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Lecture 3 - Biosafety Levels 1 & 2.pptx

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nafeesa Hanif

1) The document summarizes biosafety levels 1 and 2, including laboratory design features, equipment requirements, and waste handling procedures to protect workers and the environment. 2) Key aspects of biosafety levels 1 and 2 include procedures to minimize aerosol production, requirements for personal protective equipment, and methods for decontaminating or sterilizing infectious materials within the laboratory before disposal. 3) Training of laboratory workers in safe microbiological techniques is essential to prevent the spread of pathogens, as human error can compromise safety systems.

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LECTURE 3 MPhil – BIOTECHNOLOGY/ BIOCHEMSITRY (MORNING) BIOT-707 (1st/2ND SEMESTER) Biosafety Levels – 1 & 2 BY NAFEESA QUDSIA HANIF, PhD
Purpose of Laboratory Design • Protect the Workers • Enable the Work • Secure the Facility • Protect the Environment • Comply with Regulations 2
Table 1.Classification of infective microorganisms by risk group Risk Group 1 (no or low individual and community risk) • A microorganism that is unlikely to cause human or animal disease. Risk Group 2 (moderate individual risk, low community risk) • A pathogen that can cause human or animal disease but is unlikely to be a serious hazard to laboratory workers, the community, livestock or the environment. Laboratory exposures may cause serious infection, but effective treatment and preventive measures are available and the risk of spread of infection is limited. Risk Group 3 (high individual risk, low community risk) • A pathogen that usually causes serious human or animal disease but does not ordinarily spread from one infected individual to another. Effective treatment and preventive measures are available. Risk Group 4 (high individual and community risk) • A pathogen that usually causes serious human or animal disease and that can be readily transmitted from one individual to another, directly or indirectly. Effective treatment and preventive 3
Table 2. Relation of risk groups to biosafety levels, practices and equipments 4 BSC, biological safety cabinet; GMT, good microbiological techniques
Table 3.Summary of biosafety level requirements 5 1 2 3 4 Isolationa of laboratory No No Yes Yes Room sealable for decontamination No No Yes Yes Ventilation: — inward airflow No Desirable Yes Yes — controlled ventilating system No Desirable Yes Yes — HEPA-filtered air exhaust No No Yes/Nob Yes Double-door entry No No Yes Yes Airlock No No No Yes Airlock with shower No No No Yes Anteroom No No Yes — Anteroom with shower No No Yes/Noc No Effluent treatment No No Yes/Noc Yes Autoclave: — on site No Desirable Yes Yes — in laboratory room No No Desirable Yes — double-ended No No Desirable Yes Biological safety cabinets No Desirable Yes Yes Personnel safety monitoring capabilityd No No Desirable Yes Link for safety levels: https://www.youtube.com/watch?v=xNYASNEdgg8
Basic Laboratories – Biosafety Level 1 & 2 6
Figure 1.Biohazard warning sign for laboratory doors 7 BIOHAZARD Admittance to Authorized personnels only Biosafety Level: ______________________ Responsible Investigator:________________ In case of Emergency call:_______________ Day time phone: _______ Home phone: ______ Authorization for entrance must be obtained from the Responsible Investigator named above. Instructions: • Only authorized persons should be allowed to enter the laboratory working areas. • Laboratory doors should be kept closed. • Children should not be authorized or allowed to enter laboratory working areas. • Access to animal houses should be specially authorized. • No animals should be admitted other than those involved in the work of the laboratory.
