EPA/600/R-19/110 | September 2019
www.epa.gov/homeland-security-research
United States
Environmental Protection
Agency
&EPA
Protocol for Detection of
tularensis in Environmental Samples
During the Remediation Phase of a
Tularemia Incident
Office of Research and Development
Homeland Security Research Program
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Detection of Francisella tularensis in Environmental Samples
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Detection of Francisella tularensis in Environmental Samples
EPA/600/R-19/110
September 2019
Protocol for Detection of
Francisella tularensis in Environmental Samples
During the Remediation Phase of a
Tularemia Incident
Sanjiv R. Shah, Ph.D.
Homeland Security and Materials Management Division
Center for Environmental Solutions and Emergency Response
Office of Research and Development
U.S. Environmental Protection Agency
Washington, DC 20460
iii
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Detection of Francisella tularensis in Environmental Samples
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Detection of Francisella tularensis in Environmental Samples
Disclaimer
This document has been reviewed in accordance with U.S. Environmental Protection Agency (EPA)
policy and approved for public release. Note that approval does not signify that the contents necessarily
reflect the views of the Agency. Mention of trade names, products or services does not convey EPA
approval, endorsement, or recommendation.
Questions concerning this document, or its application should be addressed to:
Sanjiv R. Shah, Ph.D.
Disaster Characterization Branch
Homeland Security and Materials Management Division
Center for Environmental Solutions and Emergency Response
Office of Research and Development
U.S. Environmental Protection Agency
1300 Pennsylvania Avenue, NW
USEPA-8801RR
Washington, DC 20460
(202) 564-9522
shah, sani iv@epa. gov
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Detection ofFrancisella tularensis in Environmental Samples
Acknowledgements
This protocol was prepared under the leadership of Sanjiv R. Shah of the Homeland Security and
Materials Management Division (HSMMD) of the Center for Environmental Solutions and Emergency
Response (CESER) within the U.S. Environmental Protection Agency's (EPA) Office of Research and
Development (ORD).
The contributions of the following organizations and persons to this protocol are gratefully
acknowledged:
EPA Technical Reviewers
• Worth Calfee (U.S. EPA-ORD-CESER, HSMMD)
• David Bright (EPA/Office of Land and Emergency Management/Consequence Management Advisory
Division)
• Latisha Mapp (EPA/Office of Water/Water Security Division)
EPA OA Reviewers
• Eletha Brady-Roberts (EPA/ORD/CESER)
External Peer-Reviewers
• Paul Morin (U.S. Food and Drug Administration)
• Laura Rose (Centers for Disease Control and Prevention)
EPA Edit Reviewer
• Marti Sinclair (General Dynamics Information Technology)
Cover Photos: Left -Direct fluorescent antibody of Francisella tularensis; Right - Francisella tularensis
bacteria grown on chocolate agar after 72 hours (Source: Department of Health and Human Services -
CDC)
Section 10 Figure 2: Left - Francisella tularensis colonies on CHOC agar (Source: Public Health Image
Library); Right - Francisella tularensis colonies on CHAB agar (Source: Public Health Image Library)
VI
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Detection ofFrancisella tularensis in Environmental Samples
Table of Contents
Disclaimer v
Acknowledgements vi
List of Tables viii
List of Figures viii
Acronyms ix
Trademarked Products xi
Introduction 1
1.0 Scope and Application 4
2.0 Summary of Methods 4
3.0 Interferences and Contamination 5
4.0 Safety 5
4.1 Safety Precautions 5
4.2 Additional Recommended Safety Precautions 5
5.0 Supplies and Equipment 6
5.1 General Laboratory Supplies 6
5.2 Supplies for Real-time PCR Method Based Sample Analysis 7
5.3 Supplies for Culture Method Based Sample Analysis 7
5.4 Supplies for RV-PCR Based Sample Analysis 8
5.5 Equipment 8
6.0 Reagents and Standards 9
7.0 Calibration and Standardization 14
8.0 Quality Control (QC) 15
9.0 Real-time PCR Method 17
9.1 Sample Processing for Sponge-Sticks and Wipes 17
9.2 Sample Processing for Swabs 18
9.3 Sample Processing for Air Filters 19
9.4 Sample Processing for Water Samples (Large Volume [10 L-100 L], Drinking Water) 19
9.5 Sample Processing for Water Samples (Small Volume [< 50 mL], Surface or Drinking Water). 19
9.6 Sample Processing: DNA Extraction and Purification 20
9.7 Real-time PCR Analyses 23
10.0 Culture Method 28
10.1 Sample Processing and Plating for Sponge-Sticks and Wipes 28
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Detection ofFrancisella tularensis in Environmental Samples
10.2 Sample Processing and Plating for Swabs 32
10.3 Sample Processing and Plating for Air Filters 35
10.4 Sample Processing and Plating for Water Samples 38
10.5 Confirm F. tularensis Colonies by Real-time PCR Analysis 42
11.0 Rapid Viability-Polymerase Chain Reaction (RV-PCR) Method 44
11.1 RV-PCR 44
11.2 RV-PCR: Sample Processing and Plating for Water Samples 46
11.3 RV-PCR: Manual DNA Extraction/Purification Procedure Using the Promega MagneSil® Kit
Reagents 47
11.4 RV-PCR: Automated DNA Extraction/Purification Procedure (Roche MagNA Pure
Compact kit) 50
11.5 Real-time PCR Analysis of To and T30 or Tf DNA Extracts 52
12.0 Data Analysis and Calculations 54
12.1 Real-time PCR Analysis 54
12.2 Culture Analysis 55
12.3 RV-PCR Analysis 57
13.0 Method Performance 57
14.0 Pollution Prevention 57
15.0 Waste Management 58
16.0 References 58
List of Tables
Table 1. Example Concentrated Stock Preparation 10
Table 2. Example Working Stock Preparation 10
Table 3. Sample Processing Negative Controls (PNCs) 16
Table 4. Example F. tularensis Single-plex PCR Assay Master Mix Preparation for 70 Reactions 25
Table 5. PCR Thermal Cycling Conditions3'b 26
Table 6. Master Mix for Ftl and Ft2 Francisella tularensis PCR Assays 53
Table 7. PCR Thermal Cycling Conditions a'b 53
List of Figures
Figure 1. Real-time PCR Amplification 23
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Detection ofFrancisella tularensis in Environmental Samples
Figure 2. Francisella tularensis colonies on CHOC (left) and CHAB (right) agar after 48 hours 30
Figure 3. Example real-time PCR amplification curves for the initial TO aliquot and the Tf (final)
endpoint aliquot 44
Figure 4. Flow Chart for RV-PCR Analysis of Francisella tularensis Cells from Water Samples 45
Figure 5. Example logarithmic curve for Fluorogenic PCR for Bacillus anthracis 54
Acronyms
ABI Applied Biosystems® Incorporated
BD Becton, Dickinson and Company
BHI brain heart infusion
BMBL Biosafety in Microbiological and Biomedical Laboratories
BSC Biological safety cabinet
BSL Biosafety level
BVFH Brain Heart Infusion/Vitox/Fildcs/Histidinc
°C Degree(s) Centigrade
CDC Centers for Disease Control and Prevention
CESER Center for Environmental Solutions and Emergency Response
CFR Code of Federal Regulations
CFU Colony forming unit(s)
CHAB Cystine heart agar with rabbit blood and antibiotics
CHOC Chocolate agar
Ct Threshold Cycle
Ct (To) or To Ct Ct value at time zero (pre-incubation)
Ct (Tf) Ct value at time final (post-incubation)
CT (T3o) or T30 Ct Ct value after 30 hours incubation
ACt Delta threshold cycle
DNA Deoxyribonucleic acid
DQO Data quality objective
EDTA Ethylenediaminetetraacetic acid
EIC External inhibition control
EPA United States Environmental Protection Agency
ERLN Environmental Response Laboratory Network
F. tularensis Francisella tularensis
FAM 6-carboxyfluorescein
FBI Federal Bureau of Investigation
FEM Forum on Environmental Measurement
g gram(s)
h hour(s)
HSMMD Homeland Security and Materials Management Division
HSRP Homeland Security Research Program
ICLN Integrated Consortium of Laboratory Networks
IEC International Electrotechnical Commission
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Detection ofFrancisella tularensis in Environmental Samples
ISO
International Organization for Standardization
LRN
Laboratory Response Network
mg
milligram(s)
min
minute(s)
|o,L
microliter(s)
mL
milliliter(s)
mM
millimolar
NAD
Nicotinamide adenine dinucleotide (growth factor)
NG
No growth
NIST
National Institute of Standards and Technology
NTC
No template control
OSHA
Occupational Safety and Health Administration
ORD
Office of Research and Development
PBS
Phosphate buffered saline
PBST
PBS with 0.025% Tween 20
PC
Positive control
PCR
Polymerase chain reaction
pdpD
Pathogenicity determinant protein D
PMP
paramagnetic particles
PNC
[Sample] processing negative control (Blank)
PPE
Personal protective equipment
psi
Pounds per square inch
PT
Proficiency testing
QA
Quality assurance
QC
Quality control
RCF
Relative centrifugal force
rpm
Revolutions per minute
RV-PCR
Rapid viability-polymerase chain reaction
SDS
Safety data sheet
sec
second(s)
SWGFACT
Scientific Working Group on Forensic Analysis of Chemical Terrorism
To
Time 0, prior to incubation
T30
Time after 30 h of incubation
Taq
Thermus aquaticus bacterium
Tf
Time final, after incubation
TE
Tris(hydroxymethyl)aminomethane-Hydrochloride-EDTA
TNTC
Too numerous to count
TSB
Trypticase™ soy broth
UNG
Uracil-N-glycosilase
UV
Ultraviolet
VBNC
Viable but non-culturable
WLA
Water Laboratory Alliance
IX
1-fold concentrated (no concentration)
2X
2-fold concentrated
6X
6-fold concentrated
10X
10-fold concentrated
x
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Detection ofFrancisella tularensis in Environmental Samples
Trademarked Products
Trademark
Holder
Location
Acrovent™
Pall Corporation
Ann Arbor, MI
AeraSeal™
Excel Scientific
Victorville, CA
Amicon®
EMD Millipore®
Billerica, MA
AmpErase®
ThermoFisher Scientific
Waltham, MA
AmpliTaq Gold®
Life Technologies
Carlsbad, CA
Bacto™
BD Biosciences
Franklin Lakes, NJ
BD Clay Adams™ Nutator Mixer
BD Diagnostics
Sparks, MD
Biopur® Safe-Lock®
Eppendorf
United States
Applied Bio Systems®
Life Technologies™
Carlsbad, CA
BBL™
BD Diagnostics
Sparks, MD
Black Hole Quencher®
Biosearch Technologies, Inc.
