Download Module 2

Survey
yes no Was this document useful for you?
   Thank you for your participation!

* Your assessment is very important for improving the workof artificial intelligence, which forms the content of this project

page
1
page
2
page
3
page
4
page
5
page
6
page
7
page
8
page
9
page
10
page
11
page
12
page
13
page
14
page
15
page
16
page
17
page
18
page
19
page
20
page
21
page
22
page
23
page
24
page
25
page
26
page
27
page
28
page
29
page
30
page
31
page
32
page
33
page
34
page
35
page
36
page
37
page
38
page
39
page
40
page
41
page
42
page
43
page
44
page
45
page
46
page
47
page
48
page
49
page
50
page
51
page
52
page
53
page
54
page
55
page
56
page
57
page
58
page
59
page
60
page
61
page
62
page
63
page
64
page
65
page
66
page
67
page
68
page
69
page
70
page
71
page
72
page
73
page
74
page
75
page
76
page
77
page
78
page
79
page
80
page
81
page
82
page
83
page
84
page
85
page
86
page
87
page
88
page
89
page
90
page
91
page
92
page
93
page
94
page
95
page
96
page
97
page
98
page
99
page
100
page
101
page
102
page
103
page
104
page
105
page
106
page
107
page
108
page
109
page
110
page
111
page
112
page
113
page
114
page
115
page
116
page
117
page
118
page
119
page
120
page
121
page
122
page
123
page
124
page
125
page
126
page
127
page
128
page
129
page
130
page
131
page
132
page
133
page
134
page
135
page
136
page
137
page
138
page
139
page
140
page
141
page
142
page
143
page
144
page
145
page
146
page
147
page
148
page
149
page
150
page
151
page
152
page
153
Document related concepts

Marburg virus disease wikipedia , lookup

History of biological warfare wikipedia , lookup

Biological warfare wikipedia , lookup

United States biological defense program wikipedia , lookup

Bioterrorism wikipedia , lookup

Transcript 
Module 2
Principles
Definition
Biohazard
An agent of biological origin that has the
capacity to produce deleterious effects on
humans, i.e. microorganisms, toxins and
allergens derived from those organisms; and
allergens and toxins derived from higher
plants and animals.
2.1
Introduction
Development of Biosafety Practices
n
1941 - Meyer and Eddie
n
n
74 lab associated brucellosis infections
in US
1949 - Sulkin and Pike
n
n
222 viral infections (21 fatal)
Only 27% related to known accidents
2.1
Introduction
Development of Biosafety Practices
n
1951, 1965, 1976 - Sulkin and Pike
n
n
n
n
Surveys for lab-associated infections
More than 5,000 labs
Cumulative total of 3,921 cases cited
Most commonly reported:
• Hepatitis
• Tuberculosis
• Typhoid
• Venezuelan Equine Encephalitis
• Brucellosis
• Tularemia
2.1
Introduction
Development of Biosafety Practices
n
1951,1965, 1976 - Sulkin and Pike
n
n
Fewer than 20% associated with known
accidents
Exposure to infectious aerosols plausible
(but unconfirmed) for >80% of reported
cases
2.1
Introduction
Why Biosafety Practices?
Protection:
n workers
n “products”
n co-workers
n lab support personnel
n environment
2.1
Introduction
Chain of Infection
Reservoir of pathogen
Portal of escape
sk
Ri
Transmission
s/
e
c
cti ent
a
r
P i pm
Equ
E
PP
m
ss
se
As
Route of entry/infectious dose
Susceptible host
un
m
Im
t
en
Incubation period
ion
t
a
iz
ce
n
a
l
eil
v
r
Su
2.1
Principles
General Lab Requirements
n
n
Knowledgeable
supervisor
Knowledgeable personnel
n
n
n
Aware of potential hazards
Proficient in practices &
techniques
Lab specific biosafety
manual
2.2
Principles
General Lab Requirements
n
n
Biosafety Levels (BSLs)
Laboratory Practice and Technique
n
n
n
n
Standard Practices
Special Practices
Safety Equipment (Primary Barriers)
Facility Design and Construction
(Secondary Barriers)
2.1
Principles
General Lab Requirements
n
n
Biosafety cabinets (BSCs) - BSL 2/3
Personal protective clothing
n
n
n
n
n
Gloves
Gowns
Eye and face protection
Pipetting Devices
Safety centrifuge cups and rotors
2.1
Principles
Definition
Biosafety
The application of
combinations of laboratory
practice and procedure,
laboratory facilities, and
safety equipment when
working with potentially
infectious microorganisms.
