. A collection manager also prevents unauthorized access to storage areas, thus protecting samples from misplacement, accidental thawing, or contamination<ref name=Savolainen et al. 2006>Savolainen, V., M.P. Powell, K. Davies, A. Corthals, and G. Reeves (eds). 2006. DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice and Uses. Kew Publishing, Royal Botanic Garden, Kew, England. 151 pp.</ref>. Duties and reporting relationships for each staff member should be clearly outlined in a written job description. Collection managers should ensure that all personnel working in the collection have the appropriate training to undertake the duties assigned in their particular job description, especially with regard to health and safety issues. Proper maintenance of genetic resource also requires assistance from additional departments outside of those working directly with the collection, including building maintenance and operations, environmental health and safety, information technology, and security.
 <Br>
 ===Training===
-All  genetic collection staff must receive adequate training to ensure that they can perform  all aspects of their job  description and follow all policies and regulations, including those mandated by international, national, regional, and  local statutes.  All new personnel, including staff, students, interns, and volunteers, should be trained by authorized   staff to understand the details and justification for the SOP documents and comprehensive protocols. Policies should also be developed in relation to both short-term and long-term visiting researchers to ensure that they have the appropriate  training  before working with collections.  Training should outline best practice for working with genetic resources  because improper  handling can reduce the quality and long-term integrity of a sample, which can occur if it thaws or is contaminated by instruments or contacted surfaces (see GENETIC  SAMPLE  PROCESSING: Sample Transfer; USE OF  COLLECTIONS: Aliquoting Samples). In addition, personnel should be trained in database usage and the proper storage of samples in accordance with corresponding database records (see INVENTORY CONTROL AND  DATA MANAGEMENT: Databasing  for Genetic Samples). Training  should also include all aspects of safety and security, including the appropriate use of tools and equipment, proper   personal protective equipment, and risks of working with chemicals  and  biospecimens (see HEALTH AND  SAFETY). Internal  records should be kept of all approved personnel and dates of their various training events, especially because  some  training requires mandatory updates at regular intervals. All training programs should be regularly assessed to make sure that information is up to date, and it is recommended  hat training be done in collaboration with the health  and safety group  at the institution.
+All  genetic collection staff must receive adequate training to ensure that they can perform  all aspects of their job description and follow all policies and regulations, including those mandated by international, national, regional, and  local statutes.  All new personnel, including staff, students, interns, and volunteers, should be trained by authorized  staff to understand the details and justification for the SOP documents and comprehensive protocols. Policies should also be developed in relation to both short-term and long-term visiting researchers to ensure that they have the appropriate training before working with collections. Training should include the following:
+*Best practice for working with genetic resources (see [[#Sample transfer|GENETIC  SAMPLE PROCESSING: Sample transfer]]; [[#Aliquoting samples|USE OF COLLECTIONS: Aliquoting samples]])
+*Database usage and the proper storage of samples in accordance with corresponding database records (see  [[#Databasing for genetic samples|INVENTORY CONTROL AND  DATA MANAGEMENT: Databasing  for genetic samples]])
+*Safety and security, including the appropriate use of tools and equipment, proper personal protective equipment, and risks of working with chemicals and biospecimens
+Internal records should be kept of all approved personnel and dates of their various training events, especially because some training requires mandatory updates at regular intervals. All training programs should be regularly assessed to make sure that information is up to date, and it is recommended that training be done in collaboration with the health and safety group at the institution.
 <Br>
 ===Manual monitoring===
-The  viability of genetic samples is dependent on storage equipment operating at optimum efficiency. Diligent and consistent monitoring by staff ensures that the collection is maintained and all equipment  operates  properly. Cold- storage  equipment requires regular review to ensure that samples are being kept consistently at the appropriate temperature. Automatic alarms are generally present in most units, but personnel should also visually inspect and record the temperature of the equipment on a regular basis (e.g., daily, multiple times per week). The levels in liquid nitrogen cryovats should also be measured manually on a regular basis to confirm that the measured levels match the control displays to ensure the proper  functioning of the equipment.  In addition, managers should evaluate the temperature and nitrogen-level data on a weekly basis to identify any problematic trends. All transportable pressurized vessels, including dewars  (cylinders)  of LN2,  should  be examined upon receipt from outside vendors to check that the pressurization is compatible with the cold-storage equipment  and that there is no visible damage or leakage.  When in use, these vessels should be closely  monitored  to estimate rate of use and ensure that valves are functioning  properly.  Collection procedures should clearly outline how to monitor and check collection equipment, how often it should be done, and how to maintain documentation.
+The viability of genetic samples is dependent on storage equipment operating at optimum efficiency. Collection procedures should clearly outline how to monitor and check collection equipment, how often it should be done, and how to maintain documentation. Diligent and consistent monitoring of the following equipment should be completed:
-<Br>
+*Cold-storage equipment
+::- Personnel should visually inspect and record the temperature of the equipment on a regular basis (e.g., daily, multiple times per week).
+::- Levels in liquid nitrogen cryovats should be measured manually on a regular basis to confirm that the measured levels match the control displays
+::- Temperature and nitrogen-level data should be tracked on a regular basis to identify problematic trends
+*Transportable pressurized vessels, including dewars  (cylinders) of LN<sub>2</sub>, should be examined upon receipt from outside vendors
+::- Dewars should be checked to ensure that pressurization is compatible with the cold-storage equipment
+::- Dewars should have no be visible damage or leakage
+::- When in use, these vessels should be closely monitored to estimate rate of use and ensure that valves are functioning properly<Br>
 ===Equipment preventative maintenance, repair, and replacement===
-Proper functioning of cold-storage equipment is essential for the long-term  stability of genetic material.  All equipment  should have regular  routine  maintenance in accordance with the recommendations of the manufacturer. Preventative  maintenance of mechanical  freezers should include comparing the temperature set-point versus the actual temperature (see OPERATIONAL BEST PRACTICE: Manual Monitoring), testing backup  batteries,  ensuring that gaskets and seals are intact  without  tears, and routine  cleaning of freezer coils and condenser filters. Mechanical freezers also might need to be defrosted  regularly. Another benefit of preventative maintenance, in addition to increased  dependability, is that significant energy savings are associated with regular maintenance of cold-storage equipment, such as  mechanical  freezers.  Liquid  nitrogen   cryovats  should  also  have routine  maintenance to ensure that internal temperature sensors function  properly,  LN2 readings are accurate,  fill valves operate normally, and alarms activate under the defined conditions.  Maintenance of cryovats by collection personnel  should also include regular checks of the insulating  materials (e.g., polystyrene  foam)  fitted  underneath the lid to identify  cracking, which reduces the insulative properties, or  built-up   frost,  which prevents the lid from closing properly. In addition,  ice and frost build up in a sensor tube results in false readings, whereas build up in vacuum-jacketed cryogenic pipes can block the flow of liquid nitrogen  into the cryovat during  the fill cycle.
+Proper functioning of cold-storage equipment is essential for the long-term  stability of genetic material.  All equipment  should have regular routine maintenance in accordance with the recommendations of the manufacturer. Preventative  maintenance of mechanical freezers should include:
-<Br>
+*Comparing the temperature set-point versus the actual temperature (see [[#Manual monitoring|OPERATIONAL BEST PRACTICE: Manual monitoring]])
+*Testing backup batteries
+*Ensuring that gaskets and seals are intact without tears
+*Routine cleaning of freezer coils and condenser filters
+*Regular defrosting
+In addition to increased dependability, regular maintenance of cold-storage equipment, such as mechanical  freezers, is associated with significant energy savings.
+<br>
+Liquid  nitrogen cryovats should have routine maintenance to ensure:
+*Internal temperature sensors function properly
+*LN<sub>2</sub> readings are accurate
+*Fill valves operate normally
+*Alarms activate under the defined conditions
+*Insulating materials (e.g., polystyrene  foam) do not have cracks or  built-up frost
+*No ice or frost build is present in sensor tubes<br>
 <Br>
-Biosafety cabinets and chemical fume hoods should be tested and certified routinely to ensure that they are functioning   appropriately and in compliance with both local regulations and any requirements associated with biosafety level status. Oxygen monitors also need regular maintenance and/or calibration as life safety equipment (see FACILITY MANAGEMENT:  Oxygen  Monitors).  All safety equipment, including eyewashes, safety showers, fire detection units, and fire suppression  systems, should be tested regularly to ensure reliability, which is generally best accomplished in collaboration with the health and safety group of the institution. Managers should  keep records of all routine and special maintenance, including  dates, description  of  the issues (e.g., alarms, incident reports), tests performed, and actions taken to resolve any problems.  The SOP should provide plans, including instructions and schedules for preventative maintenance, calibration, repair, and replacement of equipment.
+Biosafety cabinets and chemical fume hoods should be tested and certified routinely to ensure that they are functioning appropriately and in compliance with both local regulations and any requirements associated with biosafety level status. Oxygen monitors also need regular maintenance and/or calibration as life safety equipment (see [[#Oxygen monitors|FACILITY MANAGEMENT: Oxygen monitors]]).  All safety equipment, including eyewashes, safety showers, fire detection units, and fire suppression systems, should be tested regularly to ensure reliability, which is generally best accomplished in collaboration with the health and safety group of the institution. Managers should keep records of all routine and special maintenance, including  dates, description  of  the issues (e.g., alarms, incident reports), tests performed, and actions taken to resolve any problems.  The SOP should provide plans, including instructions and schedules for preventative maintenance, calibration, repair, and replacement of equipment.
 <br>
 <Br>
-Regular assessments of equipment should be made by collection managers to help establish a timeline for replacement. ISBER  (2012) reports that generally, mechanicalfreezers last from 5 to 15+ years with manufacturers reporting  a range of 8 to 12 years, whereas liquid nitrogen cryovats generally last longer, functioning for 10 to 35 years. Collection managers should track the ages of all equipment  and know the manufacturer’s expected lifespan for each. Based on the age and performance of the equipment, long-range plans for replacement can be anticipated and replacement funding can be ensured. If a cold-storage unit should fail, written procedures should be in place to identify how to transfer the  samples from the failed unit to their emergency storage location (see OPERATIONAL BEST PRACTICE: Emergency Procedures).
+Regular assessments of equipment should be made by collection managers to help establish a timeline for replacement. Mechanical freezers generally last from 5 to 15+ years with manufacturers reporting a range of 8–12 years, whereas liquid nitrogen cryovats generally last longer, functioning for 10–35 years <ref name=ISBER>[ISBER] International Society for Biological and Environmental Repositories. 2012. 2012 Best practices for repositories: Collection, storage, retrieval, and distribution of biological materials for research. Biopreservation and Biobanking 10:79–161.</ref>. Collection managers should track the ages of all equipment  and know the manufacturer’s expected lifespan for each. Based on the age and performance of the equipment, long-range plans for replacement can be anticipated and replacement funding can be ensured. If a cold-storage unit should fail, written procedures should be in place to identify how to transfer the  samples from the failed unit to their emergency storage location  (see [[#Emergency procedures|OPERATIONAL BEST PRACTICES: Emergency procedures]]).
 <Br>
 ===Records management===
-Collection managers should maintain records that detail the collection, processing, storage, and use of each genetic sample. Copies of all relevant permits and acquisition documents  must be maintained by the institution, collection, or laboratory, which detail the legal attainment of all genetic samples either alone or associated with traditional voucher specimens (see POLICY BEST PRACTICE). Besides being a legal obligation for the institution, this information allows both collection managers and end-users to assess the sample history and quality.  Records should also  be maintained for  all curation activity in a genetic collection because of the specialized training and equipment required (see OPERATIONAL BEST PRACTICE: Training). Up-to-date records should be available that document personnel training, equipment activity(e.g., monitoring, preventative maintenance, repairs), safety inspections, and legal compliance (e.g., active permits) as outlined in the SOP.
+Collection managers should maintain records that detail collection, processing, storage and use of samples. Copies of all relevant permits and acquisition documents, which detail the legal attainment of all genetic samples either alone or associated with traditional voucher specimens, must be maintained for both legal obligation and assessment of the sample history and quality. Up-to-date records should be available that document personnel training, equipment activity (e.g., monitoring, preventative maintenance, repairs), safety inspections, and legal compliance (e.g., active permits) as outlined in the SOP.
 <Br>
-Genetic sample data can be recorded as part of an institutional database, which potentially tracks both the original  voucher  specimen and any subsequent associated genetic or genomic  derivatives, or a stand-alone tracking system that is used only for genetic  samples(see INVENTORY CONTROL AND DATA MANAGEMENT: Databasing for Genetic Samples). Documentation of  genetic  sample  locations in cold-storage units should be as precise as possible so that samples can be located quickly (see INVENTORY CONTROL AND DATA MANAGEMENT: Sample Labeling and Tracking). Dates can be easily confused because their format  differs throughout the world; thus, recorded dates should be formatted consistently and in an unambiguous manner. Security for electronic records should include password protection and automatic time-outs on computers and online databases, as well as scheduled backups for all data. Large collections should have electronic records backed up daily on a network or remote secure server, whereas small collections might consider doing local backups on a weekly basis.
+Genetic sample data can be recorded as part of an institutional database, which potentially tracks both the original  voucher  specimen and any subsequent associated genetic or genomic  derivatives, or a stand-alone tracking system that is used only for genetic samples (see [[#Databasing for genetic samples|INVENTORY CONTROL AND DATA MANAGEMENT: Databasing for genetic samples]]). Documentation of genetic  sample  locations in cold-storage units should be as precise as possible so that samples can be located quickly (see [[#Sample labeling and tracking|INVENTORY CONTROL AND DATA MANAGEMENT: Sample labeling and tracking]]). Dates can be easily confused because their format differs throughout the world; thus, recorded dates should be formatted consistently and in an unambiguous manner. Security for electronic records should include password protection and automatic time-outs on computers and online databases, as well as scheduled backups for all data. Large collections should have electronic records backed up daily on a network or remote secure server, whereas small collections might consider doing local backups on a weekly basis.