Novato, CA
Costar®
Corning
Tewksbury, MA
Cole Parmer®
Cole Parmer®
Vernon Hills, IL
Dispatch®
Clorox Company
United States
Difco™
Becton, Dickinson & Co.
Franklin Lakes, NJ
Durapore®
Millipore Corporation
Billerica, MA
DynaMag™
Life Technologies
Carlsbad, CA
Epicentre®
Epicentre Technologies Corp.
Madison, WI
Fluoropore™
Merck KGaA
Darmstadt, Germany
Invitrogen®
Life Technologies™
Carlsbad, CA
IsoVitaleX™
BD Biosciences
Franklin Lakes, NJ
Kendall™
Covidien, Inc.
Mansfield, MA
Life Technologies™
Life Technologies™
Carlsbad, CA
Masterflex®
Cole Parmer®
Vernon Hills, IL
MagNA Pure®
Roche Diagnostics
Indianapolis, IN
MagneSil® Blood Genomic
Promega
Madison, WI
MaxQ™
Thermo Scientific Inc
Lenexa, KS
MicroFunnel™
Pall Corporation
Ann Arbor, MI
Microcon®
EMD Millipore
Billerica, MA
Millipore®
Merck KGaA
Darmstadt, Germany
Nalgene®
Nalge Nunc Corporation
Rochester, NY
Primer Express™
Applied Biosystems LLC.
San Francisco, CA
Remel™
Remel Inc.
Lenexa, KS
Stomacher®
Seward
United Kingdom
TaqMan®
Life Technologies™
Carlsbad, CA
r-i-i , • TM
Trypticase soy agar
BD Diagnostics
Sparks, MD
Trypticase™ soy broth
BD Diagnostics
Sparks, MD
Tween®
Sigma-Aldrich
St. Louis, MO
Ultracel®
EMD Millipore®
Billerica, MA
xi
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Detection ofFrancisella tularensis in Environmental Samples
Trademark
Holder
Location
Ultrafree®
EMD Millipore
Billerica, MA
Versalon™
Covidien, Inc.
Mansfield, MA
Ziploc™
S.C.Johnson
Racine, WI
Xll
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Detection of Francisella tularensis in Environmental Samples
Introduction
The core mission of the U.S. Environmental Protection Agency (EPA) is to protect human health and the
environment. After the 2001 terrorist attacks and the anthrax bioterrorism incidents that resulted in
human casualties as well as public and private facility closures, this core mission was expanded to address
critical homeland security related needs. Specifically, EPA was designated as the primary federal agency
responsible for the protection of indoor/outdoor structures and water infrastructure vulnerable to
chemical, biological, and radiological terrorist attacks. EPA is working to meet the specific homeland
security roles and responsibilities that are laid out in a series of statutes, presidential directives and
national frameworks. To enhance and expand the EPA's preparedness for response to an intentional or
unintentional incident or disaster that results in chemical, biological or radiological contamination, the
Homeland Security Research Program (HSRP) within the EPA Office of Research and Development
(ORD) conducts state-of-the art research and provides science and technology needed to effectively
recover from such incidents.
Francisella tularensis (/¦'. tularensis) is the bacterium that causes tularemia infection in humans and
animals. Due to its high virulence and low infective dose (Reference 16.1), and its potential use as a
biological weapon (References 16.1-16.3), F. tularensis is considered a high priority biothreat agent.
Based on the realities of the 2001 anthrax bioterrorism incident, F. tularensis is also considered a high-
priority bioterrorism agent for which response preparedness is extremely important. Once a tularemia
incident has occurred, regardless of its origin as a natural, accidental or an intentional release, the
response activities would need to include environmental assessment of contamination, decontamination,
and clearance. Therefore, combining the homeland security and natural tularemia outbreak related
responsibilities, EPA needs to have detailed analytical methods for detection of F. tularensis in
environmental matrices, including water. To address this critical need, EPA-ORD's HSRP has generated
this protocol for detection of F. tularensis in environmental samples for use by the EPA's Environmental
Response Laboratory Network (ERLN) and Water Laboratory Alliance (WLA).
F. tularensis is a zoonotic pathogen with an extremely wide host range that includes mammals, birds and
amphibians. The primary hosts for F. tularensis are believed to be small rodents (e.g., hares, voles,
muskrats). Humans usually acquire infection by direct contact with infected animals or by animal
associated biting arthropods. Ticks, mosquitoes and biting flies have all been implicated as capable
vectors. Although less common, contaminated soil, water, infected carcasses, and aerosolized particles
have been implicated as sources of infection (Reference 16.2). F. tularensis type A strain has been
isolated from natural waters and mud contaminated by muskrats and beavers, and the organisms may be
capable of multiplication in these environments. F. tularensis type B strain has also been isolated from
surface waters, including drinking water supplies. This pathogen could remain viable for more than 100
days in water and enter a viable but non-culturable (VBNC) state (Reference 16.4). In a weaponized
form, F. tularensis can persist in the environment for a long time and the aerosolized form can cause
wide-spread outbreak (Reference 16.2).
To complement an effective sample collection strategy during a suspected F. tularensis release incident, a
systematic approach for timely and cost-effective sample analyses is critical. Such a systematic approach
also helps in effectively managing and increasing the analytical laboratory capacity. This protocol
includes the following analytical approaches for the detection of F. tularensis in various environmental
samples:
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Detection of Francisella tularensis in Environmental Samples
1. Real-time polymerase chain reaction (PCR) to detect the presence of the DNA of F. tularensis.
2. Traditional microbiological culture to detect the presence of viable F. tularensis.
3. Rapid Viability-PCR (RV-PCR) method to detect the presence of viable F. tularensis in water
samples (16.5).
This protocol has been specifically developed for use by ERLN and WLA laboratories for the analysis of
environmental samples to assist in preparing for and recovering from disasters involving contamination
from F. tularensis. It should be noted that the Laboratory Response Network [LRN] laboratories
providing support to EPA for environmental sample analyses may use LRN protocols.
Sample processing procedures are also provided for respective analytical methods for all environmental
sample types including aerosol, particulate (surface swabs, wipes, and Sponge-Sticks™) and drinking
water. Since this protocol was developed to include the analyses of diverse environmental samples, it
emphasizes appropriate sample processing as well as DNA extraction and purification steps to
significantly remove cells and/or PCR-inhibitory materials present in the samples. This protocol will be
revised and updated as improved sample processing procedures and real-time PCR assays become
available.
For drinking water samples, large volume samples may need to be analyzed after concentration to detect
low concentrations of F. tularensis. For post- decontamination phase sample analysis using the culture
method, selected isolated colonies need to be analyzed using real-time PCR to confirm the identity of F.
tularensis, as opposed to traditional biochemical and serological testing.
CAUTION: At the time of publication, this protocol has not been validated. During any F. tularensis
related emergency situations, EPA's use of non-validated methods in the absence of validated methods
must adhere to the EPA's Forum on Environmental Measurement (FEM) policy directive on method
validation. :
According to Agency Policy Directive FEM-2010-01, Ensuring the Validity of Agency Methods
Validation and Peer Review Guidelines: Methods of Analysis Developed for Emergency Response
Situations:
It is EPA's policy that all methods of analysis (e.g., chemical, radiochemical,
microbiological) must be validated and peer reviewed prior to issuance as Agency
methods. There are emergency response situations that require methods to be developed
and utilized, which may or may not have previously been validated or peer reviewed
prior to use. This policy directive addresses those situations in which a method must be
developed, validated and/or peer reviewed expeditiously for utilization in an emergency
response situation. Also, in such emergency response situations only, an analytical
method may be employed that has been validated by another established laboratory
network (e.g., the Center for Disease Control and Prevention's Laboratory Response
Network, the U.S. Department of Agriculture/Food and Drug Administration's Food
Emergency Response Network). In those instances, the responsible federal agency will
indicate that the level of validation and/or peer review that their analytical method
underwent is consistent with the Integrated Consortium of Laboratory Networks' (ICLN)
5
Guidelines for Comparison of Validation Levels between Networks. The responsible
federal agency may also refer to the Validation Guidelines for Laboratories Performing
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Detection of Francisella tularensis in Environmental Samples
6
Forensic Analysis of Chemical Terrorism in order for the receiving federal agency to
determine if the analytical method meets the intended purpose.