PERSONAL PROTECTION INSTRUCTIONS: • Laboratory coveralls, gowns or uniforms must be worn at all times for work in the laboratory. • Appropriate gloves must be worn for all procedures that may involve direct or accidental contact with blood, body fluids and other potentially infectious materials or infected animals. After use, gloves should be removed aseptically and hands must then be washed. • Personnel must wash their hands after handling infectious materials and animals, and before they leave the laboratory working areas. • Safety glasses, face shields (visors) or other protective devices must be worn when it is necessary to protect the eyes and face from splashes, impacting objects and sources of artificial ultraviolet radiation. • It is prohibited to wear protective laboratory clothing outside the laboratory, e.g. in canteens, coffee rooms, offices, libraries, staff rooms and toilets. • Open-toed footwear must not be worn in laboratories. • Eating, drinking, smoking, applying cosmetics and handling contact lenses is prohibited in the laboratory working areas. • Storing human foods or drinks anywhere in the laboratory working areas is prohibited. • Protective laboratory clothing that has been used in the laboratory must not be stored in the same lockers or cupboards as street clothing. 8
PROCEDURES…… • Pipetting by mouth must be strictly forbidden. • Materials must not be placed in the mouth. Labels must not be licked. • All technical procedures should be performed in a way that minimizes the formation of aerosols and droplets. • The use of hypodermic needles and syringes should be limited. They must not be used as substitutes for pipetting devices or for any purpose other than parenteral injection or aspiration of fluids from laboratory animals. • All spills, accidents and overt or potential exposures to infectious materials must be reported to the laboratory supervisor. A written record of such accidents and incidents should be maintained. • A written procedure for the clean-up of all spills must be developed and followed. • Contaminated liquids must be decontaminated (chemically or physically) before discharge to the sanitary sewer. An effluent treatment system may be required, depending on the risk assessment for the agent(s) being handled. • Written documents that are expected to be removed from the laboratory need to be protected from contamination while in the laboratory. 9
Laboratory working areas • The laboratory should be kept neat, clean and free of materials that are not pertinent to the work. • Work surfaces must be decontaminated after any spill of potentially dangerous material and at the end of the working day. • All contaminated materials, specimens and cultures must be decontaminated before disposal or cleaning for reuse. • Packing and transportation must follow applicable national and/or international regulations. • When windows can be opened, they should be fitted with arthropod- proof screens. 10
Biosafety Management • It is the responsibility of the laboratory director (the person who has immediate responsibility for the laboratory) to ensure the development and adoption of a biosafety management plan and a safety or operations manual. • The laboratory supervisor (reporting to the laboratory director) should ensure that regular training in laboratory safety is provided. • Personnel should be advised of special hazards, and required to read the safety or operations manual and follow standard practices and procedures. The laboratory supervisor should make sure that all personnel understand these. A copy of the safety or operations manual should be available in the laboratory. • There should be an arthropod and rodent control programme. • Appropriate medical evaluation, surveillance and treatment should be provided for all personnel in case of need, and adequate medical records should be maintained. 11
Laboratory design and facilities • In designing a laboratory and assigning certain types of work to it, special attention should be paid to conditions that are known to pose safety problems. These include: • Formation of aerosols • Work with large volumes and/or high concentrations of microorganisms • Overcrowding and too much equipment • Infestation with rodents and arthropods • Unauthorized entrance • Workflow: use of specific samples and reagents. • Examples of laboratory designs for Biosafety Levels 1 and 2 are shown in Figures 2 and 3, respectively. 12
Figure 2. A typical Biosafety Level 1 laboratory (graphics kindly provided by CUH2A, Princeton, NJ, USA) 13
Figure 3.A typical Biosafety Level 2 laboratory (graphics kindly provided by CUH2A, Princeton, NJ, USA). Procedures likely to generate aerosols are performed within a biological safety cabinet. Doors are kept closed and are posted with appropriate hazard signs. Potentially contaminated wastes are separated from the general waste stream. 14