 <Br>
 ===Emergency procedures===
-Collections  should  have emergency procedures, including evacuation procedures and detailed disaster plans, outlined in their SOP to address how personnel should respond to various situations, ranging from laboratory incidents to natural  disasters (ICOM  1993, Dorge and Jones 1999). Generally, emergency procedures and disaster preparedness should be developed to address incidents at various levels of involvement, including issues confined to the genetic collection (e.g., clean-up of chemical spills, transfer of genetic samples from a failed  cold-storage unit), building-wide or institution-wide events (e.g., flood  or  water damage as a result  of plumbing issue or roofing leak), local issues (e.g., city-wide  power  outage), or  regional  events (e.g., earthquake, hurricane, tornado, tsunami). Because emergencies with genetic resources can become disasters if immediate action is not taken, it is recommended that a risk assessment is conducted and personnel have regular reviews and drills to ensure their familiarity with emergency procedures and backup plans for every conceivable situation (see FACILITY  MANAGEMENT: Backup Precautions). It is also essential that personnel are familiar with the locations of all equipment  and tools needed to quickly and efficiently perform their responsibilities during each type of emergency, ranging  from  how  and where to transfer samples from a failed unit to how to turn on backup power during a power outage. Contact information for personnel responsible in case of emergency in the order that they should be contacted, facilities managers, and outside contacts for emergencies  (e.g., power companies, fuel supply companies, important contractors) should be included in the SOP document, provided to those responding to off-site alarms, and clearly posted in the collection. Contact information should be regularly reviewed to ensure that it remains current.
+Collections  should  have emergency procedures, including evacuation procedures and detailed disaster plans, outlined in their SOP to address how personnel should respond to various situations, ranging from laboratory incidents to natural  disasters<ref>[ICOM] International Council of Museums. 1993. Guidelines for Disaster Preparedness in Museums. http://icom.museum/fileadmin/user_upload/pdf/Guidelines/guidelinesdisasters_eng.pdf (1 January 2014). (Off-print from Museums Security and Protection: A Handbook for Cultural Heritage Institutions [D. Listen, ed.] ICOM in conjunction with Routledge, London, New York. 319 pp.)</ref> <ref>Dorge, V. and S.L. Jones. 1999. Building an Emergency Plan: A Guide for Museums and Other Cultural Institutions. Getty Conservation Institute, Los Angeles. 272 pp.</ref>. Generally, emergency procedures and disaster preparedness should be developed to address incidents at various levels of involvement, including:
+*Issues confined to the genetic collection (e.g., clean-up of chemical spills, transfer of genetic samples from a failed  cold-storage unit)
+*Building-wide or institution-wide events (e.g., flood  or  water damage as a result  of plumbing issue or roofing leak)
+*Local issues (e.g., city-wide  power  outage)
+*Regional  events (e.g., earthquake, hurricane, tornado, tsunami)
+Because emergencies with genetic resources can become disasters if immediate action is not taken, it is recommended that a risk assessment is conducted and personnel have regular reviews and drills to ensure their familiarity with emergency procedures and backup plans for every conceivable situation (see [[#Backup precautions|FACILITY MANAGEMENT: Backup precautions]]). It is also essential that personnel are familiar with the locations of all equipment and tools needed to quickly and efficiently perform their responsibilities during each type of emergency, ranging from how and where to transfer samples from a failed unit to how to turn on backup power during a power outage. Contact information for personnel responsible in case of emergency in the order that they should be contacted, facilities managers, and outside contacts for emergencies  (e.g., power companies, fuel supply companies, important contractors) should be included in the SOP document, provided to those responding to off-site alarms, and clearly posted in the collection. Contact information should be regularly reviewed to ensure that it remains current.
-==Genetic Sampling Processing==
+==Genetic Sample Processing==
 Genetic samples require specialized storage to maintain their viability, but the manner by which they are initially preserved when collected and any subsequent changes made prior to their deposition in a collection also greatly affects their utility in research.  In addition, procedures used by collection personnel to prepare the samples for deposition in long-term storage can have detrimental consequences if not completed  properly.
 <br>
 ===Initial preservation procedures===
-The methods currently used to preserve genetic material  during initial sampling vary widely owing to the sampling location, tissue type, and intended research use (Dessauer and Hafner 1984, Prendini et al. 2002, Bus´ and Allen 2014). A comprehensive treatise of methods to preserve genetic samples is discussed in Nagy  (2010). Of all the methods examined, flash-freezing  using liquid nitrogen or a mixture of dry ice and ethanol is considered  to be the one of the best ways to preserve samples because the speed by which the sample is frozen prevents large ice crystals from forming and no preservative is needed,  which maximizes the research potential of the sample. Some chemical agents or buffers (e.g., glycerol, dimethyl sulfoxide [DMSO]) are used to protect macromolecules and/or tissue integrity from damage caused by ice formation during cryopreservation techniques, such as freeze–thaw procedures or vitrification  (Withers  1980, Karlsson and  Toner  1996). Buffers, chemical preservatives, and alcohols, especially ethanol, do not require immediate refrigeration and are frequently used for the initial preservation of samples because it circumvents the complicated logistics involved with flash-freezing  samples in the field or keeping them cold during transport. All preservation techniques have caveats to their use, however, and genetic resource collections must be fully aware of both the benefits and limitations to make informed  decisions.
+The methods currently used to preserve genetic material  during initial sampling vary widely owing to the sampling location, tissue type, and intended research use. A comprehensive treatise of methods to preserve genetic samples is discussed in Nagy (2010)<ref name=Nagy2010>Nagy, Z.T. 2010. A hands-on overview of tissue preservation methods for molecular genetic analyses. Organisms Diversity & Evolution 10:91–105.</ref>. Of all the methods examined, flash-freezing  using liquid nitrogen or a mixture of dry ice and ethanol is considered  to be the one of the best ways to preserve samples because the speed by which the sample is frozen prevents large ice crystals from forming and no preservative is needed, which maximizes the research potential of the sample. Some chemical agents or buffers (e.g., glycerol, dimethyl sulfoxide [DMSO]) are used to protect macromolecules and/or tissue integrity from damage caused by ice formation during cryopreservation techniques. Buffers, chemical preservatives, and alcohols, especially ethanol, do not require immediate refrigeration and are frequently used for the initial preservation of samples because it circumvents the complicated logistics involved with flash-freezing samples in the field or keeping them cold during transport. All preservation techniques have caveats to their use, however, and genetic resource collections must be fully aware of both the benefits and limitations to make informed  decisions.
 <Br>
 <Br>
-In a recent survey of genetic resource collections associated with natural history museums, samples were found  to  be initially  preserved  in a variety of different ways (Zimkus and Ford 2014). The majority of collections surveyed included samples that were flash-frozen or preserved with ≥ 95% ethanol. Ethanol at concentrations of 95% to 99% is commonly used by researchers in the collection of zoological samples but is generally not used for the preservation of plant material.  Ethanol  can be considered expensive when compared to alternative preservatives and can be difficult to transport, especially at high concentrations, because of its flammable classification  (Williams  2007). A number of buffers and chemical preservatives are currently being used by natural  history researchers, including DMSO, RNAlaterH (Ambion, Austin, TX), and various lysis buffers. DMSO is used as a preservative in many different aqueous solutions. One of the most commonly used formulations is a salt-saturated solution of DMSO (20% DMSO, 0.25 M ethylenedi- aminetetraacetic acid [EDTA], sodium chloride [NaCl] saturated, pH 7.5; Seutin et al. 1991, Nagy  2010), which is a  cost-effective method for preserving and transporting genetic samples  from remote locations, but the long-term effects on sample quality are still unknown (Williams 2007). RNAlaterH solution and a similar product, AllprotectH Tissue Reagent (Qiagen, Valencia, CA),  are  used in sample  collecting for  the  stabilization of DNA, RNA, and  protein in tissues.  Although these solutions  minimize  the  need  to immediately process and/or  freeze tissue samples, material preserved in RNAlaterH and AllprotectH buffers cannot be stored at room temperature indefinitely if genetic samples are to remain viable.  Procedures using  lysis  buffers  to  preserve  samples  are  relatively inexpensive and can be used to yield high-molecular-weight DNA.  Queen’s lysis buffer is most often used for the preservation of DNA in nonmammalian vertebrates that possess nucleated red blood cells (Seutin et al. 1991, Nagy 2010). Although lysis buffers might not require immediate refrigeration, this type of preservation limits the ultimate  use of the sample because proteins are denatured and RNA is not preserved (Longmire  et al. 1997, Nagy 2010).
+[[File:Zimkus Ford Fig 2.tif|thumb|right|Methods and preservatives used in the initial preservation of genetic samples in surveyed collections<ref name=ZimkusFord2014/>. Responses in the “Other (F)” category included lysis buffers, buccal swabs, silica gel dessicants, and FTA paper®.]] In a recent survey of genetic resource collections associated with natural history museums, samples were found  to  be initially preserved  in a variety of different ways <ref name=ZimkusFord2014/>:
-<Br>
+*Flash-frozen
-<Br>
+*Preserved with ≥ 95% ethanol (zoological samples)
-Other sample preservation techniques that do not require the immediate cold storage of samples are available but are used  less frequently among natural history museums (Zimkus and Ford 2014). These techniques are not recommended for the preservation of samples used in genome-level sequencing (Wong et al. 2012). Buccal swabs are used to collect cells from the inside of the mouth and, more recently, skin swabs are being used to nondestructively sample amphibians to test for the presence of Batrachochytrium dendrobatidis, a disease-causing  fungus commonly known as chytrid (Boyle et al. 2004). Swabs can generally be kept at room temperature (if not exposed to extreme temperatures or direct sunlight) for approximately 1 week before they need to be placed in a freezer for long-term storage. Whatman FTAH (GE Healthcare Bio-Sciences, Pittsburgh, PA) is filter paper impregnated  with a proprietary mix of chemicals, which serve to lyse cells, prevent growth of bacteria, and protect  the DNA in the sample. This product allows for the collection and storage  of blood, cells from buccal swabs, and other  tissues, such as blood,  tissue, or saliva, by direct application of the biological sample onto  the  paper (Smith and Burgoyne 2004). DNA samples collected using FTA paper do not require immediate refrigeration because samples purportedly remain viable for at least 4 years at room  temperature. Manufacturers of this technology also report  that it allows for the collection of biological samples needed for RNA  analyses, but samples for this type of analysis are more sensitive and thus must be immediately placed in cold storage for long-term preservation. This  technique is convenient for the collection of DNA samples because of the small size of  the  collecting  product   and  no  need  for immediate cold storage, allowing ease of transport by a carrier or in personal  baggage.
+*Buffers and chemical preservatives
+::- DMSO (in many different aqueous solutions; one of the most commonly used formulations is a salt-saturated solution of DMSO (20% DMSO, 0.25 M ethylenedi- aminetetraacetic acid [EDTA], sodium chloride [NaCl] saturated, pH 7.5<ref name=Nagy2010/>)
+::- RNAlater (Ambion, Austin, TX)
+::- Allprotect Tissue Reagent
+::- Lysis buffers
+*Buccal swabs
+*Whatman FTA (GE Healthcare Bio-Sciences, Pittsburgh, PA) filter paper
 <br>
-<Br>
+Desiccation methods, commonly used to preserve botanical samples, use either physical processes or chemical agents to dehydrate samples. These methods can be very effective in preserving samples if they are maintained in a humidity-controlled environment after the desiccation process. Physical processes that lead to desiccation include:
-Desiccation methods, commonly used to preserve botanical samples, use either physical processes or chemical agents to dehydrate samples. These methods can be very effective in preserving samples if they are maintained in a humidity-controlled environment after the desiccation process. Physical processes that lead to desiccation include  sun-drying,  air-drying,  flash-drying, oven-drying, vacuum-drying, and freeze- drying, whereas substances that induce natural  desiccation include rice, sodium chloride (NaCl), calcium sulphate (CaSO4, commonly known as drierite; Liston et al. 1990, Nagy 2010), and  sodium silicate (obtainable in powder, crystal or gel form; Chase  and  Hills 1991). Freeze-drying (lyophilization  or cryodesiccation) is the controllable dehydration of samples by vacuum desiccation. This method involves the conversion of water within the sample into ice, crystallization of the sample, sublimation of ice under  a vacuum, and subsequent  evaporation of remaining water from the crystallized sample (Adams 2007). Silica  gel beads are commonly  used  by botanical collectors as a desiccant with the advantage that whole samples can be stored at room temperature as long as the material is stored in tightly  sealed containers and are regularly checked for dryness (Chase and Hills 1991); recent studies demonstrate that samples stored in containers with poor seals yield lower-quality DNA (Neubig et al. 2014). In addition,  comparisons of frozen DNA extracts stored for 7 to 12 years and new extracts of the same original silica-dried tissues indicate slightly less degradation is present in the frozen DNA extracts. Chemical desiccation, which involves adding a chemical to extract moisture from samples, can be completed using a number of different substances, including amyl acetate, hexamethyl- disilazane, xylene (which is the chemical Dimethylbenzene), methyl cellosolve/cellusolve (also known as ethylene glycol monomethyl ether), calcium oxide (CaO, commonly called lime), and sulphuric acid (H2SO4). Each of these chemical  methods has certain considerations for the  samples and personnel that should  be closely examined before working with them (Nagy  2010). Regardless of the method of desiccation, moisture content must be continuously controlled or samples quickly degrade. In addition, samples preserved in this manner are more sensitive to thermal decay at higher temperatures due to their reduced water content and should be stored in a low-temperature environment as soon as possible to ensure that samples remainviable.