Any EPA regional or program office that proposes to utilize a method in an emergency
response situation is responsible for establishing and documenting to what level and by
what process the method has been validated and/or peer reviewed in accordance with this
policy. A regional or program office may determine the level of validation and/or peer
review that is necessary to provide the objective evidence that a method is suitable for its
intended purpose; however, the office must document the validation and/or peer review
information supporting use of the method. All documentation should be preserved in
accordance with the Agency's records management policy.
5
U.S. Department of Homeland Security, Integrated Consortium of Laboratory Networks
(ICLN), ICLN Guidelines for Comparison of Validation Levels between Networks,
Original Version, https://\\cb-icln.s3-fips-us-gov-\\cst-
l.amazonaws.com/default/assets/File/ICLN-
Validation%20Levels%20Between%20Networks 003 01 (1 ).pdf
6
Federal Bureau of Investigation (FBI), Scientific Working Group on Forensic Analysis
of Chemical Terrorism (SWGFACT), Validation Guidelines for Laboratories Performing
Forensic Analysis of Chemical Terrorism, Forensic Science Communications, Volume 7,
Number 2, April 2005.
The above policy is available at:
https ://www.epa.gov/sites/production/files/2016-
11/documents/emergencv response validity policy reaffirmed nov2016.pdf
Also, EPA recognizes that having analytical data of known and documented quality is critical in making
proper decisions during all phases of a response to a bioterrorism incident and strives to establish data
quality objectives (DQOs) for each response activity.1 These DQOs are based upon needs for both
quality and response time. EPA's ERLN, which is tasked with providing laboratory support following
homeland security-related incidents, also has established data reporting procedures. Requirements for
receiving, tracking, storing, preparing, analyzing and reporting data are specified in the Environmental
Response Laboratory Network Laboratory Requirements Document at:
https://www.epa.gov/emergencv-response/environmental-response-laboratorv-network; project-specific
requirements also are included in individual Analytical Service Requests.
'Information regarding EPA's DQO process, considerations and planning is available at:
https://www.epa.gOv/qualitv/guidance-data-qualitv-obiectives-process-epa-qag-4-august-2000
3
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Detection of Francisella tularensis in Environmental Samples
Protocol for Detection of Francisella tularensis in Environmental
Samples During the Remediation Phase of a Tularemia Incident
1.0 Scope and Application
The purpose of this protocol is to provide multiple procedures and methods that can be used to detect
Francisella tularensis (/¦'. tularensis) in environmental samples. To detect the presence of the DNA of F.
tularensis, this protocol includes a real-time polymerase chain reaction (PCR) based method. Since the
PCR methods cannot determine viability of F. tularensis, this protocol includes culture/plating followed
by isolate confirmation by real-time PCR and Rapid Viability-PCR (RV-PCR). Note. The RV-PCR
procedure included in this protocol is only for water samples (16.5). During an actual incident validated
assays from other sources (e.g., Defense Biological Products Assurance Office of the Department of
Defense or Laboratory Response Network [LRN]) may be used.
This protocol will be periodically updated to include advances in sample processing and nucleic acid
extraction-purification procedures. This protocol is intended for the analyses of swabs, wipes, Sponge-
Sticks, air filters, and water for F. tularensis.
2.0 Summary of Methods
2.1 Sample Analysis for Detection of F. tularensis DNA (Real-time PCR):
Following sample processing including DNA extraction and purification, the DNA extracts are
analyzed by real-time PCR using the Applied Biosystems® Incorporated (ABI) 7500 Fast Real-
Time PCR System. Direct DNA-based analysis of samples allows for high throughput and rapid
results. Unless advised otherwise, real-time PCR based analysis should be performed using both
the PCR assays included in Section 6.9.
2.2 Sample Analyses for Detection of Viable F. tularensis:
After samples have been appropriately processed, samples are plated on chocolate agar (CHOC)
with IsoVitaleX™ and cysteine heart agar with rabbit blood and antibiotics (CHAB) (Reference
16.6) or inoculating into nutrient rich broth (e.g. Enrichment Culture and RV-PCR procedures).
Both of these methods include specific real-time PCR assay-based confirmation of the identity of
F. tularensis in the sample.
2.2.1 Culture Procedure
The culture option includes sample processing and plating serial dilutions of the
processed sample and membrane filters on CHAB medium followed by rapid
confirmation of morphologically typical isolated colonies using F. tularensis specific
real-time PCR. Unless advised otherwise, real-time PCR based analysis should be
performed using a Type strain-specific or both the PCR assays included in Section 6.9,
depending on the purpose of sample analyses.
2.2.2 RV-PCR Procedure (Water Samples)
The RV-PCR procedure serves as an alternative to the traditional culture-based methods
for detection of viable pathogens. The RV-PCR procedure integrates high-throughput
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Detection of Francisella tularensis in Environmental Samples
sample processing, short-incubation broth culture, and highly sensitive and specific real-
time PCR assays to detect low concentrations of viable bacterial threat agents.
Specifically, the procedure uses the change in real-time PCR response, referred to as the
change in cycle threshold, or ACt, between the initial cycle threshold (Ct) at time 0 (To)
(just before sample incubation) and the final Ct after incubation (Ct Tf). Example PCR
response curves are shown in Figure 3 (in Section 11.1) along with the criteria for
positive detection, namely ACt > 6. Unless advised otherwise, real-time PCR based
analysis should be performed using both the PCR assays included in Section 6.9.
3.0 Interferences and Contamination
3.1 Poor recoveries of F. tularensis may be caused by the presence of high numbers of competing or
inhibitory organisms, background debris, or toxic substances (e.g., metals or organic compounds).
3.2 Metals and organic compounds may also inhibit PCR reactions. Water samples suspected of
containing iron or rust particles should be placed on a magnetic rack to separate out the
particulates from the samples. The supernatant should be transferred to a clean sterile bottle/tube,
using care not to transfer any of the particulates.
3.3 Problems related to sample processing, such as clogging of filters and inefficient extraction, may
also result in poor recoveries.
4.0 Safety
Note: This protocol should not be misconstrued as a laboratory standard operating procedure that
addresses all aspects of safety including biosafety; the laboratory should adhere to safety
guidelines and requirements established by their organization or facility as well as the CDC.
All wastes should be handled according to the Centers for Disease Control and Prevention
(CDC) and the Biosafety in Microbiological and Biomedical Laboratories (BMBL), 5th
Edition, (Reference 16.7), BMBL waste management and disposal requirements.
4.1 Safety Precautions
Direct contact of skin or mucous membranes with infectious materials, accidental parenteral
inoculation, ingestion, and exposure to aerosols and infectious droplets have resulted in F.
tularensis infection. Due to the infectious nature of this organism, all samples should be handled
and analyzed using biosafety requirements as dictated by BMBL (Reference 16.7) or by the most
recent version and/or organizational health and safety plans. The CDC requires BSL-3 (biosafety
level-3) handling of this organism.
4.2 Additional Recommended Safety Precautions
4.2.1 Disposable materials (e.g., pipets, loops) are recommended for sample manipulations.
4.2.2 The analyst must know and observe normal safety procedures required in a microbiology
laboratory while preparing, using and disposing of media, cultures, reagents and
materials. Analysts must be familiar with the operation of sterilization equipment.
4.2.3 Personal Protective Equipment (PPE)
Laboratory personnel processing and conducting analyses of samples for F. tularensis
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Detection of Francisella tularensis in Environmental Samples
must use appropriate PPE (e.g., gloves, lab coat). Also, laboratory personnel should
familiarize themselves with the specific guidance for levels of protection and protective
gear developed by the U.S. Department of Labor, Occupational Safety and Health
Administration (OSHA), as provided in Appendix B of 29 CFR 1910.120
(https://www.osha.gov/laws-rcgs/rcgulations/standardnumbcr/1910/1910.120AppB)). In
addition to OSHA guidance, CDC developed recommendations for PPE based on
biosafety level (BSL) (Reference 16.7,
http://www.cdc.gov/biosafetv/publications/bmbl5/index.htm').
Note: Remove and don new gloves, as appropriate, to avoid contaminating hands and
surfaces between processing of each sample and to prevent cross-contamination.
Gloves should be disposed of into a biohazard autoclave bag whenever they become
visibly contaminated or the integrity of the gloves is compromised. After all work with
potentially infectious materials is completed, gloves should be removed, and hands
should be washed with soap and water.
4.2.4 This protocol does not address all safety issues associated with its use. Refer to (1)
BMBL, 5th Edition, CDC 2009 (Reference 16.7) for additional safety information; (2)
Organization-specific Health and Safety guidelines; (3) Select Agent Program
Requirements and (4) a reference file of Safety Data Sheets (SDS).
5.0 Supplies and Equipment
Note: Refer to Appendix A for supplies and equipment for large volume drinking water sample
processing.