2.1
Principles
Biosafety Levels
n
n
n
n
BSL1 - agents not known to cause disease.
BSL2 - agents associated with human
disease.
BSL3 - indigenous/exotic agents associated
with human disease and with potential for
aerosol transmission.
BSL4 - dangerous/exotic agents of life
threatening nature.
2.1
Biosafety Level 1
Introduction
uitable for work involving wellcharacterized agents not known to
cause disease in healthy adult humans
and of minimal potential hazard to
laboratory personnel and the
environment.
2.3
Biosafety Level 1
Introduction
Examples:
n
n
n
n
Bacillus subtilis
Naegleria gruberi
Infectious canine hepatitis virus
E. coli
2.3
Biosafety Level 1
Facility Design (Secondary Barrier)
2.3
Biosafety Level 1
Facility Design (Secondary Barrier)
Requirements:
n Laboratories have doors
n Sink for hand washing
n Work surfaces easily cleaned
n Bench tops are impervious to water
n Sturdy furniture
n Windows fitted with flyscreens
2.3
Biosafety Level 1
Facility Design (Secondary Barrier)
Easily cleaned
and
decontaminated
2.3
Biosafety Level 1
Facility Construction (Secondary Barrier)
Requirements:
n
Location - not separated
Structure - normal construction
n
Ventilation - none
n
2.3
Biosafety Level 1
Standard Microbiological Practices
n
n
n
Restrict or limit
access when working
Prohibit eating,
drinking and smoking
Prohibit mouth
pipetting
2.3
Biosafety Level 1
Standard Microbiological Practices
Use
mechanical
pipetting
devices
2.3
Biosafety Level 1
Standard Microbiological Practices
Wash hands
2.3
Biosafety Level 1
Standard Microbiological Practices
n
n
n
n
Minimize splashes and aerosols
Decontaminate work surfaces daily
Decontaminate wastes
Maintain insect & rodent control
program
2.3
Biosafety Level 1
Safety Equipment (Primary Barriers)
Protective clothing
n Lab coat
n Gloves
2.3
Biosafety Level 1
Safety Equipment (Primary Barriers)
Personal protective equipment
n
n
Face protection
Eye protection
2.3
Biosafety Level 1
Special Practices
2.3
Biosafety Level 1
Training Requirements
n
Supervisor
n Scientist with general training in
microbiology or related science
n
Lab Personnel
n Specific training in lab procedures
2.3
Biosafety Level 2
Introduction
uitable for work involving agents
of moderate potential hazard to
personnel and the environment.
2.4
Biosafety Level 2
Introduction
Examples:
n
n
n
n
Measles virus
Salmonellae
Toxoplasma spp.