+*Sun-drying
+*Air-drying
+*Flash-drying
+*Oven-drying
+*Vacuum-drying
+*Freeze- drying
+Substances that induce natural desiccation include:
+*Rice
+*Sodium chloride (NaCl)
+*Calcium sulphate (CaSO4, commonly known as drierite<ref name=Nagy2010/>)
+*Sodium silicate (obtainable in powder, crystal or gel form).
+Freeze-drying (lyophilization  or cryodesiccation) is the controllable dehydration of samples by vacuum desiccation. This method involves the conversion of water within the sample into ice, crystallization of the sample, sublimation of ice under  a vacuum, and subsequent  evaporation of remaining water from the crystallized sample<ref>Adams, G. 2007. The principles of freeze-drying. Methods in Molecular Biology 368:15–38.</ref>. Silica  gel beads are commonly  used by botanical collectors as a desiccant with the advantage that whole samples can be stored at room temperature as long as the material is stored in tightly  sealed containers and are regularly checked for dryness<ref>Chase, M.W. and H.G. Hills. 1991. Silica gel: An ideal material for field preservation of leaf samples for DNA studies. Taxon 40:215–220.</ref>.
+Chemical desiccation, which involves adding a chemical to extract moisture from samples, can be completed using a number of different substances, including:
+*Amyl acetate
+*Hexamethyl-disilazane
+*Xylene (which is the chemical Dimethylbenzene),
+*Methyl cellosolve/cellusolve (also known as ethylene glycol monomethyl ether)
+*Calcium oxide (CaO, commonly called lime)
+*Sulphuric acid (H<sub>2</sub>SO<sub>4</sub>)
+Each of these chemical methods has certain considerations for the samples and personnel that should  be closely examined before working with them<ref>Nagy, Z.T. 2010. A hands-on overview of tissue preservation methods for molecular genetic analyses. Organisms Diversity & Evolution 10:91–105.</ref>). Regardless of the method of desiccation, moisture content must be continuously controlled or samples quickly degrade. In addition, samples preserved in this manner are more sensitive to thermal decay at higher temperatures due to their reduced water content and should be stored in a low-temperature environment as soon as possible to ensure that samples remainviable.
 <br>
 <Br>
-Collection staff often does not have control of how genetic samples are originally preserved, and most genetic resource collections associated with natural history museums accept samples that are preserved using numerous different methods  (Zimkus and Ford 2014). As more information is discovered about preservation  methods themselves, it is becoming more important to know how samples were preserved and handled. Collection managers should make every effort to record the initial preservation  methods used and any subsequent changes to storage for their samples, including media or containers.  Both media and temperature can affect the ways that samples can be used for future molecular analysis; thus, all curation data  for genetic samples should be made available to researchers before their selection and use. Research advancements are constant in molecular studies, and future technological developments might allow for the stabilization and storage of biological samples at room temperature, which could eventually  eliminate  the need for low-temperature storage environments for newly collected samples. To determine if these new emerging technologies will be effective for existing genetic collections, the detailed curation history regarding how each individual sample was preserved, stored, and utilized will become increasingly important.
+Collection staff often does not have control of how genetic samples are originally preserved, and most genetic resource collections associated with natural history museums accept samples that are preserved using numerous different methods<ref name=ZimkusFord2014/>. As more information is discovered about preservation methods themselves, it is becoming more important to know how samples were preserved and handled. Collection managers should make every effort to record the initial preservation  methods used and any subsequent changes to storage for their samples, including media or containers.  Both media and temperature can affect the ways that samples can be used for future molecular analysis; thus, all curation data  for genetic samples should be made available to researchers before their selection and use. Research advancements are constant in molecular studies, and future technological developments might allow for the stabilization and storage of biological samples at room temperature, which could eventually  eliminate  the need for low-temperature storage environments for newly collected samples. To determine if these new emerging technologies will be effective for existing genetic collections, the detailed curation history regarding how each individual sample was preserved, stored, and utilized will become increasingly important.
 ===Storage containers===
-Genetic  resources can be stored in a variety of ways, depending
+Genetic  resources can be stored in a variety of ways, depending on the tissue type, sample size, and cold-storage  methods  used in a collection.  Primary storage containers of the samples themselves can include plastic bags, paper envelopes, reaction   plates, or  vials.  When  primary   storage   containers   are  accessioned  into  a collection, they must be examined to determine if they are appropriate for the type of cold storage being used in the collection. The SOP should clearly define acceptable storage containers  and  encourage  their in-house  researchers  to use them because any variation could involve material  and staff costs to rectify. For all types of cold storage,  the most commonly  used  sizes  of  vials  are  between  1.2  and  2.0  ml,  which  is  the  size  and configuration that  maximizes storage capacity while retaining  ease of handling <ref name=ZimkusFord2014/>.
-on the tissue type, sample size, and cold-storage  methods  used in a collection.  Primary storage containers of the samples themselves can include plastic bags, paper envelopes, reaction   plates, or  vials.  When  primary   storage   containers   are  accessioned  into  a collection, they must be examined to determine if they are appropriate for the type of cold storage being used in the collection. The SOP should clearly define acceptable storage containers  and  encourage  their in-house  researchers  to use them because any variation could involve material  and staff costs to rectify. For  all types of cold storage,  the most commonly   used  sizes  of  vials  are  between  1.2  and  2.0  ml,  which  is  the  size  and configuration that  maximizes storage  capacity while retaining  ease of handling  (Zimkus and  Ford  2014). Some additional features  that  might  be useful to  those  working  with sample vials include self-standing  vials (flat-bottom or skirted) and those that  allow for locking into a rack for one-handed operation.
 <br>
 <Br>
-One area of immense variability is with the number of vial types used in natural  history collections   (Zimkus   and   Ford   2014).  Potential   vial  issues  are  the  same  for  both mechanical  freezers and  cryovats,  although  more extreme for cryovats  because of their colder  temperatures and  quicker  temperature change.  Samples  stored  using LN2  must have vials that are rated for use with cryogenic temperatures, preferably made of polypropylene  with screw-top  caps. Glass vials are problematic  when frozen because of their fragility when handling  and vulnerability  to cracking  when stressed, and their use with LN2 is unacceptable because leakage into the vials can lead to the vessels exploding. In addition,  pop-off lids are not recommended  because this vial type can easily open on its own. Vials can have threads  located internally or externally on the vial opening; both vial types exhibit advantages  and  disadvantages. Externally-threaded closures promote more sterile conditions  because internal  threading  can allow contaminants to enter if the cap is placed on an unclean surface when removed,  but these vials can be susceptible to cracks  and  loss  of  air-tightness,   which  can  lead  to  sample  dessication  or  oxidation (Corthals   and  DeSalle  2005,  Corthals   2006).  Internally-threaded  vials  might  allow increased  storage  capacity,  depending  on  the  vial selected, but  users also suggest that material can be trapped  within the threads of this vial type (Johnson  1999). Some manufacturers  suggest  that   vial  caps  that   incorporate  a  silicone  gasket  or  O-ring (internally or externally threaded)  are ideal for vapor-phase  LN2 freezing because the seal is enhanced,  but care must be taken  if the vial cap is over-tightened  because the gasket can become distended.  In addition,  the presence of gaskets or O-ring might improve the initial performance of seals but can be problematic  when used with some alcohols  (e.g., ethanol)   because  some  gasket  material,  such  as  silicone,  is  vapor  permeable.  When working with liquid-phase  nitrogen cold storage, extra caution must be taken because the accidental entrapment of liquefied nitrogen  inside the vial leads to pressure build up and, upon  removal,  rapid  vaporization of the liquid can result in leakage or even explosion (see HEALTH AND   SAFETY:  Liquid Nitrogen Safety).  As a precaution, vial manufacturers recommend   that   samples   not   be   immersed   in   LN2    unless   they   have   secondary containment. Heat-sealing  vials into  flexible polyethylene  tubing  is recommended  for safe storage  in the liquid-phase  environment.
+One area of immense variability is with the number of vial types used in natural history collections <ref name=ZimkusFord2014/>. Potential vial issues are the same for both mechanical  freezers and  cryovats,  although  more extreme for cryovats  because of their colder temperatures and quicker temperature change.  Samples  stored using LN<sub>2</sub>  must have vials that are rated for use with cryogenic temperatures, which are most often made of polypropylene and include screw-top caps. Some additional useful information about vials include:
-Depending   on  the  size  of  the  samples  and  their  primary   storage  method   in  the collection,  various  secondary  and  tertiary   storage  containers   (e.g.,  boxes,  cassettes, sample storage canes for immersion in LN2,  racks) can be used to organize samples and maximize space. The majority  of natural  history  museums  recently surveyed organizes their collections with a vial box and rack system (Zimkus and Ford  2014). The box-and- rack system is a simple but effective way to maximize space within a cold-storage  unit and reduce the amount  of time needed to search for a specific box. The overall cost of box-and-rack systems depends on the style and number of both the boxes and racks purchased.   The  use  of  racks  also  decreases  potential   risks  to  the  collection  when personnel  are retrieving samples. Collections  without  racks often stack boxes on top of one another  within cold-storage  units, forcing personnel  to remove or displace boxes to access those  underneath or behind.  In addition, the movement  of individual  boxes to retrieve samples requires more time, increases the possibility that samples will thaw, and decreases the chance that  boxes will be put back in their original location.  Lastly, racks allow samples to be quickly moved to other freezers in the event of a freezer failure and decrease  the  possibility  that   samples  are  misplaced   while  in  a  temporary  storage location.
+[[File:Zimkus Ford Fig 3.tif|thumb|right|Vials used during initial collection (dark grey) and final storage (light grey) of genetic samples in surveyed collections<ref name=ZimkusFord2014/>. Variation in the types of vials included location of the threads internally or externally on the vial opening, and vials caps with or without gaskets.]]
+*Glass vials are not recommended because of their fragility when handling and vulnerability to cracking  when stressed.
+*Microcentrifuge vials with pop-off lids are not recommended because liquid nitrogen can enter them and cause them to open or explode.
+*Self-standing vials (flat-bottom or skirted) may be useful to curatorial staff.
+*Vials that allow for locking into a rack for one-handed operation may allow curatorial staff to process samples more quickly.
+*Vials can have threads located internally or externally on the vial opening.
+::-  Externally-threaded closures promote more sterile conditions because internal threading can allow contaminants to enter if the cap is placed on an unclean surface when removed.
+:: - Externally-threaded vials can be susceptible to cracks  and  loss  of  air-tightness,  which  can  lead  to  sample  dessication  or  oxidation <ref>Corthals, A. 2006. The Ambrose Monell Cryo-Collection: A museum-based molecular collection. Pp. 107–113 in DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice and Uses (V. Savolainen, M.P. Powell, K. Davis, G. Reeves, and A. Corthals, eds.). Kew Publishing, Royal Botanic Garden, Kew,England. 151 pp.</ref><ref>Corthals, A. and R. DeSalle. 2005. An application of tissue and DNA banking for genomics and conservation: The Ambrose Monell Cryo-Collection (AMCC). Systematic Biology 54:819–823.</ref>.
+::- Internally-threaded  vials  might  allow increased  storage  capacity,  depending  on  the  vial selected, but  users also suggest that material can be trapped within the threads of this vial type<ref>Johnson, B. 1999. Frozen in time: Ultra low freezers, dewars, and tubes. The Scientist 13(1):19.</ref>.
+*Some manufacturers  suggest  that  vial  caps that  incorporate  a  silicone  gasket  or  O-ring (internally or externally threaded)  are ideal for vapor-phase  LN<sub>2</sub> freezing because the seal is enhanced,  but care must be taken  if the vial cap is over-tightened  because the gasket can become distended.  In addition,  the presence of gaskets or O-ring might improve the initial performance of seals but can be problematic when used with some alcohols  (e.g., ethanol)  because  some  gasket  material, such  as  silicone,  is  vapor  permeable.
+*Vial manufacturers recommend that  samples  not  be  immersed   in   LN<sub>2</sub>   unless   they   have   secondary containment because the accidental entrapment of liquefied nitrogen inside the vial leads to pressure build up and, upon removal,  rapid  vaporization of the liquid can result in leakage or even explosion (see [[#Liquid nitrogen safety|HEALTH AND SAFETY:  Liquid nitrogen safety]]). Heat-sealing  vials into  flexible polyethylene  tubing  is recommended  for safe storage  in the liquid-phase  environment.
 <br>
 <Br>
-Racks  systems made from aluminum  or stainless steel can house most standard-sized boxes and can be oriented horizontally  or vertically to fit in mechanical upright  or chest freezers, as well as LN2 cryovats. Aluminum might be chosen for racks in collections that need  precise  and  controlled  freezing of samples  because  this  metal  is a better  energy conductor than  stainless  steel. Stainless  steel racks  are more  durable  and,  because  the steel does not oxidize, they remain clean. Racks most often come with a locking rod that runs through  the front of the shelves, ensuring that boxes are held in place when the rack is moved. Racks also can have spring clips instead of locking rods, which allow quicker access to boxes, but can be problematic  if the racks are bumped  or dropped.  Identifiers can  be  added  by  riveting  or  etching  onto  racks,  or  by  labels  (e.g.,  unique  locating identifiers,  barcodes)  that  can  be  affixed  to  the  tops  of  racks  and  rack  shelves (see INVENTORY CONTROL AND   DATA MANAGEMENT: Sample Labeling and Tracking).