5.1 General Laboratory Supplies
5.1.1 Gloves (e.g., latex, vinyl, or nitrile)
5.1.2 Sterile gloves (e.g., latex, vinyl, or nitrile)
5.1.3 Bleach wipes (Dispatch® Cat. No. 69150 or equivalent)
5.1.4 Ziploc® bags (large ~20" x 28", medium ~12" x 16", small ~7" x 8")
5.1.5 Sharps waste container
5.1.6 Absorbent pad, bench protector (Lab Source Cat. No. L56-149)
5.1.7 Medium and large biohazard bag(s) and wire twist ties
5.1.8 Sterile scalpels
5.1.9 Sterile stainless-steel scissors
5.1.10 Sterile disposable forceps (Cole Palmer® Cat. No. U06443-20 or equivalent)
5.1.11 Squeeze bottle with 70% isopropyl alcohol
5.1.12 Squeeze bottle with deionized water
5.1.13 Autoclave tape
5.1.14 Autoclave bags, aluminum foil, or kraft paper
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Detection of Francisella tularensis in Environmental Samples
5.1.15 Large photo-tray or similar tray for transport of racks
5.1.16 Laboratory marker
5.1.17 Timer
5.1.18 Sterile disposable serological pipets: 5 mL and 50 mL
5.1.19 Sterile disposable aerosol barrier pipet tips: 1000 (iL, 200 (iL, 20 (iL, 10 (iL (Rainin Cat.
No. SR-L1000F, SR-L200F, GP-20F, GP-10F or equivalent)
5.1.20 1.5 mL Eppendorf Snap-Cap Microcentrifuge Biopur® Safe-Lock® tubes (Fisher
Scientific Cat. No. 05-402-24B or equivalent)
5.1.21 Sterile 15 mL conical tubes (Fisher Scientific Cat. No. 339650 or equivalent)
5.1.22 Sterile 50 mL conical tubes (Fisher Scientific Cat. No. 06-443-18 or equivalent)
5.1.23 Racks for 15 mL and 50 mL conical tubes
5.1.24 Sterile 2 mL tubes, DNase, RNase-free, gasketed, screw caps (National Scientific Cat.
No. BC20NA-PS or equivalent)
5.1.25 Glass beads, acid washed, 106 |_im and finer (Sigma Cat. No. G4649 or equivalent)
5.1.26 Glass beads, acid washed, 425-600 |_im and finer (Sigma Cat. No. G8772 or equivalent)
5.1.27 PCR 8 cap strips (VWR Cat. No. 83009-684 or equivalent)
5.1.28 Amicon® Ultra-0.5 Centrifugal Filter Concentrator with Ultracel® 100 Regenerated
Cellulose Membrane (Millipore® Cat. No. UFC510096 or equivalent); Amicon®
collection tubes (Millipore® Cat. No. UFC50VL96 or equivalent)
5.1.29 0.22 (.un Ultrafree®-MC GV 0.5 mL Centrifugal Filter Unit with Durapore® PVDF
Membrane, Yellow Color Coded (Millipore® Cat. No. UFC30GV0S or equivalent)
5.1.30 0.1 |_im Ultrafree®-MC, VV Centrifugal Filter Device (Millipore® Cat. No. UFC30VV00
or equivalent)
5.1.31 Wide mouth screw cap containers, 120 mL (Fisher Scientific Cat. No. 14-375-459 or
equivalent)
5.2 Supplies for Real-time PCR Method Based Sample Analysis
5.2.1 96-well PCR plates (ABI Cat. No. 4346906 or equivalent)
5.2.2 96-well plate holders, Costar®, black (VWR Cat. No. 29442-922 or equivalent)
5.2.3 Edge seals for 96-well PCR plates (Adhesive Plate Sealers, Edge Bio Cat. No. 48461 or
equivalent)
5.2.4 Foil seals for 96-well PCR plates (Polar Seal Foil Sealing Tape, E & K Scientific Cat.
No. T592100 or equivalent), for longer storage of the plates
5.2.5 Optical seals (ABI Cat. No. 4311971 or equivalent)
5.3 Supplies for Culture Method Based Sample Analysis
5.3.1 Sterile disposable Petri dishes, 100 mm * 15 mm (If a medium is to be prepared in a
laboratory)
5.3.2 Sterile disposable inoculating loops (10 |_iL) and needles,
7
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Detection of Francisella tularensis in Environmental Samples
5.3.3 Sterile disposable cell spreaders (such as L-shaped, Fisher Scientific Cat. No. 03-392-150
or equivalent)
5.3.4 Sterile MicroFunnel™ Filter Funnels, 0.45 (.un pore-size (VWR Cat. No. 55095-060 or
equivalent)
5.3.5 Specimen Cups, 4.5 oz. (Kendall Cat. No. 17099 or equivalent)
5.3.6 Racks for 15 mL and 50 mL centrifuge tubes
5.3.7 Sterile disposable plastic 50 mL screw cap centrifuge tubes (Becton, Dickinson and
company [BD] Cat. No. 352070 or equivalent)
5.3.8 Sterile disposable plastic 15 mL screw cap centrifuge tubes (BD Cat. No. 352097 or
equivalent)
5.3.9 Sterile Pipettips with aerosol filter for 1000 |aL and 100 |aL (Rainin Cat. No. SR-L1000F
and GP-100F or equivalent)
5.3.10 Biotransport carrier (Nalgene®, Thermo Scientific Cat. No. 15-251-2 or equivalent)
5.4 Supplies for RV-PCR Based Sample Analysis
5.4.1 Disposable nylon forceps (VWR Cat. No. 12576-933 or equivalent)
5.4.2 50 mL conical tubes (VWR Cat. No. 21008-951 or equivalent)
5.4.3 Disposable serological pipets: 50 mL, 25 mL, 10 mL, 5 mL
5.4.4 Single 50 mL conical tube holder (Bel-Art Cat. No. 187950001 or equivalent)
5.4.5 Screw cap tubes, 2 mL (VWR Cat. No. 89004-298 or equivalent)
5.4.6 96-well tube rack(s) for 2 mL tubes (8 x 12 lay out) (Bel-Art Cat. No. 188450031 or
equivalent)
5.4.7 2 mL Eppendorf tubes (Fisher Scientific Cat. No. 05-402-24C or equivalent)
5.4.8 96-well 2 mL tube rack (8 x 12 format) (Bel-Art Cat. No. 188450031)
5.4.9 48-well plates (E&K Scientific Cat. No. EK-2044 or equivalent)
5.5 Equipment
5.5.1 Biological Safety Cabinet (BSC) - Class II or Class III
5.5.2 PCR preparation hood/work station
5.5.3 Balance, analytical, with Class S reference weights, capable of weighing 20 g ± 0.001 g
5.5.4 ABI 7500 Fast Real-Time PCR System (Life Technologies™)
5.5.5 Refrigerated centrifuge with PCR plate adapter and corresponding safety cups and rotors
for 5 mL and 50 mL tubes (Eppendorf Cat. No. 5804R, 5810R or equivalent) or PCR
plate spinner (placed in BSC [VWR Cat. No. 89184-608 or equivalent])
Note: Swinging bucket and fixed angle rotors for the refrigerated centrifuge may also be
necessary.
5.5.6 Refrigerated micro-centrifuge for Eppendorf tubes with aerosol-tight rotor (Eppendorf
Cat. No. 5415R/5424R or equivalent)
8
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Detection of Francisella tularensis in Environmental Samples
5.5.7 Vacuum pump with gauge (Cole Parmer® Model EW-07061-40 or equivalent) or vacuum
source capable of < 10 pounds per square inch (psi)
5.5.8 Vacuum pump filters for pump (Acrovent™ Cat. No. 4249 or equivalent)
5.5.9 Vacuum trap accessories
5.5.10 Single-tube vortexer (Fisher Scientific Cat. No. 50-143-447 or equivalent); multi-tube
adapter (Scientific Industries, Inc. Cat. No. SI-V525 or equivalent) optional
5.5.11 Single-channel micropipettors (1000 |a,L, 200 |a,L,100 (iL, 20 (iL, 10 (iL)
5.5.12 Serological pipet aid
5.5.13 Incubator(s), microbiological type, maintained at 35°C - 37°C
5.5.14 Autoclave or steam sterilizer, capable of achieving 121°C (15 psi) for 30 minutes
5.5.15 Cold block (4°C) for 2 mL tubes (Eppendorf Cat. No. 3880 001.018 or equivalent)
5.5.16 Bead-beater (BioSpec Products, Inc. Cat. No. 607 [16 place] or equivalent)
5.5.17 Tube racks, 80-place (VWR Cat. No. 30128-282 or equivalent)
5.5.18 40 kHz sonicator bath (Branson Ultrasonic Cleaner Model 1510, Process Equipment and
Supply, Inc. Cat. No. 952-116 or equivalent)
5.5.19 Stomacher® 400 Circulator (Seward Cat. No. 0400/001/AJ or equivalent) with closure
bags (Cat. No. BA6141/CLR or equivalent) and rack (Cat. No. BA6091 [1 place] and
BA6096 [10 place] or equivalent)
5.5.20 DynaMag™ magnetic stand (ThermoFisher Scientific Cat. No. 1232ID or equivalent)
5.5.21 MagNA Pure® Compact instrument (Roche Diagnostics)
6.0 Reagents and Standards
6.1 Reagent-grade chemicals must be used in all for all analysis/assays. Unless otherwise indicated,
reagents shall conform to the specifications of the Committee on Analytical Reagents of the
American Chemical Society (Reference 16.8). For suggestions regarding the testing of reagents
not listed by the American Chemical Society, see AnalaR Standards for Laboratory Chemicals,
BDH Ltd., Poole, Dorset, U.K. (Reference 16.9); and United States Pharmacopeia and National
Formulary 24, United States Pharmacopeial Convention, Md. (Reference 16.10).