Hepatitis B virus
* Immunization or antibiotic treatment is available
2.4
Biosafety Level 2
Introduction
Examples:
n
n
Bloodborne pathogens
Human body fluids/particularly when visibly
contaminated with blood
* Extreme precaution with contaminated needles or
sharp instruments
2.4
Biosafety Level 2
Facility Design (Secondary Barriers)
2.4
Biosafety Level 2
Facility Design (Secondary Barriers)
Requirements:
§ Laboratories have lockable doors
§ Sink for hand washing
§ Work surfaces easily cleaned
§ Bench tops are impervious to water
§ Sturdy furniture
2.4
Biosafety Level 2
Facility Design (Secondary Barriers)
Requirements (cont.):
§ Biological safety cabinets installed as
needed
§ Adequate illumination
§ Eyewash readily available
§ Air flows into lab without re-circulation to
non-lab areas
§ Windows fitted with flyscreens
2.4
Biosafety Level 2
Facility Design (Secondary Barrier)
Restricted
access when
work in
progress
2.4
Biosafety Level 2
Laboratory Facilities (Secondary Barriers)
n
BSL-1 Facilities PLUS:
n
n
Autoclave
available
Eyewash station
available
2.4
Biosafety Level 2
Facility Construction (Secondary Barrier)
Requirements:
n
Location - separated from public areas
n
Structure - normal construction
n
Ventilation - directional
2.4
Biosafety Level 2
Standard Microbiological Practices
2.4
Biosafety Level 2
Safety Equipment (Primary Barriers)
n
Use biosafety cabinets (class II) for
work with infectious agents involving:
n Aerosols and splashes
n Large volumes
n High concentrations
2.4
Biosafety Level 2
Safety Equipment (Primary Barriers)
n
Class II Biosafety
Cabinet
n
Airflow
2.4
Biosafety Level 2
Safety Equipment (Primary Barriers)
n
Class II Biosafety Cabinet
n
Equipment layout
2.4
Biosafety Level 2
Safety Equipment (Primary Barriers)
n
Class II Biosafety
Cabinet
n
Technique
2.4
Biosafety Level 2
Special Practices
Supervision
§ Supervisor is a competent scientist with
increased responsibilities
§ Limits access if immunocompromised
§ Restricts access to immunized
Lab Personnel
§ Aware of potential hazards
§ Proficient in practices/techniques
2.4
Biosafety Level 2
Special Practices
Needles & Sharps Precautions
n
n
Use sharps containers
DON’T break, bend, re-sheath or reuse
syringes or needles
2.4
Biosafety Level 2
Special Practices
Needles & Sharps Precautions (cont.)
n
DON’T place needles or sharps in office
waste containers
2.4
Biosafety Level 2
Special Practices
Needles and Sharps Precautions (cont.)
n
DON’T touch broken glass with hands
2.4
Biosafety Level 2
Special Practices
Needles and Sharps Precautions (cont.)
n
Use plasticware
2.4
Biosafety Level 2
Special Practices
n
n
n
n
Policies and procedures for entry
Biohazard warning signs
Biosafety manual specific to lab
Training with annual updates
2.4
Biosafety Level 2
Special Practices
n
Use leak-proof transport containers
2.4
Biosafety Level 2
Special Practices
n
n
Immunizations
Baseline serum samples
2.4
Biosafety Level 2
Special Practices
n
n
n
Decontaminate work surfaces
Report spills and accidents
No animals in laboratories
2.4
Biosafety Level 3
Introduction
Suitable for work with infectious
agents which may cause serious or
potentially lethal disease as a result
of exposure by the inhalation route.
2.5
Biosafety Level 3
Introduction
Exposure potential to pathogens
spread by aerosol
n Infection serious, possibly lethal
n Examples:
n
M. tuberculosis
n St. Louis encephalitis virus
n Coxiella burnetii
n
2.5
Biosafety Level 3
Laboratory Facilities (Secondary Barriers)
2.5
Biosafety Level 3
Laboratory Facilities (Secondary Barriers)
n
BSL-1 and 2 Facilities PLUS:
n
Separate building or isolated zone
n
Double door entry
n
Directional inward airflow
n
Single-pass air; 10-12 air changes/hour
2.5
Biosafety Level 3
Laboratory Facilities (Secondary Barriers)