Design features 1. Ample space must be provided for the safe conduct of laboratory work and for cleaning and maintenance. 2. Walls, ceilings and floors should be smooth, easy to clean, impermeable to liquids and resistant to the chemicals and disinfectants normally used in the laboratory. Floors should be slip-resistant. 3. Bench tops should be impervious to water and resistant to disinfectants, acids, alkalis, organic solvents and moderate heat. 4. Illumination should be adequate for all activities. Undesirable reflections and glare should be avoided. 5. Laboratory furniture should be sturdy. Open spaces between and under benches, cabinets and equipment should be accessible for cleaning. 6. Storage space must be adequate to hold supplies for immediate use and thus prevent clutter on bench tops and in aisles. Additional long-term storage space, conveniently located outside the laboratory working areas, should also be provided. 7. Space and facilities should be provided for the safe handling and storage of solvents, radioactive materials, and compressed and liquefied gases. 15
Design features (Cont’d.) 8. Facilities for storing outer garments and personal items should be provided outside the laboratory working areas. 9. Facilities for eating and drinking and for rest should be provided outside the laboratory working areas. 10. Hand-washing basins, with running water if possible, should be provided in each laboratory room, preferably near the exit door. 11. Doors should have vision panels, appropriate fire ratings, and preferably be self- closing. 12. At Biosafety Level 2, an autoclave or other means of decontamination should be available in appropriate proximity to the laboratory. 13. Safety systems should cover fire, electrical emergencies, emergency shower and eyewash facilities. 14. First-aid areas or rooms suitably equipped and readily accessible should be available. 16
Design features (Cont’d.) 15. In the planning of new facilities, consideration should be given to the provision of mechanical ventilation systems that provide an inward flow of air without recirculation. If there is no mechanical ventilation, windows should be able to be opened and should be fitted with arthropod-proof screens. 16. A dependable supply of good quality water is essential. There should be no cross- connections between sources of laboratory and drinking-water supplies. An anti- backflow device should be fitted to protect the public water system. 17. There should be a reliable and adequate electricity supply and emergency lighting to permit safe exit. A stand-by generator is desirable for the support of essential equipment, such as incubators, biological safety cabinets, freezers, etc., and for the ventilation of animal cages. 18. There should be a reliable and adequate supply of gas. Good maintenance of the installation is mandatory. 19. Laboratories and animal houses are occasionally the targets of vandals. Physical and fire security must be considered. Strong doors, screened windows and restricted issue of keys are compulsory. Other measures should be considered and applied, as appropriate, to augment security (see Chapter 9). 17
Laboratory Equipment • The laboratory director should, after consultation with the biosafety officer and safety committee (if designated), ensure that adequate equipment is provided and that it is used properly. Equipment should be selected to take account of certain general principles, i.e. it should be: • Designed to prevent or limit contact between the operator and the infectious material • Constructed of materials that are impermeable to liquids, resistant to corrosion and meet structural requirements • Fabricated to be free of burrs, sharp edges and unguarded moving parts • Designed, constructed and installed to facilitate simple operation and provide for ease of maintenance, cleaning, decontamination and certification testing; glassware and other breakable materials should be avoided, whenever possible. • Detailed performance and construction specifications may need to be consulted to ensure that the equipment possesses the necessary safety features 18
Essential biosafety equipment • Pipetting aids – to avoid mouth pipetting. Many different designs are available. • Biological safety cabinets, to be used whenever: • infectious materials are handled; • there is an increased risk of airborne infection • procedures with a high potential for producing aerosols are used; these may include centrifugation, grinding, blending, vigorous shaking or mixing, sonic disruption, opening of containers of infectious materials whose internal pressure may be different from the ambient pressure, intranasal inoculation of animals, and harvesting of infectious tissues from animals and eggs. • Plastic disposable transfer loops. Alternatively, electric transfer loop incinerators may be used inside the biological safety cabinet to reduce aerosol production. 19
Essential biosafety equipment Cont’d. • Screw-capped tubes and bottles. • Autoclaves or other appropriate means to decontaminate infectious materials. • Plastic disposable Pasteur pipettes, whenever available, to avoid glass. • Equipment such as autoclaves and biological safety cabinets must be validated with appropriate methods before being taken into use. Recertification should take place at regular intervals, according to the manufacturer’s instructions. 20