6.2 Tween® 80 (Fisher Cat. No. T164 or equivalent)
6.3 PCR-grade water, sterile (Teknova Cat. No. W3350 or equivalent)
6.4 Sterile 0.01 M phosphate buffered saline (PBS) pH 7.2-7.4 (Sigma Cat. No. P3813 or equivalent)
6.5 IX phosphate buffered saline with 0.025% Tween® 20 (PBST), pH 7.4 [IX phosphate buffered
saline with 0.05% Tween® 20 (PBST), pH 7.4, (Teknova Cat. No. P0201 or equivalent) diluted
1:1 with sterile PBS (Section 6.4)]
6.6 10X phosphate buffered saline (PBS), pH 7.4, (Teknova Cat. No. P0196 or equivalent)
6.7 TE buffer (IX Tris [10 mM] -HC1-EDTA [1 mM Ethylenediaminetetraacetic acid]) buffer, pH
8.0 (Fisher Scientific Cat. No. BP2473-500 or equivalent)
9
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Detection of Francisella tularensis in Environmental Samples
6.8 TaqMan® 2X Universal PCR Master Mix (Life Technologies, Cat. No. 4304437)
6.9 PCR Assays
Ftl (For !•'. tularensis Type A strain) targeting pdpD, pathogenicity determinant protein D,
hypothetical protein of F. tularensis (Reference 16.11)
• Forward Primer (Ft 1 -F) - 5' - GAGACATCAATTAAAAGAAGCAATACCTT -3'
• Reverse Primer (Ftl-R) - 5'- CCAAGAGTACTATTTCCGGTTGGT -3'
• Probe (Ft 1 -Pr) - 5' -6FAM- AAAATTCTGCTCAGCAGGATTTTGATTTGGTT -BH
Ql-3'
Ft2 (For /¦'. tularensis Type B strain) targeting a junction between lSFtu2 and a flanking 3' region
of /¦'. tularensis (Reference 16.11)
• Forward Primer (Ft2-F) - 5' - CTTGTACTTTTATTTGGCTACTGAGAAACT -3'
• Reverse Primer (Ft2-R) - 5' - CTTGCTTGGTTTGTAAATATAGTGGAA -3'
• Probe (Ft2-Pr) - 5' -6FAM- ACCTAGTTCAACCTCAAGACTTTTAGTAATGGGAATGTCA
-BHQ1-3'
6.9.1 Preparation of concentrated primer and probe working stocks
Prior to PCR analyses lyophilized primers and probes should be rehydrated in PCR-grade
water to prepare concentrated stocks. Primary concentrated storage stocks should
initially be prepared to obtain 100 |iM (0.1 nmolcs/|iL) and 40 |iM (0.04 nmolcs/|iL)
solutions of primers and probes, respectively. These primary (concentrated) stocks will
be used to prepare working stock solutions that will then be used to prepare PCR assay
mixes (Section 9.7) on the day of use. Example rehydration of lyophilized primers/probes
and dilution of rehydrated stocks to prepare working stocks are provided in Tables 1 and
2, respectively.
Table 1. Example Concentrated Stock Preparation
l.tophili/cri Primer/Pi-ohc
(ii moles)
PCR tirade
\\;i (or (ill.)
( onccnlralion
n moles/ill ¦
ii M
FWD Primer
29
290
0.1
100
REV Primer
35
350
0.1
100
Probe
17
425
0.04
40
FWD, forward; REV, reverse
Table 2. Example Working Stock Preparation
( onccnlralcd Slock
(.ill.)
PCR tirade
wilier (.ill.)
Dilution
( oncen 1 r;i I ion
nmolcs/iil.
ii M
FWD Primer
20
180
0.1
0.01
10
REV Primer
20
180
0.1
0.01
10
Probe
20
180
0.1
0.004
4
FWD, forward; REV, reverse
Working stocks will be used to prepare master mix on the day of use (Section 9.7.3).
6.10 Positive Control (PC) -DNA isolated from an appropriate virulent F. tularensis strain containing
all of the plasmids. For culture analyses, F. tularensis LVS strain (BSL-2 organism) or other
10
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Detection of Francisella tularensis in Environmental Samples
avirulent strains may be used as a PC to meet the laboratory's BSL.
6.11 Chocolate agar (CHOC) with IsoVitaleX, a selective F. tularensis mediumThe use of
commercially prepared plates is recommended (BD Cat. No. 254060 or equivalent). The
formulation of the medium is only provided to allow laboratories to ensure that their medium is
equivalent to the medium included in the protocol.
6.11.2 Medium Composition:
Hemoglobin 10 g
Pancreatic Digest of Casein 7.5 g
Selected Meat Peptone 7.5 g
Sodium Chloride 5 g
Dipotassium Phosphate 4 g
Cornstarch 1 g
Monopotassium Phosphate 1 g
Agar 12 g
Hemoglobin 10 g
IsoVitaleX Enrichment 12 mL
Pyridoxal 0.01 g
Growth Factors 0.5 g
Reagent-grade Water 1000 mL
6.11.3 BD IsoVitaleX
Glucose 100 g
Cysteine Hydrochloride 25.9 g
L-Glutamine 10 g
L-Cystine 1.1 g
Adenine 1 g
NAD (nicotinamide adenine)
dinucleotide (growth factor) 0.25 g
Thiamine Pyrophosphate 0.1 g
Guanine Hydrochloride 0.03 g
Ferric Nitrate 0.02g
P-Aminobenzoic Acid 0.013 g
Vitamin B-12 0.01 g
Thiamine Hydrochloride 0.003 g
Reagent-grade Water 1000 mL
11
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Detection of Francisella tularensis in Environmental Samples
6.12 Cystine Heart Agar with Rabbit Blood (CHAB), a selective F. tularensis medium
6.12.1. The use of commercially prepared media is recommended (Thermo Scientific Cat. No.
R01346 or equivalent). The formulation of the medium is only provided to allow
laboratories to ensure that their medium is equivalent to the medium included in the
protocol.
6.12.2. Medium Composition:
Casein Peptone 13 g
Dextrose 10 g
Sodium chloride 5 g
Yeast Extract 5g
Beef Heart Infusion 2 g
L-Cystine 1 g
Penicillin 100,000 U
Polymyxin B 100,000 U
Rabbit Blood 5 %
Agar 15 g
Reagent-grade water 1000 mL
6.13 Tryptic Soy broth with IsoVitaleX
6.13.1. The use of commercially prepared dehydrated medium (Fisher Cat. No. DF0370-17-3 or
equivalent) and IsoVitaleX (Fisher Cat. No. B11875 or equivalent) is recommended. If
commercially prepared medium is not available, prepare medium using procedures in
6.13.2-6.13.4.
6.13.2. Medium Composition
Tryptone H 15 g
Soytone 5 g
Sodium chloride 5 g
IsoVitaleX 20 mL
Reagent-grade water 1000 mL
6.13.3. Add reagents except IsoVitaleX to 950 mL of reagent-grade water and mix thoroughly
using a stir bar and hot plate. Warm slightly and stir to dissolve the powder completely.
Adjust pH to 7.3 ± 0.2 with 1.0 N HC1 or 1.0 N NaOH and bring to 1000 mL with
reagent-grade water. Autoclave at 121°C (15 psi) for 15 minutes. Do not overheat. Cool
to room temperature.
6.13.4. Aseptically add 20 mL of IsoVitaleX to the cooled medium and swirl to mix. Store at
4°C in screw cap bottles for a maximum of three months.
12
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Detection of Francisella tularensis in Environmental Samples
6.14 Promega Reagents for DNA Extraction and Purification Procedure for RV-PCR:
• MagneSil® Blood Genomic, Max Yield System, Kit (Promega Cat. No. MD1360; VWR Cat.
No. PAMD1360 or equivalent)
• Salt Wash (VWR Cat. No. PAMD1401 or equivalent)
• MagneSil Paramagnetic Particles (PMPs) (VWR Cat. No. PAMD 1441 or equivalent)
• Lysis Buffer (VWR Cat. No. PAMD 1392 or equivalent)
• Elution Buffer (VWR Cat. No. PAMD 1421 or equivalent)
• Alcohol Wash, Blood (VWR Cat. No. PAMD 1411 or equivalent)
• Anti-Foam Reagent (VWR Cat. No. PAMD 1431 or equivalent)
6.15 MagNA Pure Compact Nucleic Acid Isolation Kit I (Roche Cat. No. 03730 964001)
6.16 MagNA Pure LC Total Nucleic Acid Isolation Kit-Additional Lysis/Binding Buffer (Roche Cat.
No.03246779001)
6.17 6X BVFH - Brain Heart Infusion (BHI) Broth with 20% (v/v) Vitox Supplement (final 2% Vitox
in IX), 60% (v/v) Fildes (final 10% Fildes in IX), and 1% (w/v) L-histidine (BVFH)
• Weigh 22.2 g BactoTM Brain Heart Infusion Broth Base powder into 500 mL flask or bottle.
• Weigh 0.6 g L-histidine into the same 500 mL flask or bottle.
• Add 28 mL MilliQ® H2O or equivalent.
• Heat with frequent agitation and boil for 1 minute to completely dissolve the powder.
• Allow broth to cool down to room temperature under a BSC before storing at 4°C.
• Check pH and adjust to 7.2 ± 0.2.
• For addition of Oxoid® Vitox Supplement, reconstitute Vitox supplement in buffer provided
by vendor and add 12 mL of Vitox supplement to give a concentration of 12% in the sterilized
6X BHI+histidine broth (2% when diluted to IX).
• For addition of Remel™ Fildes Enrichment supplement, add 60 mL Fildes to give a
concentration of 60% in the sterilized 6X BHI+histidine+Vitox broth (10% when diluted to
IX).