n
BSL-1 and 2 Facilities PLUS (cont.):
n
n
n
Enclosures for aerosol generating
equipment
Room penetrations sealed
Walls, floors and ceilings are water
resistant for easy cleaning
2.5
Biosafety Level 3
Laboratory Facilities ( Secondary Barriers)
n
BSL-1 and 2 Facilities PLUS:
n Vacuum lines protected with liquid
disinfectant traps or HEPA filters
2.5
Facility Design
(Tertiary Barriers)
BSL 3
CDC
Containment
Laboratory
BSL 4
2.5
Facility Design
(Tertiary Barriers)
n
n
Lab structure
Lab ventilation
2.5
Biosafety Level 3
Standard Microbiological Practices
2.5
Biosafety Level 3
Safety Equipment (Primary Barriers)
n
BSL-1 and 2 Safety Equipment PLUS:
n
BSC class
II or III to
manipulate
infectious
material
2.5
Biosafety Level 3
Safety Equipment (Primary Barriers)
n
BSL-1 and 2 Safety Equipment PLUS:
n
Respiratory protection
may be indicated
2.5
Biosafety Level 3
Special Practices
n
BSL-2 Special Practices PLUS:
n
n
n
Work in certified BSC
Use bioaerosolcontaining equipment
Decontaminate spills
promptly
2.5
Biosafety Level 3
Special Practices
Supervision
§ Supervisor is a competent scientist
experienced working with agents
§ Establishes criteria for entry
§ Restricts access
§ Develops policies/procedures
§ Trains lab personnel
2.5
Biosafety Level 3
Special Practices
Lab Personnel
§ Strictly follow guidelines
§ Demonstrate proficiency
§ Receive appropriate training
§ Report incidents
§ Participate in medical surveillance
2.5
Biosafety Level 4
Introduction
Suitable for work with dangerous
and exotic agents that pose a high
individual risk of aerosoltransmitted laboratory infections
and life-threatening disease.
2.6
Biosafety Level 4
Introduction
Exposure potential to pathogens
spread by aerosol or with
unknown risk of transmission
n Infection possibly lethal
n Examples:
n
Ebola Zaire
n Sin Nombre virus
n Rift Valley Fever
n
Ebola
Ebola Zaire
Zaire
2.6
Biosafety Level 4
Laboratory Facilities (Secondary Barriers)
2.6
Biosafety Level 4
Laboratory Facilities (Secondary Barriers)
n
BSL-1, 2, and 3 Facilities
PLUS:
n Separate building or
isolated zone
n Double door entry
n Directional inward airflow
n Single-pass air
n Dedicated supply and
exhaust, vacuum, and
decon systems
BSL4
2.6
Biosafety Level 4
Laboratory Facilities (Secondary Barriers)
n
BSL-1, 2 and 3 Facilities PLUS (cont.):
n Enclosures for aerosol generating
equipment
n Double door autoclaves
n Room penetrations sealed
n Walls, floors and ceilings are sealed to
form an internal seal
2.6
Biosafety Level 4
Laboratory Facilities (Secondary Barriers)
n
BSL-1, 2 and 3 Facilities PLUS (cont.):
n Connecting inner and outer doors interlocked to prevent simultaneous
opening
n Liquid effluents are decontaminated by an
approved method and certified before
discharge
n Communication system between inside
and outside of the lab
2.6
Biosafety Level 4
Laboratory Facilities ( Secondary Barriers)
n
BSL 1, 2, and 3 Facilities PLUS:
n Emergency breathing air
n Emergency generator
n Emergency exit
2.6
Biosafety Level 4
Standard Microbiological Practices
2.6
Biosafety Level 4
Safety Equipment (Primary Barriers)
n
BSL 1, 2, and 3 Safety Equipment PLUS:
n
Class II (B2) or III biological safety cabinets
to manipulate
infectious
material
2.6
Biosafety Level 4
Safety Equipment (Primary Barriers)
n
BSL 1, 2, and 3 Safety
Equipment PLUS:
n
Positive pressure
personnel suit
2.6
Biosafety Level 4
Special Practices
n
BSL 3 Special
Practices PLUS:
n
n
Decontaminate all
liquid effluent
Decontaminate all
solid wastes
2.6
Biosafety Level 4
Special Practices
§ Controlled access
§ Personnel enter facility through
changing room where they are
required to change into
laboratory clothing
§ Showers are required upon
exit from the laboratory
§ Supplies enter lab through
double-door autoclave or
fumigation chamber