+Depending   on  the  size  of  the  samples  and  their  primary   storage  method   in  the collection,  various  secondary  and  tertiary   storage  containers   (e.g.,  boxes,  cassettes, sample storage canes for immersion in LN<sub>2</sub>,  racks) can be used to organize samples and maximize space. The majority  of natural  history  museums  recently surveyed organizes their collections with a vial box and rack system<ref name=ZimkusFord2014/>. The box-and-rack system is a simple but effective way to maximize space within a cold-storage unit and reduce the amount  of time needed to search for a specific box. The overall cost of box-and-rack systems depends on the style and number of both the boxes and racks purchased. The  use  of  racks  also  decreases  potential   risks  to  the  collection  when personnel  are retrieving samples. Collections  without  racks often stack boxes on top of one another  within cold-storage  units, forcing personnel  to remove or displace boxes to access those  underneath or behind.  In addition, the movement  of individual  boxes to retrieve samples requires more time, increases the possibility that samples will thaw, and decreases the chance that  boxes will be put back in their original location.  Lastly, racks allow samples to be quickly moved to other freezers in the event of a freezer failure and decrease  the  possibility  that   samples  are  misplaced   while  in  a  temporary  storage location.
-A number  of different  types  of vial storage  boxes can  be used,  such as cardboard, chipboard (paperboard), fiberboard, metal, polycarbonate, or polypropylene. It is recommended   that  moisture-proof boxes  be  used  even though  they  are  more  costly, because  water  repellency  increases  their  long-term  durability.   When  purchasing   new boxes, care should be taken to ensure that they are compatible with both the existing rack system and the cold-storage equipment. Collection managers should be aware that polypropylene  boxes with hinged lids, which are often used in the field because they are shatter-resistant and have attached  lids, might not fit in standard-sized racks. In addition, personnel  in collections  using either  the  liquid  or  vapor  phase  of nitrogen  should  use boxes with holes or slots present on the underside  of the box to allow the LN2 to drain. Collections using cryovats should confirm that particles of cardboard, chipboard (paperboard), or  fiberboard will not  prevent  equipment  from  functioning  properly  if boxes begin to degrade; otherwise, a more durable type of box should be used. Aspects of ordinary   use  are  another   important  consideration for  storage  boxes  in  a  collection. Collection  managers  should  be aware  that  boxes that  have numbered,  gridded  inserts inside might be difficult to read after being removed from cold temperatures because of frost. In contrast, boxes with grid numbering  present on the lid, rather than the box itself, can have frost easily wiped off; however, finding the correct vial may be difficult once the lid is removed  because care must  be taken  to keep the lid numbering  aligned with the internal  grid.
+<br>
+<Br>
+Racks  systems made from aluminum  or stainless steel can house most standard-sized boxes and can be oriented horizontally  or vertically to fit in mechanical upright  or chest freezers, as well as LN<sub>2</sub> cryovats. Aluminum might be chosen for racks in collections that need  precise  and  controlled  freezing of samples  because  this  metal  is a better  energy conductor than  stainless  steel. Stainless  steel racks  are more  durable  and,  because  the steel does not oxidize, they remain clean. Racks most often come with a locking rod that runs through  the front of the shelves, ensuring that boxes are held in place when the rack is moved. Racks also can have spring clips instead of locking rods, which allow quicker access to boxes, but can be problematic  if the racks are bumped  or dropped.  Identifiers can  be  added  by  riveting  or  etching  onto  racks,  or  by  labels  (e.g.,  unique  locating identifiers,  barcodes)  that  can  be  affixed  to  the  tops  of  racks  and  rack  shelves (see [[#Sample labeling and tracking|INVENTORY CONTROL AND  DATA MANAGEMENT: Sample labeling and tracking]]).
+<br>
+<Br>
+A number  of different  types  of vial storage  boxes can  be used,  such as cardboard, chipboard (paperboard), fiberboard, metal, polycarbonate, or polypropylene. It is recommended   that  moisture-proof boxes  be  used  even though  they  are  more  costly, because  water  repellency  increases  their  long-term  durability.   When  purchasing  new boxes, care should be taken to ensure that they are compatible with both the existing rack system and the cold-storage equipment. Collection managers should be aware that polypropylene  boxes with hinged lids, which are often used in the field because they are shatter-resistant and have attached  lids, might not fit in standard-sized racks. In addition, personnel  in collections  using either the liquid or vapor  phase  of nitrogen  should  use boxes with holes or slots present on the underside  of the box to allow the LN<sub>2</sub> to drain. Collections using cryovats should confirm that particles of cardboard, chipboard (paperboard), or  fiberboard will not  prevent  equipment  from  functioning  properly  if boxes begin to degrade; otherwise, a more durable type of box should be used. Aspects of ordinary   use  are  another  important  consideration for  storage  boxes  in  a  collection. Collection  managers  should  be aware  that  boxes that  have numbered,  gridded  inserts inside might be difficult to read after being removed from cold temperatures because of frost. In contrast, boxes with grid numbering  present on the lid, rather than the box itself, can have frost easily wiped off; however, finding the correct vial may be difficult once the lid is removed  because care must  be taken  to keep the lid numbering  aligned with the internal  grid.
 <br>
-===Sample Transfer===
+===Sample transfer===
-When samples are received by collection staff, they might need to be transferred into new primary storage containers,  especially if they are stored in a manner that is incompatible with the cold-storage system or if initially preserved in sub-optimal conditions for long-term storage (e.g., preservatives need to be removed; Williams 2007). Collection personnel should ensure that contact between different specimens is avoided and all instruments used in the tissue transfer process are handled in such a way that ensures that biological contaminants are destroyed. Disposable equipment (e.g., single-use  blades, disposable forceps) replaced  after on  use greatly reduces the chances of sample contamination, but this practice can become too costly for many collections. Several methods (e.g., heat/flame, chemical agents, steam sterilization in an autoclave) can be used to prevent contamination between genetic samples, but collection managers must be sure that their particular procedures denature or destroy all contaminating genetic material. Some practices, such as cleaning instruments  using detergent and water, render instruments  and surfaces safe to touch, but these methods do not protect samples from cross-contamination. Disinfection of work surfaces, decontamination of equipment, and sterilization procedures are all needed to ensure safe operations for both staff and genetic samples, and these techniques can vary depending on the task at hand.
+When samples are received by collection staff, they might need to be transferred into new primary storage containers, especially if they are stored in a manner that is incompatible with the cold-storage system or if initially preserved in sub-optimal conditions for long-term storage (e.g., preservatives need to be removed). Collection personnel should ensure that contact between different specimens is avoided and all instruments used in the tissue transfer process are handled in such a way that ensures that biological contaminants are destroyed. Disposable equipment (e.g., single-use  blades, disposable forceps) replaced  after on  use greatly reduces the chances of sample contamination, but this practice can become too costly for many collections. Several methods (e.g., heat/flame, chemical agents, steam sterilization in an autoclave) can be used to prevent contamination between genetic samples, but collection managers must be sure that their particular procedures denature or destroy all contaminating genetic material. Some practices, such as cleaning instruments using detergent and water, render instruments and surfaces safe to touch, but these methods do not protect samples from cross-contamination. Disinfection of work surfaces, decontamination of equipment, and sterilization procedures are all needed to ensure safe operations for both staff and genetic samples, and these techniques can vary depending on the task at hand.
 <br>
 <Br>
-Comprehensive procedures should clearly outline which handling methods are appropriate for the various tasks when working  with samples. Some techniques, such as autoclaving and use of UV light, destroy all biological matter but require a longer time to accomplish, and thus are better utilized before and after processing a batch of samples. Alternatively, other methods, such as heat/flame or hydrogen peroxide, could be used to immediately decontaminate subsampling tools and ensure no cross-contamination while working  through  a batch of samples, because ease and speed of use is important. If a chemical  agent such  as  hydrogen  peroxide  or  bleach is used to clean equipment or surfaces, procedures should ensure that those agents do not contaminate samples because these techniques destroy biological matter (e.g., dry instruments thoroughly before manipulating samples). Personnel should also be careful not to inadvertently contaminate the samples by touching their own body or clothes, or allowing hair to come in contact with samples. In addition, they should always wear the proper PPE to protect genetic samples and for their own personal safety (see HEALTH AND SAFETY: Personal Protective Equipment).
+Comprehensive procedures should clearly outline which handling methods are appropriate for the various tasks when working with samples. Some techniques, such as autoclaving and use of UV light, destroy all biological matter but require a longer time to accomplish, and thus are better utilized before and after processing a batch of samples. Alternatively, other methods, such as heat/flame or hydrogen peroxide, could be used to immediately decontaminate subsampling tools and ensure no cross-contamination while working  through  a batch of samples, because ease and speed of use is important. If a chemical  agent such  as  hydrogen  peroxide  or  bleach is used to clean equipment or surfaces, procedures should ensure that those agents do not contaminate samples because these techniques destroy biological matter (e.g., dry instruments thoroughly before manipulating samples). Personnel should also be careful not to inadvertently contaminate the samples by touching their own body or clothes, or allowing hair to come in contact with samples. In addition, they should always wear the proper PPE to protect genetic samples and for their own personal safety (see [[#Personal protective equipment|HEALTH AND SAFETY: Personal protective equipment]]).
 <br>
 ==Inventory Control and Data Management==
-The ability to find a specimen is essential for the curation of any natural history collection. The manner  by which the physical locations of genetic samples are tracked is particularly important in their curation because it is virtually impossible for personnel to search the entire collection if a particular sample is missing. In addition, proper inventory and data management allows collection managers to maximize the capacity of their cold- storage units while reducing the amount  of time needed to locate samples, which is crucial given that the quality of some genetic material can be reduced  with each freeze–thaw event; more research is needed to understand these effects on various sample types over both  short-term and  long-term  storage(Shikama 1965, Ross et al. 1990, Davis et al. 2000).
+The ability to find a specimen is essential for the curation of any natural history collection. The manner by which the physical locations of genetic samples are tracked is particularly important in their curation because it is virtually impossible for personnel to search the entire collection if a particular sample is missing. In addition, proper inventory and data management allows collection managers to maximize the capacity of their cold- storage units while reducing the amount of time needed to locate samples, which is crucial given that the quality of some genetic material can be reduced with each freeze–thaw event.
 <Br>
 ===Sample labeling and tracking===
-Proper sample tracking is key to ensuring that cold-storage equipment does not have to remain open for long periods, or samples are not repeatedly exposed to temperatures that initiate thawing. An appropriate tracking system could include  sample labeling, multiple levels of container labeling, and the use of a database to record sample location data.  Using a convention for numbering that assigns unique locating identifiers, such as barcodes, to all levels of sample storage  (including primary, secondary, and tertiary containers) allows for quick location and retrieval from a complex cold-storage  system (see GENETIC SAMPLE PROCESSING: Storage Containers). It is recommended that for maximum efficiency, sample vials stored within LN2 cryovats or mechanical freezers should have unique locating identifiers  assigned to the cryogenic vials, as well as unique locating identifiers assigned to the associated boxes, shelves within racks, racks in their entirety, and individual cold-storage units. Each sample vial can then be located in the collection by a unique location number combination. Any labels placed on vials or storage containers should be typewritten or computer-generated; hand-written identifiers might be difficult to read due to the handwriting  or decomposition of the ink as a result of cold temperatures or mechanical friction.  Upon arrival to a collection, samples might need further curation to meet collection standards, including the addition of typewritten or computer-generated labels to vials or the transfer of samples into the appropriate type of vials. Extreme care must be taken because most genetic samples are initially labeled using reference numbers  written on the vial by the researcher. All label placements should be tested under projected environmental conditions to ensure that ink, adhesive, and the label itself withstands the cold-storage temperatures. On secondary containers, such as boxes or racks, labels should be placed in areas where friction is minimal to reduce the risk that  the label face is worn down by repeated scratching or rubbing.
+Proper sample tracking is key to ensuring that cold-storage equipment does not have to remain open for long periods, or samples are not repeatedly exposed to temperatures that initiate thawing. An appropriate tracking system could include:
+*Sample labeling
+*Multiple levels of container labeling
+*Use of a database to record sample location data
+*Using a convention for numbering that assigns unique locating identifiers (e.g., barcodes) to all levels of sample storage (e.g., primary, secondary, and tertiary containers)
+It is recommended that for maximum efficiency, sample vials stored within LN<sub>2</sub> cryovats or mechanical freezers should have unique locating identifiers assigned to the cryogenic vials, as well as unique locating identifiers assigned to the associated boxes, shelves within racks, racks in their entirety, and individual cold-storage units. Each sample vial can then be located in the collection by a unique location number combination. Any labels placed on vials or storage containers should be typewritten or computer-generated; hand-written identifiers might be difficult to read due to the handwriting  or decomposition of the ink as a result of cold temperatures or mechanical friction.  Upon arrival to a collection, samples might need further curation to meet collection standards, including the addition of typewritten or computer-generated labels to vials or the transfer of samples into the appropriate type of vials. Extreme care must be taken because most genetic samples are initially labeled using reference numbers  written on the vial by the researcher. All label placements should be tested under projected environmental conditions to ensure that ink, adhesive, and the label itself withstands the cold-storage temperatures. On secondary containers, such as boxes or racks, labels should be placed in areas where friction is minimal to reduce the risk that  the label face is worn down by repeated scratching or rubbing.
 <Br>
-Barcodes labels rated for cryogenic conditions or vials manufactured with barcodes are commonly used by genetic resource   collections to facilitate sample tracking, including for primary and other hierarchies of containers  (Zimkus  and  Ford  2014). Preprinted or self-printed barcode labels that are mostly transparentand wrap completely around  vials, allow  information  hand-written on the vials to be viewed when positioned over the  writing.  Vials manufactured with barcodes  on  the side or bottom are less commonly used, most likely because these vials rarely have an area where researchers can  include hand-written information. Barcodes inserted into vial caps do facilitate  the barcoding process because they require less handling time when compared to vial-wrapping labels, but there are added risks that inserts could fall out or a cap  could become disassociated  from  the  vial itself. Radio frequency identification (RFID) tags transmit unique locating identifiers  associated  with tagged  objects and, unlike traditional barcodes, these tags do not need to be within the line of sight of the reader. RFID technology is currently being used only to track secondary and tertiary containers (e.g., boxes, racks) within the natural history community, but this method could potentially  be used to track  primary containers when the tag size and associated costs decrease (Zimkus  and  Ford  2014).