• Test samples of the 6X BVFH product for sterility by incubating a 0.6 mL aliquot into 5.4 mL
buffer in a 50-mL conical tube and incubating at 37°C for 3 days. Confirm sterility before use
in the RV-PCR assay.
6.18 10% Bleach pH-amended (prepared daily), optional
Add 2 parts water to 1 part bleach, then add 5% acetic acid (1 part) and remaining water (6 parts).
Measure pH and add bleach (to increase pH) or acetic acid (to decrease pH) as needed to obtain a
final pH between 6 and 7. A pH meter, as opposed to pH strips or kit, should be used to measure
pH. When mixed, place a lid on the mixture to reduce chlorine escape and worker exposure.
6.19 100% Ethanol (200-proof) for preparation of 70% ethanol by dilution with PCR-grade water.
13
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Detection of Francisella tularensis in Environmental Samples
7.0 Calibration and Standardization
7.1 Each laboratory that uses this protocol is required to operate a formal quality assurance (QA)
program that addresses and documents instrument and equipment maintenance and performance,
reagent quality and performance, analyst training and certification, and records storage and
retrieval. International Organization for Standardization (ISO)/International Electrotechnical
Commission (IEC) 17025 (International Standard: General requirements for the competence of
testing and calibration laboratories, Section Edition 2005-05-15) provides a quality framework
that could be used to develop a formal QA program.
7.2 Check temperatures in incubators twice daily with a minimum of 4 hours between each reading to
ensure operation within stated limits. Record the temperature in a log book.
7.3 Check temperature in refrigerators/freezers at least once daily to ensure operation is within the
storage requirements for samples, reagents, and media. Record daily measurements in a
refrigerator/freezer log book.
7.4 Check thermometers, including those on instrumentation (e.g., digital display), at least annually
against a National Institute of Standards and Technology (NIST) certified thermometer or one
that meets the requirements of NIST Monograph SP 250-23. Check columns for breaks.
7.5 Calibrate pH meter following manufacturer's instructions prior to each use with at least two of
three standards (e.g., pH 4.0, 7.0 or 10.0) closest to the range being tested.
7.6 Verify balance calibration every two months with reference weights (e.g., ASTM Class 2).
7.7 Micropipettors should be calibrated at least annually and tested for accuracy on a weekly basis.
7.8 Follow manufacturer instructions for calibration of real-time PCR instruments.
7.9 Re-certify BSCs annually. Re-certification must be performed by a qualified technician.
7.10 Autoclave maintenance should be conducted at least annually. Autoclave temperature and total
sterilization cycle time should be checked on a quarterly basis. Record the data in a log book.
Spore strips or spore ampules should be used monthly as bioindicators to confirm sterilization.
7.11 Refrigerated centrifuges should be checked to confirm temperature and revolutions per minute
(rpm) on a quarterly basis. Record the data in a log book.
7.12 Vacuum pressure (e.g., pumps, in house system) should be checked on a regular basis to ensure
that the pressure is 5-10 psi. Higher or lower vacuum pressure could negatively impact
recoveries.
7.13 Sample integrity — Samples should be checked for loss of integrity (e.g., improperly packaged,
temperature exceedance, leaking). Samples may be rejected if the integrity has been
compromised. Alternately, if sample integrity has been compromised, the sample may be
analyzed, and the data qualified and marked accordingly (e.g., if a sample exceeded temperature
during transport - data are flagged and marked as exceeding temperature), so that a decision can
be made regarding whether the data should be considered valid/invalid.
7.14 Analyst qualifications — Only those analysts who have been trained and have demonstrated
proficiency with these analytical techniques should perform this procedure.
7.15 Proficiency testing (PT) — The laboratory should have analysts analyze test samples annually, at
a minimum, to ensure they are maintaining proficiency. In addition, analysts should analyze PT
samples to demonstrate proficiency prior to analyzing field samples. For laboratories not
14
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Detection of Francisella tularensis in Environmental Samples
routinely using this protocol, analysts should analyze PT samples biannually. If a PT failure
occurs, the laboratory should identify and resolve any issues and then request and analyze
additional PT samples. Field samples should not be analyzed until the laboratory passes the PT.
8.0 Quality Control (QC)
8.1 Quality assurance and quality control are closely related. However, this section will describe
them separately to highlight QC considerations specific to this protocol.
8.2 Media sterility check — The laboratory should test media sterility by incubating a single unit
(tube or Petri dish) from each batch of medium (CHOC with IsoVitaleX and CHAB) at 35°C -
37°C for 24 ± 2 hours and observe for growth. Absence of growth indicates media sterility. On
an ongoing basis, the laboratory should perform media sterility checks every day that samples are
analyzed.
8.3 Culture: Positive control (PC) — The laboratory should analyze PCs (known quantity of cells) to
ensure that all media and reagents are performing properly. F. tularensis LVS strain (BSL-2
organism) or other avirulent strains may be used as a PC to meet the laboratory's BSL. PCs
should be analyzed whenever a new batch of media or reagents is used. On an ongoing basis, the
laboratory should run a PC every day that samples are analyzed.
8.4 PCR: Positive control (PC) — DNA isolated from an appropriate virulent F. tularensis strain
containing all the plasmids should be used as the PC. The laboratory should analyze a PC in
triplicate reactions with each PCR run. Prepare the PC at a concentration of 50 pg of purified F.
tularensis total DNA per 5 |_iL of PCR-grade water. All PCs should result in a cycle threshold
(Cx)< 40 and replicates should be within ± 1 Ct of each other.
8.5 External inhibition control (EIC, also referred to as sample matrix control) of 50 pg genomic
DNA from F. tularensis — For determination of presence of DNA by real-time PCR, the
laboratory should analyze an EIC for each environmental sample DNA extract to determine if the
matrix is causing inhibition potentially resulting in false negative results. Prepare the EIC at a
concentration of 50 pg of purified F. tularensis DNA per 1 (.iL of PCR-grade water. Using a 10
(.iL pipettor, carefully add 1 (.iL of the DNA to the EIC wells on a PCR plate and then add 5 (.iL of
sample DNA extract to each well and mix thoroughly. The PCR results from the PC and EICs
(both containing 50 pg of F. tularensis DNA) are then compared. Lower or similar Ct values for
the EIC indicate there is no inhibition. A higher Ct value for the EIC (>3 Ct values) is indicative
of matrix inhibition.
Note: To minimize cross contamination, the EICs should not be placed next to the field samples
when setting up the PCR plate.
8.6 No template control (NTC, also referred to as reagent blank) — The laboratory should analyze
NTCs (5 (.iL of PCR-grade water is added to the NTC wells on a PCR plate in place of the DNA
or the sample DNA extract) to ensure that reagents are not contaminated. On an ongoing basis,
the laboratory should analyze NTCs in triplicate PCR reactions with each PCR run. The NTC
must not exhibit fluorescence above the background level (i.e., no Ct value). If Ct values are
obtained as a result of a possible contamination or cross-contamination, prepare fresh PCR
Master Mix and repeat the analysis.
8.7 Field blank — The laboratory should request that the sampling team provide a field blank with
each batch of samples. A field blank is defined as either a sample collection tool (e.g., wipe,
15
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Detection of Francisella tularensis in Environmental Samples
swab) or sterile reagent-grade water that is taken out to the field, opened and exposed to the
environment, but not used to collect a sample, and then placed in a bag and sealed and transported
to the laboratory along with the field samples. The field blank is treated as a sample in all
respects, including exposure to sampling location conditions, storage, preservation and all
analytical procedures. Field blanks are used to assess any contamination due to sampling location
conditions, transport, handling and storage. The laboratory should process and analyze this
control along with each batch of environmental samples. The field blanks should not exhibit
fluorescence (i.e., Ct > 45).
Note: The field blank for large volume water samples should also be concentrated using
ultrafiltration prior to analyses. A smaller volume of water (e.g., 10-20 L) may be used for the
field blank to minimize the burden on the laboratory
8.8 Sample processing negative control (PNC) or method blank — The laboratory should process and
analyze a PNC in the same manner as a sample to verify the sterility of equipment, materials and
supplies. Absence of growth indicates lack of contamination from the target organism. Refer to
Table 3 for appropriate PNC.
8.9 For RV-PCR based analysis, the To and T30 or Tf extracts are analyzed (in triplicate). PCR
positive and negative controls must be analyzed using the same preparation of the PCR Master
Mix and must be run on the same 96-well plate as the To and T30 or Tf extracts.
Table 3. Sample Processing \egali\c Controls (P\Cs)
Matrix
PNC
Wipes
Clean (unused) wipe
Swabs
Clean (unused) swab
Air filters
Clean (unused) air filter
Sponge-Sticks
Clean (unused) Sponge-Stick
Drinking water and decontamination
waste water
100 mL of sterile reagent-grade water
Large volume water samples
10 - 20 L of sterile reagent-grade water
16
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Detection of Francisella tularensis in Environmental Samples
9.0 Real-time PCR Method
Real-time PCR allows for rapid detection of F. tularensis in samples based simply on the presence
of the target DNA. However, since the DNA from non-viable cells can also be detected by this
method, the positive sample analysis result does not confirm the presence of viable cells.
Therefore, this method is usually used for a time- and cost-effective presumptive analysis of
samples. This section includes a real-time PCR method with appropriate sample processing
procedures for detection of F. tularensis.