3.5
Biosafety Level 4
Special Practices
Supervision
§ Supervisor is a competent scientist
trained and experienced working with
agents
§ Establishes criteria for entry
§ Restricts access
§ Develops policies/procedures
§ Trains lab personnel
2.6
Biosafety Level 4
Special Practices
Lab Personnel
§ Strictly follow guidelines
§ Demonstrate proficiency
§ Receive appropriate training
§ Report incidents
§ Receive available immunizations
§ Participate in medical surveillance
2.6
Principles of Biosafety
Summary
n
BSL 1 - 4
n
n
n
n
n
Standard Practices
Special Practices
Safety Equipment (Primary Barriers)
Laboratory Facilities (Secondary
Barriers)
Building (Tertiary Barriers)
2.6
2.7
Biological Safety Cabinets
Purpose
n
n
n
Product protection
Personal protection
Environmental
protection
2.7
Biological Safety Cabinets
Types
A. Class I
n
n
inward airflow protects worker
exhaust to outside (w/wo HEPA filter)
B. Class II
n
n
n
n
worker, product, environmental protection
“sterile” work area
use for work with aerosol-transmissible microorganisms
use also for tissue culture/ virology
C. Class III
n
n
totally enclosed, ventilated, air-tight
suitable for work with BSL3/4 agents
2.7
Biological Safety Cabinets
Types
Class II
n
n
n
n
Type A
Type B3
Type B1
Type B2
30% exhausted to room
30% exhausted to outside
70% exhausted to outside
100% exhausted to outside
2.7
Biological Safety Cabinets
Component
HEPA Filter
n “High efficiency particulate air” filter
n Traps particulates only; chemicals,
fumes, vapors pass through
n Traps particulates 0.3u
2.7
Biological Safety Cabinets
Component
HEPA Filter
n Metal or wood framed
n Continuous sheet of
flat filter medium with
aluminum separators
n Gasket sealed
n Adhesive bond
between filter pack
and frame
2.7
Biological Safety Cabinets
Operating Location
§ Isolated from other work areas
§ Removed from high traffic areas
§ Away from airflow ducts
§ Away from laboratory entry doors
2.7
Biological Safety Cabinets
Airflow
Exhaust
Typical Class II
Intake
100
ft/min
2.7
Biological Safety Cabinets
Operating Procedure
1.
2.
3.
4.
5.
6.
7.
8.
Load BSC with all needed supplies.
Turn BSC on and allow to run for 10-15 minutes.
Check inward airflow with a piece of tissue.
Enter straight into cabinet and perform work in a
slow, methodical manner.
At end of work, decontaminate all items to be
taken out of cabinet.
Decontaminate interior of BSC.
Allow cabinet to run for 10-15 minutes.
Shut off.
2.7
Biological Safety Cabinets
Safe Operation
■
■
■
■
■
Always enter straight into cabinet - no
sweeping motions
Place materials well within the cabinet - not
on front grill
Place discard pan within cabinet
Watch for disruptions of laminar air flow
Decontaminate materials before removal
from cabinet
2.7
Biological Safety Cabinets
Safe Operation
■
■
■
■
■
Not designed for chemical use
May use for non-volatile toxic chemicals or
low-level radioactive materials
May use for “minute” amounts of volatile
chemicals
Ensure annual certification
Place all work materials into cabinet before
starting
2.7
Biological Safety Cabinets
Safe Operation
CAUTIONS
n Chemicals may damage HEPA filter
n
n
Volatile chemicals NOT retained by HEPA
filter
n
n
Exposure risk - chemical/infectious agents
Exposes personnel if not exhausted
BSC fans NOT spark proof
n
n
Chemical use may result in fire/ explosion
Never use NFPA 4 flammables
2.7
2.8
Centrifuges
Types
Microcentrifuges
Speeds (rpm)
~15,000
Low/high speed
2,000 – 20,000
Ultracentrifuges
~ 120,000
2.8
Centrifuges
Hazards
n
Mechanical failure of machine
n
Lab equipment failure (tubes etc.)
n
Aerosol generation
n
Operator error
2.8
Centrifuges
Operating Procedure
1.
2.
3.
4.
Check tubes for cracks/chips.
Use matched sets of tubes, buckets etc.
Tightly seal all tubes and safety cups.