+Barcodes labels rated for cryogenic conditions or vials manufactured with barcodes are commonly used by genetic resource   collections to facilitate sample tracking, including for primary and other hierarchies of containers  <ref name=ZimkusFord2014/>. Preprinted or self-printed barcode labels that are mostly transparentand wrap completely around vials, allow  information hand-written on the vials to be viewed when positioned over the  writing.  Vials manufactured with barcodes on the side or bottom are less commonly used, most likely because these vials rarely have an area where researchers can  include hand-written information. Barcodes inserted into vial caps do facilitate  he barcoding process because they require less handling time when compared to vial-wrapping labels, but there are added risks that inserts could fall out or a cap  could become disassociated  from  the  vial itself. Radio frequency identification (RFID) tags transmit unique locating identifiers  associated  with tagged  objects and, unlike traditional barcodes, these tags do not need to be within the line of sight of the reader. RFID technology is currently being used only to track secondary and tertiary containers (e.g., boxes, racks) within the natural history community, but this method could potentially  be used to track  primary containers when the tag size and associated costs decrease <ref name=ZimkusFord2014/>.
 <Br>
 ===Databasing for genetic samples===
-By their  nature, genetic resource collections generate and track a large amount of data associated with their samples.  A computer-based inventory system, such as a stand-alone database, internal spreadsheet, or networked database, is essential so that all sample metadata, including location data and loan/gift sampling history, can be tracked (Cable and Fulcher  2006). The system should have the capacity to assign a unique identifier to each genetic sample entered in the database   and  associate all  erived genetic samplings and derivatives with the original specimen,  which  might be the original  genetic sample itself or a traditional voucher specimen. It is essential that a tissue sample or genetic extract can be readily linked to the traditional voucher specimen. Changes/updates to data, including taxonomic  identification, should  be  made  to all preparation types, even if data are tracked separately for the traditional voucher specimen and genetic sample, The chosen database should accommodate for museum-wide variables given that traditional voucher specimens are likely housed  apart  from  their  associated genetic samples due to their  different storage and conservation needs and, in addition,  personnel  curating these two collections are likely different.  Regardless of the chosen database, data standards are also critical to ensure that the format of the information, syntax and punctuation are consistent (Cable and Fulcher  2006, Miller  2014). Data  consistency allows databases  to function as research and curation tools when used in basic queries, enhances the exchange of data  among research and informatics partners, and facilitates the utilization of data with data  aggregators (e.g.,  Global  Biodiversity  Information Facility [GBIF], iDigBio, VertNet).
+By their  nature, genetic resource collections generate and track a large amount of data associated with their samples.  A computer-based inventory system, such as a stand-alone database, internal spreadsheet, or networked database, is essential so that all sample metadata can be tracked<ref> Cable, S. and T.K. Fulcher. 2006. Databasing and information technology. Pp. 61–65 in DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice and Uses (V. Savolainen, M.P. Powell, K. Davis, G. Reeves, and A. Corthals, eds.). Kew Publishing, Royal Botanic Garden, Kew, England. 151 pp.</ref>. The system should have the capacity to assign a unique identifier to each genetic sample entered in the database and associate all derived genetic samplings and derivatives with the original specimen, which  might be the original  genetic sample itself or a traditional voucher specimen. It is essential that a tissue sample or genetic extract can be readily linked to the traditional voucher specimen. Changes/updates to data, including taxonomic  identification, should  be  made  to all preparation types, even if data are tracked separately for the traditional voucher specimen and genetic sample, The chosen database should accommodate for museum-wide variables given that traditional voucher specimens are likely housed  apart  from  their  associated genetic samples due to their  different storage and conservation needs and, in addition,  personnel  curating these two collections are likely different.  Regardless of the chosen database, data standards are also critical to ensure that the format of the information, syntax and punctuation are consistent, allowing databases to function as research and curation tools when used in basic queries, enhances the exchange of data  among research and informatics partners, and facilitates the utilization of data with data  aggregators (e.g.,  Global  Biodiversity  Information Facility [GBIF], iDigBio, VertNet).
 <Br>
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-Those curating genetic resource collections associated with natural history museums are currently using a number of different platforms to track data, including free-access database  application systems developed for museums (e.g., Arctos, Specify), commercial database application systems (e.g., FileMaker Pro, Microsoft Access, FreezerProH), web delivery through data  aggregators (e.g., GBIF, HerpNET, ORNIS), and internally written applications (Zimkus and Ford 2014). All of the systems currently  being used have  benefits and drawbacks;  before selecting a system, collection managers should evaluate  the size of their genetic resource collection  and internal computing  resources, and  determine how to  integrate or  link  data associated with genetic samples and traditional voucher specimens. Free database application systems developed for natural history collections can easily associate specimen parts, but these systems might need to be customized to include  data   fields specific to genetic  samples, such as changes to preservation, freeze–thaw events, and remaining volume. Some commercial systems (e.g., KE  EMu) can accommodate genetic sample data, but some collection managers  might find annual  license fees too costly to maintain.  Also, some specialized systems (e.g., FreezerProH) can prioritize sample location  data, which is important for a larger genetic collection, but disassociates traditional voucher specimen data from genetic samples. The use of a web-based data aggregator (e.g., Global Genome Biodiversity Network [GGBN; Coddington et al. 2014], GBIF) can allow external users to access data, but an internal platform is still necessary to allow collection personnel to track genetic sample metadata. Internally written applications might seem ideal because they can be tailored, but they require personnel dedicated to their development and maintenance, and who have an understanding of how to build the system with the flexibility and scalability needed for data and metadata growth.
+Those curating genetic resource collections associated with natural history museums are currently using a number of different platforms to track data, including<ref name=ZimkusFord2014/>:
+*Free-access database application systems developed for museums (e.g., Arctos, Specify)
+*Commercial database application systems (e.g., FileMaker Pro, Microsoft Access, FreezerPro)
+*Web delivery through data  aggregators (e.g., GBIF, HerpNET, ORNIS)
+*Internally written applications
+All of the systems currently  being used have  benefits and drawbacks;  before selecting a system, collection managers should evaluate the size of their genetic resource collection and internal computing  resources, and determine how to integrate o  link  data associated with genetic samples and traditional voucher specimens. Free database application systems developed for natural history collections can easily associate specimen parts, but these systems might need to be customized to include  data  fields specific to genetic  samples, such as changes to preservation, freeze–thaw events, and remaining volume. Some commercial systems (e.g., KE  EMu) can accommodate genetic sample data, but some collection managers  might find annual  license fees too costly to maintain.  Also, some specialized systems (e.g., FreezerProH) can prioritize sample location  data, which is important for a larger genetic collection, but disassociates traditional voucher specimen data from genetic samples. The use of a web-based data aggregator (e.g., Global Genome Biodiversity Network [GGBN<ref>Coddington, J., K. Barker, G. Droege, J.J. Astrin, P. Bartels, C. Butler, D. Cantrill, F. Forest, B. Gemeinholzer, D. Hobern, J. Mackenzie-Dodds, E.O. Tuama, G. Petersen, O. Sanjur, D. Schindel, and O. Seberg. 2014. GGBN: Making genomic collections discoverable for research through a networked community of biodiversity repositories. Pp. 165–168 in DNA Banking for the 21st Century. Proceedings of the U.S. Workshop on DNA Banking (W.L. Applequist and L. Campbell, eds.). William L. Brown Center, St. Louis, Missouri. 187 pp.</ref>], GBIF) can allow external users to access data, but an internal platform is still necessary to allow collection personnel to track genetic sample metadata. Internally written applications might seem ideal because they can be tailored, but they require personnel dedicated to their development and maintenance, and who have an understanding of how to build the system with the flexibility and scalability needed for data and metadata growth.
 ==Use of Collections==
@@ Line 250: / Line 395: @@
 ===Loan policies===
-In the  context of natural history  museums, a loan is a temporary transfer  of a single specimen or lot of specimens, generally for research, for a specified period of time. Most loan policies for traditional natural history specimens are applicable to genetic samples  but, owing  to the consumptive nature of this resource and unique issues related to custodianship, clear policies should be developed in relation to the distribution of genetic samples. Baker and Hafner  (1984) suggested that the term ‘‘loan’’ be replaced with ‘‘gift’’ or ‘‘donation’’ when discussing transfer of genetic  samples between collections  and researchers because the specimens are not returned; however, Zimkus and Ford (2014) found that  some genetic collections do request unused samples to be sent back. Loan/gift policies should be explicit how custodianship issues, as well as permissions to approve the transfer of genetic material, are made, especially for institutions with a centralized repository.  Unlike traditional natural history specimens within an institution, genetic samples might be part of a voucher specimen that was accessioned by another collection before the sample itself was deposited in the genetic collection.
+In the  context of natural history  museums, a loan is a temporary transfer  of a single specimen or lot of specimens, generally for research, for a specified period of time. Most loan policies for traditional natural history specimens are applicable to genetic samples  but, owing  to the consumptive nature of this resource and unique issues related to custodianship, clear policies should be developed in relation to the distribution of genetic samples. Baker and Hafner  (1984) suggested that the term ‘‘loan’’ be replaced with ‘‘gift’’ or ‘‘donation’’ when discussing transfer of genetic  samples between collections  and researchers because the specimens are not returned; however, Zimkus and Ford (2014)<ref name=ZimkusFord2014/> found that  some genetic collections do request unused samples to be sent back. Loan/gift policies should be explicit how custodianship issues, as well as permissions to approve the transfer of genetic material, are made, especially for institutions with a centralized repository.  Unlike traditional natural history specimens within an institution, genetic samples might be part of a voucher specimen that was accessioned by another collection before the sample itself was deposited in the genetic collection.
 <br>
 <Br>
 Because genetic collections are consumptive, loan/gift policies should clearly outline the required information that should  be submitted in sample requests to justify that a material transfer is warranted. The following information is recommended for inclusion in loan/gift requests:
-* Objectives of the proposed research and its scientific merit;
+* Objectives of the proposed research and its scientific merit
-* Taxa and total number of genetic samples requested;
+* Taxa and total number of genetic samples requested
-* Experimental protocol to be employed;
+* Experimental protocol to be employed
-* Amount of genetic material requested per sample;
+* Amount of genetic material requested per sample
-* Desired  method of transport (e.g., room  temperature in preservative, frozen on dry
+* Desired  method of transport (e.g., room  temperature in preservative, frozen on dry ice)
-* ice); and
+* Plans for the dissemination of knowledge gained from the proposed research with the originating institution and scientific community, including:
-* Plans for the dissemination of knowledge gained from the proposed research with the originating institution and scientific community, including publications resulting from use of the samples and online publication of sequence data.
+::- Publications resulting from use of the samples
+::- Online publication of sequence data
 <br>
-Loan/gift policies should also clearly state the allowable use of genetic samples and associated metadata. Policies should  stipulate that loans/gifts may not  be transferred from  one institution to another without the written permission of the originating institution, ensuring that  material is used only for approved  purposes.  This also ensures that those receiving samples do not patent or otherwise profit from the use of specimens (as outlined in the Convention on Biological Diversity),  which could compromise any original collecting agreement with the country where the  specimens originated or any other entity that might have donated  material to the collection. Researchers might also be obliged to acknowledge the institution in all publications resulting from use of their loan/ gift material and make available citations or reprints of such publications.
+Loan/gift policies should also clearly state the allowable use of genetic samples and associated metadata. Policies should  stipulate that loans/gifts may not be transferred from one institution to another without the written permission of the originating institution. This also ensures that those receiving samples do not patent or otherwise profit from the use of specimens (as outlined in the Convention on Biological Diversity). Researchers might also be obliged to acknowledge the institution in all publications resulting from use of their loan/ gift material and make available citations or reprints of such publications.
 <Br>
 <Br>
-Loan/gift policies for genetic resources differ from those of other types of natural history specimens because genetic sequence data is generated from their consumptive use. The majority of genetic resource collections surveyed by Zimkus and Ford (2014) request that researchers submit genetic sequence data to a public genetic sequence database, such as NCBI GenBank (http://www.ncbi.nlm.nih.gov/). This requirement is important for consumable  collections because it ensures that sequence data is available to other researchers, unnecessary work is not duplicated, and originating institutions comply with granting  agreements to make data  accessible. Whenever possible, collections should link the end products of research (e.g., genetic sequences) captured in communal databases  to the original genetic samples and/or voucher specimen records found in the originating institution’s database. To ensure compliance, it is recommended that collection managers should follow up with researchers annually and consider loans/gifts ‘‘closed’’ only when all policy requirements  are met.
+Loan/gift policies for genetic resources differ from those of other types of natural history specimens because genetic sequence data is generated from their consumptive use. The majority of genetic resource collections surveyed request that researchers submit genetic sequence data to a public genetic sequence database, such as NCBI GenBank (http://www.ncbi.nlm.nih.gov/)<ref name=ZimkusFord2014/>. This requirement is important for consumable collections because it ensures that sequence data is available to other researchers, unnecessary work is not duplicated, and originating institutions comply with granting agreements to make data accessible. Whenever possible, collections should link the end products of research (e.g., genetic sequences) captured in communal databases to the original genetic samples and/or voucher specimen records found in the originating institution’s database. To ensure compliance, it is recommended that collection managers should follow up with researchers annually and consider loans/gifts ‘‘closed’’ only when all policy requirements are met.