Acceptable sample types: Gauze wipes (2" * 2" 50% rayon/50% polyester [Kendall™ Versalon™
Cat. No. 8042 or equivalent]), air filters (37 mm Fluoropore™ [Millipore® Cat. No. FSLW04700 or
equivalent]), swabs (macrofoam [VWR Cat. No. 89022-994 small swabs or 89022-984 extra-large
swabs, or equivalent]), Sponge-Stick sampling tools (3M™ Inc. Cat. No. SSL10NB or equivalent),
drinking water and decontamination waste water
9.1 Sample Processing for Sponge-Sticks and Wipes
Note: All subsequent procedures involving manipulation of Sponge-Sticks and wipes must be carried
out in a BSC using appropriate PPE (e.g., gloves, lab coat). The CDC requires BSL-3 handling
of this organism. All wastes should be handled according to the CDC and the BMBL handling
and disposal requirements.
9.1.1 If the Sponge-Stick sponge/wipe sample is not in a Stomacher® bag, aseptically transfer it
to a Stomacher®bag using sterile forceps.
9.1.2 Using aseptic technique, remove the plastic stick base holding the sponge together. Place
gloved hands on the outside of the Stomacher® bag, grip the Sponge-Stick head on both
sides and peel the sponge away from the base and unfold the sponge. Be careful not to
puncture bag with edge of stick base. Using sterile forceps remove stick base from bag
and discard in a biohazard autoclave bag. Change forceps between samples.
9.1.3 Add 90 mL of PBST (0.05% Tween® 20, Section 6.5) to each bag. Set Stomacher®
(Section 5.5.19) to 200 rpm.
9.1.4 Place a bag containing a sample into the Stomacher® (Section 5.5.19) so the Sponge-
Stick sponge/wipe rests evenly between the homogenizer paddles and stomach each
sample for 1 minute at 200 rpm.
9.1.5 Open the door of the Stomacher® (Section 5.5.19) and remove the bag. Grab the
sponge/wipe from the outside of the bag with your hands. With the bag closed, move the
sponge/wipe to the top of the bag while using your hands to squeeze excess liquid from
the sponge/wipe.
9.1.6 Open the bag, remove the sponge/wipe using sterile forceps and discard in an
autoclavable biohazard bag.
9.1.7 Follow steps described above for each sample, changing forceps between samples.
9.1.8 Allow bags to sit for 10 minutes to allow elution suspension foam to settle.
9.1.9 Gently mix the elution suspension in the Stomacher® bag up and down 3 times with a
sterile 50 mL pipet. Remove half of the suspension volume (-47 mL) and place it in a
labeled 50 mL screw cap centrifuge tube. Place the remaining suspension (-47 mL) into
a second 50 mL tube. Adjust the suspension volumes in both the tubes to ensure they are
similar.
17
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Detection of Francisella tularensis in Environmental Samples
9.1.10 Process elution suspension for each sample as described above.
9.1.11 Place the 50 mL tubes from step 9.1.9 into sealing centrifuge buckets and decontaminate
the outside of the centrifuge buckets before removing them from the BSC.
9.1.12 Centrifuge tubes at maximum speed (-3200 x g) with the brake off, for 15 minutes in a
swinging bucket rotor at 4°C.
9.1.13 Using a sterile 50 mL pipet for each sample, remove 44 mL of the supernatant from each
sample tube and discard it in an autoclavable biohazard container. The pellet may be
easily disturbed and not visible, so keep the pipet tip away from the bottom of the tube.
9.1.14 Set the vortexer (Section 5.5.10) to the high setting. Set the sonicator water bath to high.
9.1.15 Vortex the tubes for 30 seconds and transfer the tubes to the sonicator water bath and
sonicate for 30 seconds. Repeat the vortex and sonication cycles two more times.
Note: As an alternative to sonication, tubes may be vortex mixed for two minutes in 10
second bursts, if possible use a vortexer with a multi-tube adapter to reduce processing
time for multiple samples.
9.1.16 Remove suspension from both tubes with a sterile 5 mL pipet and combine into a 15 mL
conical tube. Measure final volume of suspension with 5 mL pipet and record the result
on the tube and data sheet.
9.1.17 Centrifuge tubes at 3200 x g with the brake off, for 15 minutes in a swinging bucket rotor
at 4°C.
9.1.18 Using a sterile 5 mL pipet, remove 3 mL of supernatant (from ~ 6 mL), and discard in an
autoclavable biohazard bag.
9.1.19 Vortex the tube for 1 minute in 10 second bursts.
9.1.20 Repeat steps 9.1.1 through 9.1.19 for each sponge-stick or wipe sample.
9.1.21 Use a 1.5 mL aliquot for DNA extraction using bead-beating, as described in Section 9.6.
9.2 Sample Processing for Swabs
Note: All subsequent procedures involving manipulation of swabs and membranes must be carried out
in a BSC using appropriate PPE. Sterile gloves should be used and changed between samples
and as indicated below. The CDC requires BSL-3 handling of this organism. All wastes should
be handled according to the CDC and the BMBL waste management and disposal requirements.
9.2.1 If the swabs are not in 15 mL centrifuge tubes, transfer each swab to a sterile, labeled 15
mL centrifuge tube using sterile forceps.
9.2.2 If necessary, cut the handle of the swab to fit into the tube using sterile forceps and
scissors for each sample.
9.2.3 Add 2 mL of sterile PBS for smaller swabs and 3 mL of sterile PBS for larger swabs to
each tube and vortex at the highest setting for two minutes. Additional PBS may be
added in 0.5 mL increments to ensure that a minimum volume of 2 mL is available for
PCR analysis.
9.2.4 Using sterile forceps, remove the swab from the 15 mL centrifuge tube. Use the forceps
to press the tip of the swab against the inside of the tube to remove extra liquid from the
foam tip before discarding the swab in an autoclavable biohazard bag.
18
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Detection of Francisella tularensis in Environmental Samples
9.2.5 Repeat steps 9.2.1 through 9.2.4 for each swab sample.
9.2.6 Use 1.5 mL aliquot for DNA extraction using bead-beating, as described in Section 9.6.
9.3 Sample Processing for Air Filters
Note: All subsequent procedures involving manipulation of air filters must be carried out in a BSC
using appropriate PPE. Sterile gloves should be used and changed between samples and as
indicated below. The CDC requires BSL-3 handling of this organism. All wastes should be
handled according to the CDC and the BMBL waste management and disposal requirements.
9.3.1. If the air filters are not in 50 mL tubes, aseptically transfer each sample to a sterile 50 mL
tube using sterile forceps. Change forceps between samples.
9.3.2. Add 3 mL of PBS to each tube and vortex at the highest setting for 2 minutes.
9.3.3. Open the tube and using a sterile transfer pipet; depress the air filter against the side of
the tube to expel as much liquid as possible before discarding filter using sterile forceps
into a biohazard autoclave bag.
9.3.4. Repeat steps 9.3.1 through 9.3.3 for each air filter sample.
9.3.5. Use 1.5 mL aliquot for DNA extraction using bead-beating, as described in Section 9.6.
9.4 Sample Processing for Water Samples (Large Volume [10 L-100 L], Drinking Water)
It is anticipated that the large volume water sample has undergone primary and secondary
concentration and the resultant concentrated sample has been filtered through a membrane filter.
Therefore, this sub-section describes the procedure for processing of such a membrane filter
received in a 50 mL screw cap tube or other appropriate container.
Note: All subsequent procedures involving manipulation of water samples and membranes must be
carried out in a BSC using appropriate PPE. Sterile gloves should be used and changed
between samples and as indicated below. The CDC requires BSL-3 handling of this organism.
All wastes should be handled according to the CDC and the BMBL waste management and
disposal requirements.
9.4.1 If the membranes are not in 50 mL tubes, aseptically transfer each membrane to a sterile
50 mL tube using sterile forceps. Change forceps between samples.
9.4.2 Add 5 mL of sterile PBS to 50 mL screw cap tube containing a membrane filter and
vortex at the highest setting for 2 minutes with 10 seconds bursts.
9.4.3 Using sterile forceps, remove membrane from the tube and discard in an autoclavable
biohazard bag.
9.4.4 Repeat steps 9.4.1 through 9.4.3 for each membrane sample.
9.4.5 Use 1.5 mL aliquot for DNA extraction using bead-beating, as described in Section 9.6.
9.5 Sample Processing for Water Samples (Small Volume [< 50 mL], Surface or Drinking
Water)
Note: All subsequent procedures involving manipulation of water samples must be carried out in a
BSC using appropriate PPE. Sterile gloves should be used and changed between samples and
as indicated below. The CDC requires BSL-3 handling of this organism. All wastes should be
handled according to the CDC and the BMBL waste management and disposal requirements.
9.5.1 Transfer no more than 30 mL of the water sample to a 50 mL screw cap tube.
19
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Detection of Francisella tularensis in Environmental Samples
9.5.2 Add 10 mL of sterile PBS and mix by vortexing for 30 seconds.
9.5.3 Centrifuge at 3200 x g, with the brake off, for 15 minutes at 4°C.
9.5.4 Remove approximately 37 mL of the supernatant without disturbing/dislodging the pellet.
The volume of supernatant remaining should not be below the conical portion of the tube.
Resuspend the pellet by vortexing for 30 seconds in the remaining volume.
9.5.5 Repeat steps 9.5.1 through 9.5.4 for each water sample.
9.5.6 Use 1.5 mL aliquot for DNA extraction using bead-beating, as described in Section 9.6
9.6 Sample Processing: DNA Extraction and Purification
Note: Alternate DNA extraction-purification procedures may be used (e.g., MagNA-Pure LC
instrument).