Health and Medical Surveillance • The employing authority, through the laboratory director, is responsible for ensuring that there is adequate surveillance of the health of laboratory personnel. The objective of such surveillance is to monitor for occupationally acquired diseases. Appropriate activities to achieve these objectives are: • Provision of active or passive immunization where indicated. • Facilitation of the early detection of laboratory-acquired infections. • Exclusion of highly susceptible individuals (e.g. pregnant women or immuno- compromised individuals) from highly hazardous laboratory work • Provision of effective personal protective equipment and procedures. 21
Guidelines for the surveillance of laboratory workers - Handling microorganisms at Biosafety Level 1 • Historical evidence indicates that the microorganisms handled at this level are unlikely to cause human disease or animal disease of veterinary importance. Ideally, however, all laboratory workers should undergo a pre-employment health check at which their medical history is recorded. Prompt reporting of illnesses or laboratory accidents is desirable and all staff members should be made aware of the importance of maintaining GMT. 22
Guidelines for the surveillance of laboratory workers - handling microorganisms at Biosafety Level 2 • A pre-employment or preplacement health check is necessary. The person’s medical history should be recorded and a targeted occupational health assessment performed. • Records of illness and absence should be kept by the laboratory management. • Women of childbearing age should be made aware of the risk to an unborn child of occupational exposure to certain microorganisms, e.g. rubella virus. The precise steps taken to protect the fetus will vary, depending on the microorganisms to which the women may be exposed. 23
Training Human error and poor technique can compromise the best of safeguards to protect the laboratory worker. Thus, a safety-conscious staff, well informed about the recognition and control of laboratory hazards, is key to the prevention of laboratory. Staff training should always include information on safe methods for highly hazardous procedures that are commonly encountered by all laboratory personnel and which involve: • Inhalation risks (i.e. aerosol production) when using loops, streaking agar plates, pipetting, making smears, opening cultures, taking blood/serum samples, centrifuging, etc. • Ingestion risks when handling specimens, smears and cultures • Risks of percutaneous exposures when using syringes and needles • Bites and scratches when handling animals • Handling of blood and other potentially hazardous pathological materials • Decontamination and disposal of infectious material. 24
Waste Handling…… • Waste is anything that is to be discarded. • In laboratories, decontamination of wastes and their ultimate disposal are closely interrelated. In terms of daily use, few if any contaminated materials will require actual removal from the laboratory or destruction. Most glassware, instruments and laboratory clothing will be reused or recycled. The overriding principle is that all infectious materials should be decontaminated, autoclaved or incinerated within the laboratory. • The principal questions to be asked before discharge of any objects or materials from laboratories that deal with potentially infectious microorganisms or animal tissues are: • Have the objects or materials been effectively decontaminated or disinfected by an approved procedure? • If not, have they been packaged in an approved manner for immediate on-site incineration or transfer to another facility with incineration capacity? • Does the disposal of the decontaminated objects or materials involve any additional potential hazards, biological or otherwise, to those who carry out the immediate disposal procedures or who might come into contact with discarded items outside the facility? 25
Decontamination…… • Steam autoclaving: It is the preferred method for all decontamination processes. Materials for decontamination and disposal should be placed in containers, e.g. autoclavable plastic bags, that are colour-coded according to whether the contents are to be autoclaved and/or incinerated. Alternative methods may be envisaged only if they remove and/or kill microorganisms 26
27
Handling and disposal procedures for contaminated materials and wastes • An identification and separation system for infectious materials and their containers should be adopted. National and international regulations must be followed. Categories should include: • Non-contaminated (non-infectious) waste that can be reused or recycled or disposed of as general, “household” waste • Contaminated (infectious) “sharps” – hypodermic needles, scalpels, knives and broken glass; these should always be collected in puncture-proof containers fitted with covers and treated as infectious • Contaminated material for decontamination by autoclaving and thereafter washing and reuse or recycling • Contaminated material for autoclaving and disposal • Contaminated material for direct incineration. 28