Ensure that rotor is locked to spindle
and bucket seated.
5. Close lid during operation.
6. Allow to come to complete stop before
opening.
2.8
Centrifuges
Safe Operation
§
§
§
§
§
Use safety cups whenever possible
Disinfect weekly and after all spills or
breakage's
Lubricate O-rings and rotor threads
weekly
Do not use rotors that have been dropped
Contact your centrifuge rep for specific
information
2.8
2.9
Shipping Biological Specimens
Guideline Documents
n
Recommendations
of the United
Nations Committee
on Dangerous
Goods
2.9
Shipping Biological Specimens
Regulations
n
n
n
n
n
PHS: 42 CFR Part 72.
DOT: 49 CFR Part 171-178
USPS: Domestic Mail
Manual
IATA: International Air
Transport Association
ICAO: International Civil
Aviation Organization
2.9
Shipping Biological Specimens
Infectious Substance
Definition
n Contains or has high probability of
containing an infectious material…known or
reasonably believed to cause disease in
humans or animals
n
n
n
virus, prion, genetic elements
bacterium, rickettsia, parasite, fungus
Contains a microbial toxin known to be
pathogenic
2.9
Shipping Biological Specimens
Infectious Substance
Packaging
n Primary Container
n
n
Positive seal
Absorbent material
2.9
Shipping Biological Specimens
Infectious Substance
Packaging
n Secondary packaging
n
Watertight/leakproof
2.9
Shipping Biological Specimens
Infectious Substance
Packaging
n Between Secondary and Outer
Container
n
n
List of Contents
Shippers label
n
n
n
Name
Address
Phone number
2.9
Shipping Biological Specimens
Infectious Substance
Packaging
n Outer container
2.9
Shipping Biological Specimens
Infectious Substance
Packaging
n Performance tests
n
49 CFR 178.609
2.9
Shipping Biological Specimens
Infectious Substance
Packaging label
2.9
Shipping Biological Specimens
Infectious Substance
Containers
2.9
Shipping Biological Specimens
Clinical Specimen
Definition
Human or animal material…collected
for the purpose of diagnosis or
research….not known to contain
viable infectious agents
2.9
Shipping Biological Specimens
Clinical Specimen
Packaging
n Primary receptacle
n
Positive seal
n
Biohazard label
n
Absorbent material
2.9
Shipping Biological Specimens
Clinical Specimen
Packaging
n Between the secondary and outer
packaging
n
List of contents
2.9
Shipping Biological Specimens
Clinical Specimen
Packaging
n Outer packaging
2.9
Shipping Biological Specimens
Clinical Specimen
Package Label
2.9
Shipping Biological Specimens
Clinical Specimen
Packaging
n Performance test
2.9
Biosafety Manuals
Components
n
Biosafety Level Descriptions
n
n
n
n
n
n
Standard Practices & Principles
Special Practices & Procedures
Containment Devices
Facility Design
Animal Safety Practices
Agent Summary Statements
2.9
Biosafety Manuals
Components
n
n
n
n
n
Equipment Descriptions
Specimen Handling
Security
Waste
Special Lab Practices
n
n
Tissue culture
Toxins
2.9
2.10
Decontamination
Definition
n
Sterilization
The use of a physical or chemical procedure
to destroy all microbial life, including large
numbers of highly resistant bacterial
spores.
2.10
Decontamination
Definition
n
Disinfection
The use of a physical or chemical procedure
to virtually eliminate all recognized
pathogenic microorganisms but not all
microbial forms (bacterial endospores) on
inanimate objects.
2.10
Decontamination
Definition
n
Antisepsis
A germicide that is used on skin or living
tissue for the purpose of inhibiting or
destroying microorganisms.