 <Br>
 <Br>
-If the institution provides the appropriate amount  of material, the genetic samples loaned/gifted  should be completely consumed by the researcher (see USE OF  COLLECTIONS: Aliquoting Samples). If a portion  of a genetic sample remains unused  after the project, however, researchers might be unclear about what to do with the remaining samples. In a recent collection survey, institutions requested that researchers address leftover samples in various ways, including destroying the remaining samples, returning samples to the originating institution for destruction or reuse, or accessioning samples into the researcher’s personal or institutional collection (Zimkus and Ford 2014). The loan/gift policy should  clearly outline the requirements of researchers  in regards to any unused genetic material. It is recommended that subsamples that are returned to loaning collections for potential future reuse be maintained separately from the original samples in case the returning sample’s integrity was compromised (e.g., contaminated, mislabeled, improperly stored) while on loan. The use history of each sample is important to track, especially for returned material, because this allows personnel to inventory and use only returned samples if all other portions  have been consumed (see INVENTORY CONTROL AND DATA MANAGEMENT: Databasing for Genetic Samples).  When returned samples are reused, tracking also allows collection  managers  to  inform  researchers  of the chain  of custody of the returned sample, so that future researchers can evaluate the risks of use of such samples.
+If the institution provides the appropriate amount  of material, the genetic samples loaned/gifted  should be completely consumed by the researcher (see USE OF  COLLECTIONS: Aliquoting Samples). If a portion  of a genetic sample remains unused  after the project, however, researchers might be unclear about what to do with the remaining samples. In a recent collection survey, institutions requested that researchers address leftover samples in various ways, including destroying the remaining samples, returning samples to the originating institution for destruction or reuse, or accessioning samples into the researcher’s personal or institutional collection <ref name=ZimkusFord2014/>. The loan/gift policy should clearly outline the requirements of researchers  in regards to any unused genetic material. It is recommended that subsamples that are returned to loaning collections for potential future reuse be maintained separately from the original samples in case the returning sample’s integrity was compromised (e.g., contaminated, mislabeled, improperly stored) while on loan. The use history of each sample is important to track, especially for returned material, because this allows personnel to inventory and use only returned samples if all other portions  have been consumed (see [[#Databasing for genetic samples|INVENTORY CONTROL AND DATA MANAGEMENT: Databasing for genetic samples).  When returned samples are reused, tracking also allows collection manager  to inform researchers of the chain of custody of the returned sample, so that future researchers can evaluate the risks of use of such samples.
 <Br>
 ===Aliquoting samples===
-To maximize their use and research potential, genetic resources should  not  be  sent in their entirety; rather genetic  samples should be aliquoted  for internal or external use (see USE  OF  COLLECTIONS: Loan Policies). Regardless  of the end user, subsampling methods should be employed that maximize collection utility by minimally handling samples, effectively removing the smallest sampling amount, and reducing freeze–thaw events while manipulating samples. Implementing efficient organizational methods, from storage containers  to database  management systems, minimizes  the amount of time required to locate samples (see GENETIC SAMPLE PROCESSING: Storage Containers; INVENTORY CONTROL AND DATA MANAGEMENT: Sample Labeling and Tracking). At any one time, only a manageable number of samples should be retrieved, so that  cold-storage units do not remain open and the time that storage containers are kept outside of these units is minimized. During the subsampling process, samples should be kept as close to their normal storage temperature as possible. Depending on the temperature from which the samples were taken, liquid nitrogen, dry ice, or wet ice can be used to help keep samples cold during processing.
+To maximize their use and research potential, genetic resources should not  be sent in their entirety; rather genetic samples should be aliquoted for internal or external use (see [[#Loan policies|USE  OF COLLECTIONS: Loan policies]]). Regardless of the end user, subsampling methods should be employed that maximize collection utility by minimally handling samples, effectively removing the smallest sampling amount, and reducing freeze–thaw events while manipulating samples. Implementing efficient organizational methods, from storage containers to database management systems, minimizes the amount of time required to locate samples. At any one time, only a manageable number of samples should be retrieved, so that cold-storage units do not remain open and the time that storage containers are kept outside of these units is minimized. During the subsampling process, samples should be kept as close to their normal storage temperature as possible. Depending on the temperature from which the samples were taken, liquid nitrogen, dry ice, or wet ice can be used to help keep samples cold during processing.
 <Br>
 <Br>
-The amount of a genetic sample provided to a researcher should be scaled to their individual reques  to ensure  long-term  availability of the original sample for other researchers. The SOP should provide baseline standards to guide the amount  of genetic material sent as a loan/gift, including considerations for the type of preparation requested (e.g., tissue subsample, aliquot of extraction, PCR product) and the experimental protocol to be implemented. In a recent collection survey, collections were found to set these sampling criteria in various ways (Zimkus and Ford 2014). Over one-third of the surveyed collections provided the approximate amount of tissue needed for two to three DNA extractions; fewer collections quantified  the amount of a sample sent (i.e., ranging from 1 mm² to 6 mm² in size, weighing from 10 mg to 2 g), likely because measuring or weighing individual  samples is a time-consuming process that most collections cannot afford. Collection managers  should  also consider whether to extract DNA, rather than send tissue samples, especially when rare samples or those with low remaining  volumes are requested. Regardless of the general criteria, personnel working with genetic samples should   be  knowledgeable of the sample amounts needed for methods commonly conducted  (e.g., DNA  extraction,  RNA  extraction,  PCR,  cloning).  It is recommended that if researchers require more than the standard amount  needed, justification should be provided in their sample request (see USE  OF  COLLECTIONS: Loan Policies).
+The amount of a genetic sample provided to a researcher should be scaled to their individual request to ensure  long-term  availability of the original sample for other researchers. The SOP should provide baseline standards to guide the amount of genetic material sent as a loan/gift, including considerations for the type of preparation requested (e.g., tissue subsample, aliquot of extraction, PCR product) and the experimental protocol to be implemented. In a recent collection survey, collections were found to set these sampling criteria in various ways <ref name=ZimkusFord2014/>. Over one-third of the surveyed collections provided the approximate amount of tissue needed for two to three DNA extractions; fewer collections quantified  the amount of a sample sent (i.e., ranging from 1 mm² to 6 mm² in size, weighing from 10 mg to 2 g), likely because measuring or weighing individual samples is a time-consuming process that most collections cannot afford. Collection managers  should  also consider whether to extract DNA, rather than send tissue samples, especially when rare samples or those with low remaining  volumes are requested. Regardless of the general criteria, personnel working with genetic samples should  be knowledgeable of the sample amounts needed for methods commonly conducted  (e.g., DNA  extraction,  RNA  extraction,  PCR,  cloning).
 <Br>
 ===Packaging and shipping loans/gifts===
-As with traditional natural history specimens, loan/gift shipments of genetic samples should include loan paperwork  on institutional letterhead that documents the contents, handling requirements, and policies of use (see USE OF COLLECTIONS: Loan Policies). Before any loans/gifts are processed, collection personnel must determine all the national or international laws and regulations pertaining to the genetic samples and  the shipment, especially if a short shipping  time is critical. Copies of all permits and certificates should be included with the shipment and placed in a location that is easily accessible on the outside of the package. Confirmation of the receipt of the samples should be documented for all  loans/gifts and can be accomplished in the same manner as traditional natural history specimens; namely, a loan invoice form  is sent with the shipment  to be signed and returned by the researcher. In addition to the regular import/export permits  required for international loans, special permits  or  requirements might be necessary for genetic material, depending on the countries involved with the shipment. <ref>Renner, S.C., D. Neumann, M. Burkart, U. Feit, P. Giere, A. Paulsch, C. Paulsch, M. Sterz, C.L. Ha¨ user, and K. Vohland. 2012. Import and export of biological samples  from  tropical countries — Considerations and guidelines for research teams. Organisms Diversity & Evolution  12:81–98.</ref> In addition, specific taxa might be regulated, including those monitored by the US Department of Agriculture (USDA) and/or  those  protected under the International Treaty on Plant Genetic Resources for Food and Agriculture (PGRFA)<ref>Moore,  G.K. and W. Tymowski. 2005. Explanatory  guide to the International  Treaty on Plant Genetic Resources for Food and Agriculture. IUCN Environmental Policy and Law Paper No. 57. IUCN, Gland, Switzerland. 212 pp. </ref>, the Convention on International Trade in Endangered Species of Wild Fauna and Flora (CITES)<ref>Davis, K., C. Williams, M. Wolfson, and J. Donaldson. 2006. Practical implementation of the CBD and CITES. Pp. 36–46 in DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice  and Uses (V. Savolainen, M.P. Powell, K. Davis, G. Reeves,and A. Corthals, eds.). Kew Publishing, Royal  Botanic Garden,  Kew, England.  151 pp.</ref> <ref>Donaldson, J. 2006. CITES and DNA  banking.  Pp. 30–35 in DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice and Uses (V. Savolainen, M.P. Powell, K. Davis, G. Reeves, and  A. Corthals, eds.). Kew Publishing, Royal Botanic Garden, Kew, England. 151 pp.</ref>, and various US domestic laws, including the Endangered Species Act (ESA)<ref name=Applequist/>, the Lacey Act<ref name=Applequist/>, and the Migratory Bird Treaty Act (MBTA).  As the legal landscape evolves, collection personnel must receive the appropriate training, with applicable updates, in both national and  international  regulations, including the shipment of biological samples and dangerous  goods (e.g., DOT, International Air Transport Association [IATA] Special Provision  A180), and the recent ratification of the Convention on Biological Diversity Nagoya Protocol on Access and Benefit-Sharing.
+As with traditional natural history specimens, loan/gift shipments of genetic samples should include loan paperwork on institutional letterhead that documents the contents, handling requirements, and policies of use (see [[#Loan policies|USE OF COLLECTIONS: Loan policies]]). Before any loans/gifts are processed, collection personnel must:
+*Determine all the national or international laws and regulations pertaining to the genetic samples and the shipment
+*Include copies of all permits and certificates with the shipment in a location that is easily accessible on the outside of the package
+*Include invoice that can be signed and returned by the researcher upon receipt of the samples
+*Determine if special permits or requirements are necessary, including:<ref>Renner, S.C., D. Neumann, M. Burkart, U. Feit, P. Giere, A. Gröger,  A. Paulsch, C. Paulsch, M. Sterz and K. Vohland. 2012. Import and export of biological samples from  tropical countries — Considerations and guidelines for research teams. Organisms Diversity & Evolution  12:81–98.</ref>
+::- US Department of Agriculture (USDA)
+::- International Treaty on Plant Genetic Resources for Food and Agriculture (PGRFA)<ref>Moore, G.K. and W. Tymowski. 2005. Explanatory  guide to the International Treaty on Plant Genetic Resources for Food and Agriculture. IUCN Environmental Policy and Law Paper No. 57. IUCN, Gland, Switzerland. 212 pp. </ref>
+::- Convention on International Trade in Endangered Species of Wild Fauna and Flora (CITES)<ref>Davis, K., C. Williams, M. Wolfson, and J. Donaldson. 2006. Practical implementation of the CBD and CITES. Pp. 36–46 in DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice  and Uses (V. Savolainen, M.P. Powell, K. Davis, G. Reeves,and A. Corthals, eds.). Kew Publishing, Royal  Botanic Garden,  Kew, England.  151 pp.</ref> <ref>Donaldson, J. 2006. CITES and DNA  banking.  Pp. 30–35 in DNA and Tissue Banking for Biodiversity and Conservation: Theory, Practice and Uses (V. Savolainen, M.P. Powell, K. Davis, G. Reeves, and  A. Corthals, eds.). Kew Publishing, Royal Botanic Garden, Kew, England. 151 pp.</ref>, and various US domestic laws, including the Endangered Species Act (ESA)<ref name=Applequist/>
+::- Lacey Act<ref name=Applequist/>
+::- Migratory Bird Treaty Act (MBTA)
+As the legal landscape evolves, collection personnel must receive the appropriate training, with applicable updates, in both national and  international  regulations, including the shipment of biological samples and dangerous  goods (e.g., DOT, International Air Transport Association [IATA] Special Provision  A180), and the recent ratification of the Convention on Biological Diversity Nagoya Protocol on Access and Benefit-Sharing. See [[Shipping and Handling of Dangerous Goods|Shipping and Handling of Dangerous Goods]] for additional information.
 <Br>
 <Br>
-Loans/gifts of genetic samples can be shipped  using various methods and, depending on the sample type and ultimate  use, material transfers  might require  special means of shipping to preserve specimen integrity and quality.  Cold or frozen material should be shipped in a manner that will maintain the appropriate temperature for the duration of the shipment with allowance for delay in arrival time. ISBER (2012) suggested  that refrigerant  should last an additional 24 to 72 hours, depending on whether the shipment is domestic or international, especially because customs will be involved for the latter.  It is advised that refrigerated or frozen shipments  are not sent on days that require transit over a weekend or holiday  period, so as to avoid delays and ensure that recipients are available  for immediate receipt of the samples.  The  coordination of shipping  and receiving samples is important for all parties, so to avoid mishaps, both the shipper and recipient should track the package while in transit. Collection personnel should contact the recipient before sending the shipment to confirm that they are present to receive the package as scheduled and, again, contact the researcher to  notify  them when the shipment is specifically scheduled to arrive.
+Loans/gifts of genetic samples can be shipped using various methods and, depending on the sample type and ultimate use, material transfers might require special means of shipping to preserve specimen integrity and quality.  Cold or frozen material should be shipped in a manner that will maintain the appropriate temperature for the duration of the shipment with allowance for delay in arrival time. Refrigerant  should last an additional 24−72 hours, depending on whether the shipment is domestic or international, especially because customs will be involved for the latter<ref name=ISBER/>.  It is advised that refrigerated or frozen shipments are not sent on days that require transit over a weekend or holiday period, so as to avoid delays and ensure that recipients are available  for immediate receipt of the samples.  The coordination of shipping  and receiving samples is important for all parties, so to avoid mishaps, both the shipper and recipient should track the package while in transit. Collection personnel should contact the recipient before sending the shipment to confirm that they are present to receive the package as scheduled and, again, contact the researcher to  notify  them when the shipment is specifically scheduled to arrive.