Sharps….. • After use, hypodermic needles should not be recapped, clipped or removed from disposable syringes. The complete assembly should be placed in a sharps disposal container. Disposable syringes, used alone or with needles, should be placed in sharps disposal containers and incinerated, with prior autoclaving if required. • Sharps disposal containers must be puncture-proof/-resistant and must not be filled to capacity. When they are three-quarters full they should be placed in “infectious waste” containers and incinerated, with prior autoclaving if laboratory practice requires it. Sharps disposal containers must not be discarded in landfills. 29
30
Contaminated (potentially infectious) materials for autoclaving and reuse • No pre-cleaning should be attempted of any contaminated (potentially infectious) materials to be autoclaved and reused. Any necessary cleaning or repair must be done only after autoclaving or disinfection. 31
Contaminated (potentially infectious) materials for disposal • Apart from sharps, which are dealt with above, all contaminated (potentially infectious) materials should be autoclaved in leak proof containers, e.g. autoclavable, colour-coded plastic bags, before disposal. • After autoclaving, the material may be placed in transfer containers for transport to the incinerator. If possible, materials deriving from health- care activities should not be discarded in landfills even after decontamination. • Discard containers, pans or jars, preferably unbreakable (e.g. plastic), should be placed at every work station. When disinfectants are used, waste materials should remain in intimate contact with the disinfectant (i.e. not protected by air bubbles) for the appropriate time, according to the disinfectant used. The discard containers should be decontaminated and washed before reuse. • Incineration of contaminated waste must meet with the approval of the public health and air pollution authorities, as well as that of the laboratory biosafety officer. 32

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Lecture 3 - Biosafety Levels 1 & 2.pptx

  • 1. LECTURE 3 MPhil – BIOTECHNOLOGY/ BIOCHEMSITRY (MORNING) BIOT-707 (1st/2ND SEMESTER) Biosafety Levels – 1 & 2 BY NAFEESA QUDSIA HANIF, PhD
  • 2. Purpose of Laboratory Design • Protect the Workers • Enable the Work • Secure the Facility • Protect the Environment • Comply with Regulations 2
  • 3. Table 1.Classification of infective microorganisms by risk group Risk Group 1 (no or low individual and community risk) • A microorganism that is unlikely to cause human or animal disease. Risk Group 2 (moderate individual risk, low community risk) • A pathogen that can cause human or animal disease but is unlikely to be a serious hazard to laboratory workers, the community, livestock or the environment. Laboratory exposures may cause serious infection, but effective treatment and preventive measures are available and the risk of spread of infection is limited. Risk Group 3 (high individual risk, low community risk) • A pathogen that usually causes serious human or animal disease but does not ordinarily spread from one infected individual to another. Effective treatment and preventive measures are available. Risk Group 4 (high individual and community risk) • A pathogen that usually causes serious human or animal disease and that can be readily transmitted from one individual to another, directly or indirectly. Effective treatment and preventive 3
  • 4. Table 2. Relation of risk groups to biosafety levels, practices and equipments 4 BSC, biological safety cabinet; GMT, good microbiological techniques
  • 5. Table 3.Summary of biosafety level requirements 5 1 2 3 4 Isolationa of laboratory No No Yes Yes Room sealable for decontamination No No Yes Yes Ventilation: — inward airflow No Desirable Yes Yes — controlled ventilating system No Desirable Yes Yes — HEPA-filtered air exhaust No No Yes/Nob Yes Double-door entry No No Yes Yes Airlock No No No Yes Airlock with shower No No No Yes Anteroom No No Yes — Anteroom with shower No No Yes/Noc No Effluent treatment No No Yes/Noc Yes Autoclave: — on site No Desirable Yes Yes — in laboratory room No No Desirable Yes — double-ended No No Desirable Yes Biological safety cabinets No Desirable Yes Yes Personnel safety monitoring capabilityd No No Desirable Yes Link for safety levels: https://www.youtube.com/watch?v=xNYASNEdgg8
  • 6. Basic Laboratories – Biosafety Level 1 & 2 6
  • 7. Figure 1.Biohazard warning sign for laboratory doors 7 BIOHAZARD Admittance to Authorized personnels only Biosafety Level: ______________________ Responsible Investigator:________________ In case of Emergency call:_______________ Day time phone: _______ Home phone: ______ Authorization for entrance must be obtained from the Responsible Investigator named above. Instructions: • Only authorized persons should be allowed to enter the laboratory working areas. • Laboratory doors should be kept closed. • Children should not be authorized or allowed to enter laboratory working areas. • Access to animal houses should be specially authorized. • No animals should be admitted other than those involved in the work of the laboratory.