2.10
Decontamination
Agent Selection
Degree of microbial killing required
n Nature of item/surface to be treated
n Ease of use
n Safety
n Cost
n
2.10
Decontamination
Agent Efficacy
n
n
n
n
n
n
n
n
Type of organism
Number of organisms
Amount of organic material present
Type & configuration of material to be treated
Type & concentration of germicide
Time and temperature or exposure
pH
Humidity
2.10
Decontamination
Methods
Heat
n Chemical
n Radiation
n
2.10
Decontamination
Heat
n
Types
n
n
n
Moist – steam
Dry
Incineration
*The most effective method of sterilization
2.10
Decontamination
Heat
n
Steam sterilization practices
n
n
n
n
Ensure proper functioning of autoclave
Vessels should not be capped or plugged
Large loads require longer contact time
Excessive amounts of liquid should not be
added to load
2.10
Decontamination
Heat
n
Steam sterilization
verification
n
n
n
n
Direct assay
Thermocouples
Chemical indicators
Biological indicators
(Bacillus
stearothermophilis)
2.10
Decontamination
Heat
n
Dry heat sterilization
n
n
Denaturation of proteins: 1600 – 1700 C/2-4
hours
Effective on impervious non-organic
materials like glass
2.10
Decontamination
Heat
n
Incineration
n
n
Method of choice
for animal
carcasses
Requires certified
incinerator
2.10
Decontamination
Chemical
n
Types
n
n
Liquids, I.e. chlorox,
hydrogen peroxide
Gases, I.e. ethylene
oxide
2.10
Decontamination
Chemical
n
Agent selection - complexity
n
n
n
Over 14,000 registered products
Over 300 active ingredients
14 ingredients present in 92% of products
2.10
Decontamination
Chemical
n
Agent selection - activity
n
n
n
HLD – high level disinfection
ILD – intermediate level disinfection
LLD – low level disinfection
2.10
Decontamination
Chemical
n
High level disinfection - sporocides
n
n
n
Kills all microorganisms except high
numbers of bacterial spores
Require 5-10 min. exposure
Examples: aldehydes, hydrogen peroxide,
paracetic acid
2.10
Decontamination
Chemical
n
Intermediate level disinfection tuberculocides
n
n
n
Kills M. tuberculosis var. bovis and all
vegetative bacteria, fungi, and most
viruses
Require minimum 20 min. exposure
Examples: phenolics, iodophores, chlorine
compounds, alcohols
2.10
Decontamination
Chemical
n
Low level disinfection – hospital
germicides used for housekeeping
n
n
n
Kills most vegetative bacteria and some
fungi, but not M. tuberculosis var. bovis
Require minimum 20 min. exposure
Examples: quartenary ammonium
compounds
2.10
Decontamination
Summary
Bacterial Spores
B. subtilis
Mycobacterium
MTB var. bovis
Non-lipid Viruses
PolioRhinoFungi
Cryptococcus sp,
Candida sp.
Vegatative Bacteria
Pseudomonas sp.
Staphylococcus sp.
Salmonella sp.
Lipid Viruses
Herpes
CMV
HBV
HIV
Sterilization
HLD
ILD
LLD
2.10
Decontamination
Chemical
n
General Lab Use - Hypochlorite Solutions
n
Large Spills/Large Organic Load
n
n
Small Spills/Virus Inactivation
n
n
undiluted from bottle
10% - 1:9
General Surface Disinfection
n
1% - 1:99
2.10
Decontamination
2.10
2.11
Biological Waste
n
Types
n
n
n
n
n
cultures, stocks, isolates
materials containing or contaminated with
blood
sharps
pipettes, wrappers, tips
All materials used in the lab
2.11
Biological Waste
nDisposal
n
n
n
puncture-proof, leak-proof, sealable
receptacles
avoid over-filling
dispose properly
2.11
Biological Waste
§ Disposal
- Never place lab waste into office waste containers
- Place sharps into “sharps” container
- Line discard containers with autoclave bag
- Decontaminate discard pans before they leave the
lab:
1. Disinfect outside
2. Label
3. Tape ends with
autoclave
4. Tape
5. Secure for transport to
autoclave
2.11
Biological Waste
Decontamination
n
n
To render the object/material safe by
reducing or removing the bioburden
Methods
n
n
n
n
chemical ... match, contact time
physical ... Heat, steam and pressure
incineration
other choices, i.e. shredding + chemical
2.11
2.12
Medical Surveillance
Criteria
n
n
n
Based on risk assessment
Pre-placement
n evaluate physical requirements
Periodic review
2.12
Medical Surveillance
Risk Assessment
n
n
n
The probability of infection
Implies an estimate of numbers exists
Predict an outcome given similar events
2.12
Medical Surveillance
Risk Assessment
n
n
n
n
n
What is the natural host?