 <br>
 <Br>
-When packing, genetic samples should be positioned in the package so that they are surrounded by refrigerant on all sides, rather than having samples placed on top of or underneath refrigerant.  Any empty space between samples and refrigerant should be filled with dunnage  material (e.g., loosefill non-biodegradable peanuts, padding material). Specimens that are sensitive to humidity  (e.g., botanical samples) should  be shipped  in sealed bags with desiccant to ensure that humidity  levels are controlled in transit. The following are typical temperature conditions required for shipment of genetic samples, including the insulation and/or refrigerant that can be used to maintain the desired temperature (modified from ISBER  2012).
+When packing, genetic samples should be positioned in the package so that they are surrounded by refrigerant on all sides, rather than having samples placed on top of or underneath refrigerant.  Any empty space between samples and refrigerant should be filled with dunnage material (e.g., loosefill non-biodegradable peanuts, padding material). Specimens that are sensitive to humidity  (e.g., botanical samples) should  be shipped  in sealed bags with desiccant to ensure that humidity  levels are controlled in transit. The following are typical temperature conditions required for shipment of genetic samples, including the insulation and/or refrigerant that can be used to maintain the desired temperature (modified<ref name=ISBER/>).
-# Ambient (20° to 30°C): insulated packaging  with a minimum of 4-cm-thick walls to protect from fluctuations in ambient  temperature; chemical  preservative might or might not be necessary, depending on sample type.
+[[File:Dry Ice.jpg|thumb|right|UN 1845 label for shipments including dry ice.]]
-# Refrigerated (2° to 8°C): insulated packaging  with a minimum of 4-cm-thick walls with wet ice or gel packs (conditioned at  215°C); chemical preservative might or might not be necessary, depending on sample type.
-# Frozen (-20°C): insulated packaging with a minimum of 4-cm-thick walls with gel packs designed for frozen temperatures (conditioned at or below -20°C).
+# Ambient (20°–30°C): insulated packaging with a minimum of 4-cm-thick walls to protect from fluctuations in ambient temperature; chemical preservative might or might not be necessary, depending on sample type.
-# Frozen (-70°C): insulated  packaging  with a minimum of 4-cm-thick walls with dry ice pellets, sheets, or blocks. Note that  dry ice (solid CO2) is considered a hazardous material and appropriate labeling should  be included in accordance with DOT  and IATA  regulations.
+# Refrigerated (2°–8°C): insulated packaging with a minimum of 4-cm-thick walls with wet ice or gel packs; chemical preservative might or might not be necessary, depending on sample type.
-# Frozen (at or below -150°C): LN2 dry shipper. Dry nitrogen shippers are insulated containers that contain LN2 that is fully absorbed in a porous material within the walls and, therefore, considered a non-dangerous product by DOT and IATA regulations.
+# Frozen (-20°C): insulated packaging with a minimum of 4-cm-thick walls with gel packs designed for frozen temperatures.
+# Frozen (-70°C): insulated packaging  with a minimum of 4-cm-thick walls with dry ice pellets, sheets, or blocks. Note: dry ice (solid CO<sub>2</sub>) is considered a hazardous material.
+# Frozen (at or below -150°C): LN<sub>2</sub> dry shipper. Dry nitrogen shippers are insulated containers that contain LN<sub>2</sub> that is fully absorbed in a porous material within the walls and, therefore, considered a non-dangerous product by DOT and IATA regulations.
 <Br>
-Recently surveyed genetic resource collections were found to most frequently ship samples frozen using dry ice, or at ambient temperature using ethanol or DMSO as a preservative.<ref name=ZimkusFord2014/> Shipping methods among collections likely differed due to overall cost, shipping  restrictions, ease of shipment, and the intended use of the samples. With increasing regulations on shipments and shipping training for personnel, expenses have become prohibitive for many institutions and, as a result, many collections are either requesting or requiring that researchers offset the associated costs (see FUNDING AND  BUDGET). Even 30 years ago, it was recommended that researchers planning to obtain samples from genetic resource collections include these costs in grant budgets.<ref>Baker, R.J. and M.S. Hafner. 1984. Curation of collections of frozen tissues: Curatorial problems unique to frozen tissue collections. Pp. 35–40 in Collections of Frozen Tissues: Value, Management,   Field  and Laboratory Procedures, and Directory of Existing Collections (H.C.  Dessauer  and  M.S.  Hafner,  eds.). Association  of Systematics Collections, Lawrence, Kansas. 74 pp.</ref>
+Recently surveyed genetic resource collections were found to most frequently ship samples frozen using dry ice, or at ambient temperature using ethanol or DMSO as a preservative.<ref name=ZimkusFord2014/> Shipping methods among collections likely differed due to overall cost, shipping restrictions, ease of shipment, and the intended use of the samples. With increasing regulations on shipments and shipping training for personnel, expenses have become prohibitive for many institutions and, as a result, many collections are either requesting or requiring that researchers offset the associated costs.
 ==Health & Safety==
@@ Line 300: / Line 458: @@
 ===General laboratory practices===
-Good laboratory practices should be implemented in genetic  resource collections to protect staff from exposure to various  hazards (e.g., potential pathogens, chemicals, sharps). For staff safety, certain  activities should be prohibited in the laboratory or collection space, including eating, drinking, storing food, smoking, applying cosmetics, or handling contact lenses. Mechanical pipetting devices should be used in the laboratory; for safety concerns, mouth pipetting must be prohibited. For collections harvesting genetic samples from traditional voucher specimens, collection managers must ensure that any biosafety waste is processed in accordance with institutional regulations  and any pertinent local, state, or national guidelines. Policies should be instituted for the safe handling and disposal of sharps (e.g., needles, razor blades, scalpels). Lastly, good laboratory practice includes washing hands at the end of preparation work, after gloves are removed, and prior to leaving the laboratory.
+Good laboratory practices should be implemented in genetic  resource collections to protect staff from exposure to various  hazards (e.g., potential pathogens, chemicals, sharps). For staff safety, certain activities should be prohibited in the laboratory or collection space, including:
+*Eating
+*Drinking
+*Storing food
+*Smoking
+*Applying cosmetics
+*Handling contact lenses
+*Mouth pipetting
+For collections harvesting genetic samples from traditional voucher specimens, collection managers must ensure that any biosafety waste is processed in accordance with institutional regulations  and any pertinent local, state, or national guidelines. Policies should be instituted for the safe handling and disposal of sharps (e.g., needles, razor blades, scalpels). Lastly, good laboratory practice includes washing hands at the end of preparation work, after gloves are removed, and prior to leaving the laboratory.
 ===Personal protective equipment===
@@ Line 306: / Line 472: @@
 ===Liquid nitrogen safety===
-Those collections that use LN2 storage equipment require additional safety precautions and equipment specifically rated  for cryogenic conditions. Specialized ventilation  and oxygen monitors might be needed to protect  personnel from the risk of oxygen depletion and possible asphyxiation (see FACILITY MANAGEMENT: Ventilation; FACILITY MANAGEMENT: Oxygen Monitors).  When working with LN2, appropriate PPE is recommended to protect the eyes and skin from cryogenic burns. Cryogenic gloves, which are water-resistant insulated gloves rated for cryogenic temperatures, should be used at all times to protect the hands  when working with LN2 equipment (e.g., cryovats,  dewars,  hoses), storage equipment (e.g., racks, boxes), and samples. Cryogenic gloves will not protect the skin when immersed in the nitrogen liquid itself, so additional precautions must be taken to insure that  gloves are only exposed to vapor. Cryogenic aprons are essential to protect the body when using the liquid phase of nitrogen but are also a good precaution when working with the vapor phase of LN2. Eye protection should be worn when working with samples that have been stored in the liquid and vapor phase of nitrogen, but there is an added danger with the liquid phase because sample vials can burst without warning if LN2 enters them through minute cracks while in storage and then rapidly expands when thawing. When dispensing LN2, goggles and/or a face shield, rather than  simple safety glasses, are recommended  to additionally  protect the face and eyes from possible splashing. Closed-toe shoes that cover the entire foot are required in genetic labs but, when working with LN2, it is additionally  recommended that footwear  can be quickly removed (e.g., few laces, buckles, zippers). Therefore, if a spill occurs and liquefied gas enters the shoes, footwear can be easily removed, preventing severe burns that result when LN2 surrounds the foot with nitrogen and is held in the shoe material. Canvas shoes are not recommended  because LN2 can easily permeate the material.  With  regard to clothing, lab coats are essential, and it is recommended  that pants not have cuffs nor be tucked into shoes or boots because LN2 can become trapped if spilled.
+[[File:IMG 1229.JPG|thumb|right|Cryogenic apron, cryogenic gloves and face shield. (Photograph by B. Zimkus.)]]
+Those collections that use LN<sub>2</sub> storage equipment require additional safety precautions and equipment specifically rated  for cryogenic conditions. Specialized ventilation  and oxygen monitors might be needed to protect  personnel from the risk of oxygen depletion and possible asphyxiation (see [[#Ventilation|FACILITY MANAGEMENT: Ventilation]];  [[#Oxygen monitors|FACILITY MANAGEMENT: Oxygen monitors]]). When working with LN<sub>2</sub>, appropriate PPE is recommended:
+*Cryogenic gloves, which are water-resistant insulated gloves rated for cryogenic temperatures, to protect the hands from cold temperatures and nitrogen vapor
+*Cryogenic aprons to protect the body when using the liquid phase of nitrogen
+*Eye protection (e.g., safety glasses) when working with samples that have been stored in the liquid phase of nitrogen because sample vials can burst without warning if LN<sub>2</sub> enters them through minute cracks
+*Goggles and/or a face shield when dispensing LN<sub>2</sub> to additionally  protect the face and eyes from possible splashing
+*Closed-toe shoes (not canvas) that can be quickly removed (e.g., few laces, buckles, zippers)
+*Lab coats
+*Pants without cuffs; pants should not be tucked into shoes or boots because LN<sub>2</sub> can become trapped if spilled<Br>
+If nitrogen in the liquid form contacts the skin or eyes, the tissue should be immediately flooded or soaked with tepid or warm water (105°F –115°F [41°C–46°C]). Hot water (above 46°C) should never be used because this can cause additional damage to the skin. In addition, the skin must not be rubbed because this can damage the tissue; thus, any contact should involve only gentle patting or dabbing. If LN<sub>2</sub> comes in contact with the eyes, contact lenses should be removed immediately and the eyes flushed with tepid or warm water for at least 15 minutes, and the upper and lower eyelids should be lifted occasionally during the flushing process. If any injury occurs from  a cryogenic burn, medical attention should be sought as soon as possible.
 <Br>
 <Br>
-If nitrogen in the liquid form contacts the skin or eyes, the tissue should be immediately flooded or soaked with tepid or warm water (105°F to 115°F [41°C to 46°C]). Hot water (above 46°C) should never be used because this can cause additional damage to the skin. In addition, the skin must not be rubbed because this can damage the tissue; thus, any contact should involve only gentle patting or dabbing. If LN2 comes in contact with the eyes, contact lenses should be removed immediately and the eyes flushed with tepid or warm water for at least 15 minutes, and the upper and lower eyelids should be lifted occasionally during the flushing process. If any injury occurs from  a cryogenic burn, medical attention should be sought  as soon as possible.
+Cryogenic  fluids must be handled and stored only in containers  specifically designed for these products. Unapproved materials can become brittle and shatter or become over-pressurized, causing risks of explosion. All cryogenic vessels must be equipped with pressure-relief devices (e.g., relief valve, venting lid/stopper) to prevent excessive pressure build-up. A tremendous amount of force can be generated if liquid nitrogen rapidly vaporizes, so pressure-relief  devices on LN<sub>2</sub> equipment should  be monitored to ensure that they are functioning  properly.  Transfer operations involving open cryogenic containers, such as dewars, should  be conducted slowly to minimize boiling, splashing, and thermal shock to the receiving vessel. A phase separator (i.e., fitting that  attaches to end of a transfer hose that  separates gas from liquid)can also be used to control the vapor path while dispensing.  When  dispensing or  pouring  LN<sub>2</sub>, receiving vessels should  be placed as close as possible to the source; a table  or other sturdy  surface can be used to position the vessel in the proper location. Funnels should not be used to channel LN<sub>2</sub> because they can freeze, creating a splash hazard, or be propelled upwards if the container is overfilled.
-<Br>
-<Br>
-Cryogenic  fluids must be handled and stored only in containers  specifically designed for these products  in accordance  with SOP. Unapproved materials can become brittle and shatter or become over-pressurized, causing risks of explosion. All cryogenic vessels must be equipped with pressure-relief devices (e.g., relief valve, venting lid/stopper) to prevent excessive pressure build-up. A tremendous amount of force can be generated if liquid nitrogen rapidly vaporizes, so pressure-relief  devices on LN2 equipment should  be monitored to ensure that they are functioning  properly.  Transfer operations involving open cryogenic containers, such as dewars, should  be  conducted slowly to minimize boiling, splashing, and thermal shock to the receiving vessel. A phase separator (i.e., fitting that  attaches to end of a transfer  hose that  separates gas from liquid)can also be used to control the vapor path while dispensing.  When  dispensing or  pouring  LN2, receiving vessels should  be placed as close as possible to the source; a table  or other sturdy  surface can be used to position the vessel in the proper location. Funnels should not be used to channel LN2 because they can freeze, creating a splash hazard, or be propelled  upwards by the LN2 if the container is overfilled.
 <Br>
 ===Dry ice safety===
-Use  of dry  ice (i.e., solid phase  of CO2) is regulated and requires specialized training  for  use in shipments. When dry ice is used, collection managers should ensure that there is adequate ventilation because CO2 can displace  oxygen, causing loss of consciousness or even asphyxiation. All confined areas should be closely monitored when dry ice is in use. Walk-in freezers should be kept free of dry ice because carbon dioxide can rapidly build up without regular air exchange; owing to this inherent danger, proper signage should  be posted outside walk-in freezers to prevent staff from placing dry ice into walk-in freezers.