  • 8. PERSONAL PROTECTION INSTRUCTIONS: • Laboratory coveralls, gowns or uniforms must be worn at all times for work in the laboratory. • Appropriate gloves must be worn for all procedures that may involve direct or accidental contact with blood, body fluids and other potentially infectious materials or infected animals. After use, gloves should be removed aseptically and hands must then be washed. • Personnel must wash their hands after handling infectious materials and animals, and before they leave the laboratory working areas. • Safety glasses, face shields (visors) or other protective devices must be worn when it is necessary to protect the eyes and face from splashes, impacting objects and sources of artificial ultraviolet radiation. • It is prohibited to wear protective laboratory clothing outside the laboratory, e.g. in canteens, coffee rooms, offices, libraries, staff rooms and toilets. • Open-toed footwear must not be worn in laboratories. • Eating, drinking, smoking, applying cosmetics and handling contact lenses is prohibited in the laboratory working areas. • Storing human foods or drinks anywhere in the laboratory working areas is prohibited. • Protective laboratory clothing that has been used in the laboratory must not be stored in the same lockers or cupboards as street clothing. 8
  • 9. PROCEDURES…… • Pipetting by mouth must be strictly forbidden. • Materials must not be placed in the mouth. Labels must not be licked. • All technical procedures should be performed in a way that minimizes the formation of aerosols and droplets. • The use of hypodermic needles and syringes should be limited. They must not be used as substitutes for pipetting devices or for any purpose other than parenteral injection or aspiration of fluids from laboratory animals. • All spills, accidents and overt or potential exposures to infectious materials must be reported to the laboratory supervisor. A written record of such accidents and incidents should be maintained. • A written procedure for the clean-up of all spills must be developed and followed. • Contaminated liquids must be decontaminated (chemically or physically) before discharge to the sanitary sewer. An effluent treatment system may be required, depending on the risk assessment for the agent(s) being handled. • Written documents that are expected to be removed from the laboratory need to be protected from contamination while in the laboratory. 9
  • 10. Laboratory working areas • The laboratory should be kept neat, clean and free of materials that are not pertinent to the work. • Work surfaces must be decontaminated after any spill of potentially dangerous material and at the end of the working day. • All contaminated materials, specimens and cultures must be decontaminated before disposal or cleaning for reuse. • Packing and transportation must follow applicable national and/or international regulations. • When windows can be opened, they should be fitted with arthropod- proof screens. 10
  • 11. Biosafety Management • It is the responsibility of the laboratory director (the person who has immediate responsibility for the laboratory) to ensure the development and adoption of a biosafety management plan and a safety or operations manual. • The laboratory supervisor (reporting to the laboratory director) should ensure that regular training in laboratory safety is provided. • Personnel should be advised of special hazards, and required to read the safety or operations manual and follow standard practices and procedures. The laboratory supervisor should make sure that all personnel understand these. A copy of the safety or operations manual should be available in the laboratory. • There should be an arthropod and rodent control programme. • Appropriate medical evaluation, surveillance and treatment should be provided for all personnel in case of need, and adequate medical records should be maintained. 11
  • 12. Laboratory design and facilities • In designing a laboratory and assigning certain types of work to it, special attention should be paid to conditions that are known to pose safety problems. These include: • Formation of aerosols • Work with large volumes and/or high concentrations of microorganisms • Overcrowding and too much equipment • Infestation with rodents and arthropods • Unauthorized entrance • Workflow: use of specific samples and reagents. • Examples of laboratory designs for Biosafety Levels 1 and 2 are shown in Figures 2 and 3, respectively. 12
  • 13. Figure 2. A typical Biosafety Level 1 laboratory (graphics kindly provided by CUH2A, Princeton, NJ, USA) 13
  • 14. Figure 3.A typical Biosafety Level 2 laboratory (graphics kindly provided by CUH2A, Princeton, NJ, USA). Procedures likely to generate aerosols are performed within a biological safety cabinet. Doors are kept closed and are posted with appropriate hazard signs. Potentially contaminated wastes are separated from the general waste stream. 14
  • 15. Design features 1. Ample space must be provided for the safe conduct of laboratory work and for cleaning and maintenance. 2. Walls, ceilings and floors should be smooth, easy to clean, impermeable to liquids and resistant to the chemicals and disinfectants normally used in the laboratory. Floors should be slip-resistant. 3. Bench tops should be impervious to water and resistant to disinfectants, acids, alkalis, organic solvents and moderate heat. 4. Illumination should be adequate for all activities. Undesirable reflections and glare should be avoided. 5. Laboratory furniture should be sturdy. Open spaces between and under benches, cabinets and equipment should be accessible for cleaning. 6. Storage space must be adequate to hold supplies for immediate use and thus prevent clutter on bench tops and in aisles. Additional long-term storage space, conveniently located outside the laboratory working areas, should also be provided. 7. Space and facilities should be provided for the safe handling and storage of solvents, radioactive materials, and compressed and liquefied gases. 15