Does agent cross species barriers?
Wild-type agent or attenuated?
Infectious for normal healthy adult?
What if adult is immunocompromised?
2.12
Medical Surveillance
Risk Assessment
n
Mode of transmission?
n contact
n fomites
n mucous membrane exposure
n ingestion
n inoculation or insect bites
n inhalation
n sex
2.12
Medical Surveillance
Risk Assessment
n
n
n
n
n
Volume being manipulated?
Concentration of agent?
Infectious dose?
Past history of lab-associated infection?
Secondary spread in community?
2.12
Medical Surveillance
Risk Assessment
n
Prophylaxis
n
n
n
n
Immunizations available?
Pharmaceuticals?
Effectiveness?
Post-Exposure
n
n
n
Anti-microbial agents?
Pharmaceuticals?
Effectiveness?
2.12
Medical Surveillance
Risk Assessment
n
Dealing with an unknown agent?
n epidemiological data
n patterns parallel to other agents
n data from animal studies
n route of infection
2.12
Medical Surveillance
Risk Management
n
Top management
n
n
n
Supervisor
n
n
n
overall safety policy
resource allocation
implement policies
training, practices & procedures, access
Workers
n
n
strict & rigorous attention to details of
practices and procedures
report incidents and exposures
2.12
Medical Surveillance
Risk Management
n
n
n
n
n
Occupational Health Clinic
Immunizations, chemotherapy
Medical surveillance programs
Incident (emergency) response
Incident investigation
2.12
2.13
Emergency Response
Personal Contamination
1. Alert co-workers
2. Clean exposed surface with soap/water,
eyewash (eyes), or saline (mouth)
3. Apply first aid and treat as an emergency
4. Notify supervisor or security desk (after
hours)
5. Report to medical clinic for
treatment/counseling
2.13
Emergency Response
Surface Contamination
1.
2.
3.
4.
5.
Alert co-workers
Define/isolate contaminated area
Put on appropriate PPE
Remove glass/lumps with forceps or scoop
Apply absorbent towel(s) to spill; remove bulk
& reapply if needed
6. Apply disinfectant to towel surface
6. Allow adequate contact time (20”)
8. Remove towel, mop up; clean with alcohol or
soap/water
9. Properly dispose of materials
10. Notify supervisor
2.13
Related documents
Biosafety Levels - A Simple Understanding
Biosafety Levels - A Simple Understanding
CELL SORTING BIOSAFETY SHEET
CELL SORTING BIOSAFETY SHEET
Procedure for working with pathogens or rDNA
Procedure for working with pathogens or rDNA
Principles and Practices of Biosafety
Principles and Practices of Biosafety
Summary of Recommended Biosafety Levels for Infectious Agents
Summary of Recommended Biosafety Levels for Infectious Agents
Name: shirgba sonter Jacob
Name: shirgba sonter Jacob
UK Flow Cytometry Biosafety Questionnaire
UK Flow Cytometry Biosafety Questionnaire
Bio - UC CEAS - University of Cincinnati
Bio - UC CEAS - University of Cincinnati
Challenges in Latin America for Implementing a Biorisk
Challenges in Latin America for Implementing a Biorisk
Biosafety Level 3
Biosafety Level 3
Biohazard Risk Assessment Worksheet
Biohazard Risk Assessment Worksheet
Table 2. Summary of Recommended Biosafety Levels for Infectious Agents
Table 2. Summary of Recommended Biosafety Levels for Infectious Agents
Risk Assessment - University of Texas Health Science
Risk Assessment - University of Texas Health Science
BSL 2 - UniMAP Portal
BSL 2 - UniMAP Portal
Why Biosafety Practices?
Why Biosafety Practices?