+Use  of dry  ice (i.e., solid phase  of CO<sub>2</sub>) is regulated and requires specialized training  for  use in shipments. When dry ice is used, collection managers should ensure that there is adequate ventilation because CO<sub>2</sub> can displace  oxygen, causing loss of consciousness or even asphyxiation. All confined areas should be closely monitored when dry ice is in use. Walk-in freezers should be kept free of dry ice because carbon dioxide can rapidly build up without regular air exchange; owing to this inherent danger, proper signage should  be posted outside walk-in freezers to prevent staff from placing dry ice into walk-in freezers.
 ===Biosafety===
-Collection  managers  should consult  all federal biosafety and biocontain- ment regulations relevant to the activities conducted that involve potentially hazardous biological materials  within the collection. Policies should incorporate all regulations  that outline standard and special practices, safety equipment,  and facility requirements  to minimize potential  hazards  to laboratory personnel and the environment. USDA permits could be needed for work  with some specific taxa,  such as birds,  some mammals,  and plants.  Depending  on the biosafety level required for the collection as determined  by the USDA,   certain  requirements   might  need  to  be  met,  including  training   in  handling pathogenic  agents,  restrictions  to collection access when work  is being conducted,  and conduction of particular work in a biological safety cabinet. A biosafety cabinet (BSC), also known  as a biological or microbiological  safety cabinet,  is an enclosed, ventilated workspace for handling  materials  potentially  contaminated with pathogens (e.g., Exotic Newcastle Disease, Foot-and-Mouth Disease, Hantavirus, Highly Pathogenic  Avian Influenza).  BSCs differ from fume hoods because BSC exhaust air is HEPA-filtered as it exits. BSCs are classified as one of three classes by their level of protection provided to personnel  and  the  environment (i.e.,  Class I, II, III). Class II Type A2 BSC, which includes a minimum inflow velocity of 100 ft/min (30.5 m/min), is the most commonly used  BSC providing  protection for personnel, the  environment, and the samples. Collection managers should be aware that gas lines should not be installed into BSCs because air is contained within, rather than being exhausted from the cabinet, leading to the potential build up of flammable materials. Additionally, open flames, such as those generated  by Bunsen burners, can detrimentally affect airflow in a BSC, disrupting the pattern of HEPA-filtered air supplied to the work surface. To provide  adequate protection, BSCs require proper use, monitoring, and regular maintenance. SOP documents must outline these approved  activities, including  appropriate height of the sash opening to minimize airflow, methods used to decontaminate surfaces,  as well as testing and certification  protocols  for the unit itself (see OPERATIONAL BEST  PRACTICE: Equipment Preventative Maintenance, Repair, and Replacement).
+Collection  managers  should consult  all federal biosafety and biocontainment regulations relevant to the activities conducted that involve potentially hazardous biological materials  within the collection. Policies should incorporate all regulations  hat outline standard and special practices, safety equipment, and facility requirements  to minimize potential hazards to laboratory personnel and the environment. USDA permits could be needed for work with some specific taxa, such as birds, some mammals, and plants.  Depending  on the biosafety level required for the collection as determined  by the USDA,  certain requirements   might  need  to  be  met,  including:
+*Training   in  handling pathogenic  agents
+*Restrictions  to collection access when work  is being conducted
+*Conduction of particular work in a biological safety cabinet
+A biosafety cabinet (BSC), also known as a biological or microbiological  safety cabinet, is an enclosed, ventilated workspace for handling materials  potentially  contaminated with pathogens (e.g., Exotic Newcastle Disease, Foot-and-Mouth Disease, Hantavirus, Highly Pathogenic  Avian Influenza). BSCs differ from fume hoods because BSC exhaust air is HEPA-filtered as it exits. BSCs are classified as one of three classes by their level of protection provided to personnel  and  the  environment (i.e.,  Class I, II, III). Class II Type A2 BSC, which includes a minimum inflow velocity of 100 ft/min (30.5 m/min), is the most commonly used  BSC providing protection for personnel, the  environment, and the samples. Collection managers should be aware that gas lines should not be installed into BSCs because air is contained within, rather than being exhausted from the cabinet, leading to the potential build up of flammable materials. Additionally, open flames, such as those generated  by Bunsen burners, can detrimentally affect airflow in a BSC, disrupting the pattern of HEPA-filtered air supplied to the work surface. To provide  adequate protection, BSCs require proper use, monitoring, and regular maintenance. SOP documents must outline these approved  activities, including  appropriate height of the sash opening to minimize airflow, methods used to decontaminate surfaces,  as well as testing and certification protocols for the unit itself (see [[#Equipment preventative maintenance, repair, and replacement|OPERATIONAL BEST  PRACTICE: Equipment preventative maintenance, repair, and replacement]]).
 <Br>
 ===Chemical safety===
-Genetic resource collections should maintain an inventory of all chemicals used and access to Safety Data Sheets (SDS) for every chemical used within the collection. A chemical hygiene plan should  also be included in SOP documents, which outlines the appropriate use of chemicals in the collection, as well as their containment and  procedures for clean-up if spills occur. Personnel should have the appropriate training for all procedures related to chemical safety, which frequently  involves training by institutional groups, such as health and safety and the fire group (see OPERATIONAL BEST  PRACTICE: Training).
+Genetic resource collections should maintain an inventory of all chemicals used and access to Safety Data Sheets (SDS) for every chemical used within the collection. A chemical hygiene plan should  also be included in SOP documents, which outlines the appropriate use of chemicals in the collection, as well as their containment and  procedures for clean-up if spills occur. Personnel should have the appropriate training for all procedures related to chemical safety, which frequently  involves training by institutional groups, such as health and safety and the fire group (see [[#Training|OPERATIONAL BEST  PRACTICE: Training]]).
 ===Fire safety===
-Collection personnel must comply with all local fire and building codes. Automatic fire detection units and suppression  systems, including appropriate hand-held fire extinguishers and sprinkler systems, are recommended. The SOP should include information regarding major fire hazards  and potential ignition sources, as well as what working materials are flammable hazards (e.g., ethanol). Personnel  should be trained in fire prevention and emergency procedures relating to evacuation  if a fire occurs (see OPERATIONAL BEST PRACTICE: Training).  All fire detection systems and suppression systems should be tested on a regular basis and frequently involve health and safety, fire, and building facility  personnel at the  institution (see OPERATIONAL BEST PRACTICE: Equipment Preventative Maintenance, Repair, and Replacement).
+Collection personnel must comply with all local fire and building codes. Automatic fire detection units and suppression  systems, including appropriate hand-held fire extinguishers and sprinkler systems, are recommended. The SOP should include information regarding major fire hazards  and potential ignition sources, as well as what working materials are flammable hazards (e.g., ethanol). Personnel  should be trained in fire prevention and emergency procedures relating to evacuation  if a fire occurs (see [[#Training|OPERATIONAL BEST PRACTICE: Training]]).  All fire detection systems and suppression systems should be tested on a regular basis and frequently involve health and safety, fire, and building facility  personnel at the  institution (see [[#Equipment preventative maintenance, repair, and replacement|OPERATIONAL BEST  PRACTICE: Equipment preventative maintenance, repair, and replacement]]).
 ==Ethical and Legal Best Practice==
-The accumulation and use of genetic samples involve numerous ethical and legal issues. Most natural history museums have institutional policies that address legal compliance and ethical standards, but many times, genetic samples are present in  individual laboratories or stand-alone collections whose activities might not be specifically addressed in the broader   institutional policies. In these instances, dedicated  policies might not be in place to govern broad aspects of legal and ethical issues associated with the initial collection, transport, and use of genetic samples. Genetic resource collections are subject to the same regulations, laws, and consequences as traditional natural  history collections. As such, they must have accessioning practices that ensure and document that all samples are legally collected, transported, and acquired by the collection. Copies of all necessary permits, including collecting permits, relevant Material Transfer Agreements, export  permits from the country of origin, and import permits  into  the country of the genetic collection, must be on file within the institution or genetic resource collection (see POLICY BEST  PRACTICE). The accession process should also ensure and document that all animals collected were done so in a manner consistent with pertinent guidelines, such as Institutional Animal Care and Use Committee(IACUC)regulations.
+The accumulation and use of genetic samples involve numerous ethical and legal issues. Most natural history museums have institutional policies that address legal compliance and ethical standards, but many times, genetic samples are present in  individual laboratories or stand-alone collections whose activities might not be specifically addressed in the broader   institutional policies. In these instances, dedicated  policies might not be in place to govern broad aspects of legal and ethical issues associated with the initial collection, transport, and use of genetic samples. Genetic resource collections are subject to the same regulations, laws, and consequences as traditional natural  history collections. As such, they must have accessioning practices that ensure and document that all samples are legally collected, transported, and acquired by the collection. Copies of all necessary permits, including collecting permits, relevant Material Transfer Agreements, export permits from the country of origin, and import permits  into  the country of the genetic collection, must be on file within the institution or genetic resource collection. The accession process should also ensure and document that all animals collected were done so in a manner consistent with pertinent guidelines, such as Institutional Animal Care and Use Committee (IACUC) regulations.
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@@ Line 335: / Line 511: @@
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 <br>
-To document compliance and provide responsible stewardship for consumptive genetic resources, collection personnel  should track the use history of all genetic samples and their derivatives, and link this information to the available  metadata (e.g., NCBI GenBank; see INVENTORY CONTROL AND DATA MANAGEMENT: Databasing for Genetic Samples). Loan/gift policy must,  therefore, be explicit in the approved uses of genetic samples and associated  metadata, as well as expectations  for what the researcher should do with any samples remaining after the completion of the research (see USE OF COLLECTIONS: Loan  Policies). Policy should also clearly outline requirements resulting from use of the genetic material, which can include the acknowledgement  of the collection in publications, notification of any resulting  publications to the originating  collection, and submission of genetic sequence data to a public genetic sequence database. Research users and collection  managers  should both make a dedicated  effort to ensure that collections are formally acknowledged for use of their samples and collections are notified of published studies that result from the use of their  material. Knowledge of sample use is  vital to genetic resource collections, because they must justify their significance in research to both their  institution and outside funding bodies. Lastly, copyright and intellectual property rights in relation to genetic sample metadata provided to researchers or presented on public websites should be accompanied by policy that outlines the terms and conditions of its use, including the requirements to share results from the research.
+To document compliance and provide responsible stewardship for consumptive genetic resources, collection personnel  should track the use history of all genetic samples and their derivatives, and link this information to the available metadata (e.g., NCBI GenBank; see [[#Databasing for genetic samples|INVENTORY CONTROL AND DATA MANAGEMENT: Databasing for genetic samples]]). Loan/gift policy must,  therefore, be explicit in the approved uses of genetic samples and associated  metadata, as well as expectations  for what the researcher should do with any samples remaining after the completion of the research (see [[#Loan  policies|USE OF COLLECTIONS: Loan  policies]]). Policy should also clearly outline requirements resulting from use of the genetic material. Research users and collection managers  should both make a dedicated effort to ensure that collections are formally acknowledged for use of their samples and collections are notified of published studies that result from the use of their material. Knowledge of sample use is  ital to genetic resource collections, because they must justify their significance in research to both their  institution and outside funding bodies. Lastly, copyright and intellectual property rights in relation to genetic sample metadata provided to researchers or presented on public websites should be accompanied by policy that outlines the terms and conditions of its use, including the requirements to share results from the research.
 <br>
-<br>
-Genetic and genomic resource collections, by their nature, are very process and equipment-dependent, requiring dedicated space, personnel, and funding to function properly. Operating at suboptimal levels can have deleterious and catastrophic effects on both the genetic samples and collection personnel. Institutions and/or laboratories that form genetic and genomic resource collections must be aware of the commitments associated with operating, monitoring,and maintaining these collections, including legal obligations and safety requirements. It is the responsibility of those overseeing genetic resource collections to properly assess and control risk hazards ensuring that personnel can work safely and samples are proficiently curated.
-==Contributors==
+==Source Material==
-[[User:BredaZimkus|Breda Zimkus]], Linda Ford
+Zimkus, B.M. and L.S. Ford. 2014. [[Media:Zimkus Ford 2014 Best Practices.pdf|Best Practices for Genetic Resources Associated with Natural History Collections Recommendations for Practical Implementation]][[File:Pdf logo - small.gif|link=]]. ''Collection Forum'' 28(1-2), pp. 77-112.
-==Source Material==
+==Links==
-Zimkus, Breda M. and Linda Ford [[Media:Zimkus Ford 2014 Best Practices.pdf|Best Practices for Genetic Resources Associated with Natural History Collections Recommendations for Practical Implementation]][[File:Pdf logo - small.gif|link=]], 2014. ''Collection Forum'' 28(1-2), pp. 77-112. Society for the Preservation of Natural History Collections.
+*[https://www.idigbio.org/genetic-resources DNA Banks and Genetic Resources Repositories in the United States]
+*[http://www.isber.org International Society for Biological and Environmental Repositories]
+*[http://www.ggbn.org The Global Genome Biodiversity Network]
+*[https://www.cbd.int/abs/about/ The Nagoya Protocol on Access to Genetic Resources and the Fair and Equitable Sharing of Benefits Arising from their Utilization (ABS) to the Convention on Biological Diversity]
+*[https://nature.ca/en/research-collections/collections/cryobank National Biodiversity Cryobank of Canada]
 ==References==
@@ Line 352: / Line 530: @@
-[[Category:Best_Practices]]
+[[Category:Best_Practices]][[Category:Curation Practices]][[Category:Cryogenic Collections]][[Category:Specimen and Material Type]]