  • 16. Design features (Cont’d.) 8. Facilities for storing outer garments and personal items should be provided outside the laboratory working areas. 9. Facilities for eating and drinking and for rest should be provided outside the laboratory working areas. 10. Hand-washing basins, with running water if possible, should be provided in each laboratory room, preferably near the exit door. 11. Doors should have vision panels, appropriate fire ratings, and preferably be self- closing. 12. At Biosafety Level 2, an autoclave or other means of decontamination should be available in appropriate proximity to the laboratory. 13. Safety systems should cover fire, electrical emergencies, emergency shower and eyewash facilities. 14. First-aid areas or rooms suitably equipped and readily accessible should be available. 16
  • 17. Design features (Cont’d.) 15. In the planning of new facilities, consideration should be given to the provision of mechanical ventilation systems that provide an inward flow of air without recirculation. If there is no mechanical ventilation, windows should be able to be opened and should be fitted with arthropod-proof screens. 16. A dependable supply of good quality water is essential. There should be no cross- connections between sources of laboratory and drinking-water supplies. An anti- backflow device should be fitted to protect the public water system. 17. There should be a reliable and adequate electricity supply and emergency lighting to permit safe exit. A stand-by generator is desirable for the support of essential equipment, such as incubators, biological safety cabinets, freezers, etc., and for the ventilation of animal cages. 18. There should be a reliable and adequate supply of gas. Good maintenance of the installation is mandatory. 19. Laboratories and animal houses are occasionally the targets of vandals. Physical and fire security must be considered. Strong doors, screened windows and restricted issue of keys are compulsory. Other measures should be considered and applied, as appropriate, to augment security (see Chapter 9). 17
  • 18. Laboratory Equipment • The laboratory director should, after consultation with the biosafety officer and safety committee (if designated), ensure that adequate equipment is provided and that it is used properly. Equipment should be selected to take account of certain general principles, i.e. it should be: • Designed to prevent or limit contact between the operator and the infectious material • Constructed of materials that are impermeable to liquids, resistant to corrosion and meet structural requirements • Fabricated to be free of burrs, sharp edges and unguarded moving parts • Designed, constructed and installed to facilitate simple operation and provide for ease of maintenance, cleaning, decontamination and certification testing; glassware and other breakable materials should be avoided, whenever possible. • Detailed performance and construction specifications may need to be consulted to ensure that the equipment possesses the necessary safety features 18
  • 19. Essential biosafety equipment • Pipetting aids – to avoid mouth pipetting. Many different designs are available. • Biological safety cabinets, to be used whenever: • infectious materials are handled; • there is an increased risk of airborne infection • procedures with a high potential for producing aerosols are used; these may include centrifugation, grinding, blending, vigorous shaking or mixing, sonic disruption, opening of containers of infectious materials whose internal pressure may be different from the ambient pressure, intranasal inoculation of animals, and harvesting of infectious tissues from animals and eggs. • Plastic disposable transfer loops. Alternatively, electric transfer loop incinerators may be used inside the biological safety cabinet to reduce aerosol production. 19
  • 20. Essential biosafety equipment Cont’d. • Screw-capped tubes and bottles. • Autoclaves or other appropriate means to decontaminate infectious materials. • Plastic disposable Pasteur pipettes, whenever available, to avoid glass. • Equipment such as autoclaves and biological safety cabinets must be validated with appropriate methods before being taken into use. Recertification should take place at regular intervals, according to the manufacturer’s instructions. 20
  • 21. Health and Medical Surveillance • The employing authority, through the laboratory director, is responsible for ensuring that there is adequate surveillance of the health of laboratory personnel. The objective of such surveillance is to monitor for occupationally acquired diseases. Appropriate activities to achieve these objectives are: • Provision of active or passive immunization where indicated. • Facilitation of the early detection of laboratory-acquired infections. • Exclusion of highly susceptible individuals (e.g. pregnant women or immuno- compromised individuals) from highly hazardous laboratory work • Provision of effective personal protective equipment and procedures. 21
  • 22. Guidelines for the surveillance of laboratory workers - Handling microorganisms at Biosafety Level 1 • Historical evidence indicates that the microorganisms handled at this level are unlikely to cause human disease or animal disease of veterinary importance. Ideally, however, all laboratory workers should undergo a pre-employment health check at which their medical history is recorded. Prompt reporting of illnesses or laboratory accidents is desirable and all staff members should be made aware of the importance of maintaining GMT. 22
  • 23. Guidelines for the surveillance of laboratory workers - handling microorganisms at Biosafety Level 2 • A pre-employment or preplacement health check is necessary. The person’s medical history should be recorded and a targeted occupational health assessment performed. • Records of illness and absence should be kept by the laboratory management. • Women of childbearing age should be made aware of the risk to an unborn child of occupational exposure to certain microorganisms, e.g. rubella virus. The precise steps taken to protect the fetus will vary, depending on the microorganisms to which the women may be exposed. 23
  • 24. Training Human error and poor technique can compromise the best of safeguards to protect the laboratory worker. Thus, a safety-conscious staff, well informed about the recognition and control of laboratory hazards, is key to the prevention of laboratory. Staff training should always include information on safe methods for highly hazardous procedures that are commonly encountered by all laboratory personnel and which involve: • Inhalation risks (i.e. aerosol production) when using loops, streaking agar plates, pipetting, making smears, opening cultures, taking blood/serum samples, centrifuging, etc. • Ingestion risks when handling specimens, smears and cultures • Risks of percutaneous exposures when using syringes and needles • Bites and scratches when handling animals • Handling of blood and other potentially hazardous pathological materials • Decontamination and disposal of infectious material. 24
  • 25. Waste Handling…… • Waste is anything that is to be discarded. • In laboratories, decontamination of wastes and their ultimate disposal are closely interrelated. In terms of daily use, few if any contaminated materials will require actual removal from the laboratory or destruction. Most glassware, instruments and laboratory clothing will be reused or recycled. The overriding principle is that all infectious materials should be decontaminated, autoclaved or incinerated within the laboratory. • The principal questions to be asked before discharge of any objects or materials from laboratories that deal with potentially infectious microorganisms or animal tissues are: • Have the objects or materials been effectively decontaminated or disinfected by an approved procedure? • If not, have they been packaged in an approved manner for immediate on-site incineration or transfer to another facility with incineration capacity? • Does the disposal of the decontaminated objects or materials involve any additional potential hazards, biological or otherwise, to those who carry out the immediate disposal procedures or who might come into contact with discarded items outside the facility? 25
  • 26. Decontamination…… • Steam autoclaving: It is the preferred method for all decontamination processes. Materials for decontamination and disposal should be placed in containers, e.g. autoclavable plastic bags, that are colour-coded according to whether the contents are to be autoclaved and/or incinerated. Alternative methods may be envisaged only if they remove and/or kill microorganisms 26
  • 27. 27
  • 28. Handling and disposal procedures for contaminated materials and wastes • An identification and separation system for infectious materials and their containers should be adopted. National and international regulations must be followed. Categories should include: • Non-contaminated (non-infectious) waste that can be reused or recycled or disposed of as general, “household” waste • Contaminated (infectious) “sharps” – hypodermic needles, scalpels, knives and broken glass; these should always be collected in puncture-proof containers fitted with covers and treated as infectious • Contaminated material for decontamination by autoclaving and thereafter washing and reuse or recycling • Contaminated material for autoclaving and disposal • Contaminated material for direct incineration. 28
  • 29. Sharps….. • After use, hypodermic needles should not be recapped, clipped or removed from disposable syringes. The complete assembly should be placed in a sharps disposal container. Disposable syringes, used alone or with needles, should be placed in sharps disposal containers and incinerated, with prior autoclaving if required. • Sharps disposal containers must be puncture-proof/-resistant and must not be filled to capacity. When they are three-quarters full they should be placed in “infectious waste” containers and incinerated, with prior autoclaving if laboratory practice requires it. Sharps disposal containers must not be discarded in landfills. 29
  • 30. 30
  • 31. Contaminated (potentially infectious) materials for autoclaving and reuse • No pre-cleaning should be attempted of any contaminated (potentially infectious) materials to be autoclaved and reused. Any necessary cleaning or repair must be done only after autoclaving or disinfection. 31
  • 32. Contaminated (potentially infectious) materials for disposal • Apart from sharps, which are dealt with above, all contaminated (potentially infectious) materials should be autoclaved in leak proof containers, e.g. autoclavable, colour-coded plastic bags, before disposal. • After autoclaving, the material may be placed in transfer containers for transport to the incinerator. If possible, materials deriving from health- care activities should not be discarded in landfills even after decontamination. • Discard containers, pans or jars, preferably unbreakable (e.g. plastic), should be placed at every work station. When disinfectants are used, waste materials should remain in intimate contact with the disinfectant (i.e. not protected by air bubbles) for the appropriate time, according to the disinfectant used. The discard containers should be decontaminated and washed before reuse. • Incineration of contaminated waste must meet with the approval of the public health and air pollution authorities, as well as that of the laboratory biosafety officer. 32