9.6.1 In a clean room, using the 8 cap strips, transfer two level capfuls (-100 mg) of the 106
(.im glass beads and two level capfuls (-100 mg) of the 425-600 |_im glass beads (using a
clean strip of caps between bead sizes) into each gasketed, capped 2 mL bead-beating
tube.
9.6.2 In the BSC, pipet 1.5 mL of the suspension (sample eluent) into a pre-labeled, gasketed,
capped bead-beating 2 mL tube containing glass beads. Replace cap on tube securely.
Wipe outside of tube with a 10% pH amended bleach solution (Section 6.18) or bleach
wipes (Section 5.1.3). Store the remaining suspension at 4°C. Repeat for each sample.
9.6.3 Insert tubes in tube holders of the bead-beater (Section 5.5.16) and set the timer for 3
minutes (180 seconds). Bead-beat at 3450 oscillations/minute to disrupt cells to release
the DNA.
9.6.4 Remove tubes from bead-beater (tubes will be warm), and place in a cold block (4°C) for
2 minutes (or until cool to touch). If tubes leak during bead-beating, wipe tubes and
bead-beater thoroughly with a 10% pH amended bleach solution (Section 6.18) or bleach
wipes (Section 5.1.3).
9.6.5 Supernatant Separation and Transfer
• For each sample, label the following: one 1.5 mL microcentrifuge tube, two yellow-top
0.22 |_im Ultrafree®-MC filter units (Section 5.1.29; Millipore® Cat. No. UFC30GV0S),
two Amicon Ultra filter inserts, and six Amicon Ultra collection tubes (Section 5.1.28;
Millipore® Cat. No. UFC510096) with sample ID for each bead-beating tube (Section
9.6.4); and one 0.1 |_im Ultrafree®-MC centrifugal filter device (Section 5.1.30;
Millipore® Cat. No. UFC30VV00).
Note: It may not be necessary to label all the collection tubes as long as the Amicon Ultra
filter insert is clearly labeled.
• In a BSC, centrifuge the bead-beating tubes (Section 9.6.4) at 7000 rpm for 2 minutes in
a microcentrifuge using a fixed angle rotor to pellet beads and particulate matter.
• Using a micropipettor, carefully transfer 0.5 mL of the supernatant to each of the two
0.22 (im yellow top filter units (Section 5.1.29; Millipore® Cat. No. UFC30GV0S).
Avoid beads and particulate matter at bottom of bead-beating tube). Cap the filter units.
• Centrifuge (Section 5.5.6; Eppendorf 5415R/5424R) at 7000 rpm for 3 minutes at 4°C.
20
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Detection of Francisella tularensis in Environmental Samples
Note: Ensure that the supernatant has been filtered. Centrifuge for an additional 2 minutes
if there is any supernatant in the filter.
• Open the filter units; remove the yellow top filter inserts with sterile disposable forceps
(gripping only on the sides) and discard the insert and forceps in an autoclavable
biohazard bag. Transfer 0.5 mL of the filtrate from the collection tube to Amicon® Ultra
filter inserts (Section 5.1.28; Millipore® Cat. No. UFC510096). Do not transfer any
particulate matter that may be evident at bottom of the tubes. Place filter inserts into new
collection tubes (Section 5.1.28; Millipore® Cat. No. UFC50VL96). Cap the filter units.
• Centrifuge (Section 5.5.6; Eppendorf 5415R/5424R) at 7000 rpm for 2 minutes at 4°C.
• Open the filter units. Remove the Amicon® Ultra filter inserts (Section 5.1.28; Millipore®
Cat. No. UFC510096) with disposable forceps (gripping only the sides) and transfer to
new collection tubes (Section 5.1.28; Millipore® Cat. No. UFC50VL96). Dispose of old
collection tubes with filtrate as per CDC BSL-3 requirements (in an autoclavable
biohazard bag).
• Transfer the remaining (0.5 mL) filtrate from all the second yellow top filter units to the
corresponding Amicon® Ultra filter inserts (Section 5.1.28; Millipore® Cat. No.
UFC510096). Do not transfer any particulate matter that may be evident at bottom of
tubes. Cap the filter units.
• Centrifuge at 7000 rpm for 3 minutes at 4°C.
• Open the filter units. Remove the Amicon® Ultra filter inserts using disposable forceps
(gripping only the sides) and transfer to new collection tubes (Section 5.1.28; Millipore®
Cat. No. UFC50VL96). Dispose of old collection tubes with filtrate as per CDC BSL-3
requirements (in an autoclavable biohazard bag).
9.6.6 First Wash
• Add 400 |_iL of IX TE buffer (Section 6.7) to the filter.
• Centrifuge at 7000 rpm for 2 minutes at 4°C.
• Open the filter units. Carefully remove the retentate from the top of the Amicon® Ultra
filter inserts (Section 5.1.28; Millipore® Cat. No. UFC510096), avoiding any particulate
matter visible on filter surface (tilt the tube for better viewing) and transfer liquid into
new Amicon® Ultra filter inserts (Section 5.1.28; Millipore® Cat. No. UFC510096)
inserted in the collection tubes (Section 5.1.28; Millipore; Cat. No. UFC50VL96).
Discard the used Amicon® Ultra filter inserts (Section 5.1.28; Millipore® Cat. No.
UFC510096) and collection tubes (Section 5.1.28; Millipore® Cat. No. UFC50VL96) in
an autoclavable biohazard bag.
9.6.7 Second Wash
• Add 400 |_iL IX TE buffer (Section 6.7) to the Amicon® Ultra filters. Cap the filter units.
• Centrifuge at 7000 rpm for 3 minutes at 4°C.
• Open the filter units. Transfer the Amicon® Ultra filter inserts (Section 5.1.28; Millipore®
Cat. No. UFC510096) with disposable forceps (gripping only the sides) to new collection
tubes (Section 5.1.28; Millipore® Cat. No. UFC50VL96).
21
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Detection of Francisella tularensis in Environmental Samples
9.6.8 Third Wash
• Add 400 |_iL IX TE buffer (Section 6.7) to the Amicon® Ultra filters. Cap the filter units.
• Centrifuge at 7000 rpm for 3 minutes at 4°C.
• Open the filter units. Transfer the Amicon® Ultra filter inserts (Section 5.1.28; Millipore®
Cat. No. UFC510096) with disposable forceps (gripping only the sides) to new collection
tubes (Section 5.1.28; Millipore® Cat. No. UFC50VL96).
9.6.9 Fourth Wash
• Add 400 |_iL of PCR-grade water (Section 6.3) to the Amicon® Ultra filters. Cap the filter
units.
• Centrifuge at 7000 rpm for 1 minute at 4°C.
• Check fluid level in the Amicon® Ultra filter inserts (Section 5.1.28; Millipore® Cat. No.
UFC510096). If fluid level is above 200 (iL, pulse spin for about 10 seconds (or less)
until about 100 |_iL of fluid is retained on top of white base.
• If there is less than 100 |_iL of extract, transfer DNA extract back to the same Amicon®
Ultra filter insert (Section 5.1.28; Millipore® Cat. No. UFC510096) and add 100 |_iL
PCR-grade water and pulse spin to obtain about 100 |_iL on filter.
Note: Very dirty samples may require additional washes to remove any potential inhibitors.
9.6.10 Filtration of DNA Extract Using 0.1 Centrifugal Filter Device (Section 5.1.30)
Centrifugal filtration with 0.1 -|im Ultrafree®-MC filter device following extraction of
DNA allows for the removal of any F. tularensis cells which may have contaminated
DNA preparations, making the samples safe without compromising the sensitivity of the
real-time PCR assay (Reference 16.12).
• Using a micropipettor, carefully remove all of the retentate (~ 100 |aL) from the 0.22 (.un
Amicon® Ultra filter inserts (Section 5.1.28; Millipore® Cat. No. UFC510096) and
transfer to corresponding 0.1 |_im Ultrafree®-MC filter devices (Section 5.1.30; Millipore®
Cat. No. UFC30VV00). Do not allow the micropipettor tip to touch the filter membrane.
Avoid transferring any particulate matter that may be evident at bottom of the tubes.
Close the caps. Discard the Amicon® Ultra filter inserts (Section 5.1.28; Millipore® Cat.
No. UFC510096) with collection tubes (Section 5.1.28; Millipore® Cat. No.
UFC50VL96) into abiohazard autoclave bag.
• Repeat the above step for all the samples/retentates.
• Place the 0.1 |_im Ultrafree®-MC filter devices (Section 5.1.30; Millipore® Cat. No.
UFC30VV00) into a centrifuge (Section 5.4.6; Eppendorf 5415R/5424R).
• Centrifuge at 8000 x g (approximately, 9200 rpm) for 2 minutes at 4°C (Reference
16.12).
• Carefully open the caps and remove the Ultrafree®-MC filter inserts (Section 5.1.30;
Millipore® Cat. No. UFC30VV00) using disposable forceps (gripping only the sides), cap
the collection tubes and dispose of the Ultrafree®-MC inserts (Section 5.1.30; Millipore®
Cat. No. UFC30VV00) and the forceps in an autoclavable biohazard bag. Place the
collection tubes in a cold block (4°C).
22
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Detection ofFrancisella tularensis in Environmental Samples
• Carefully wipe the outside of the collection tubes containing sample DNA extract with a
10% pH amended bleach solution (Section 6.18) or bleach wipes (Section 5.1.3).
• Using clean gloves, place the cold block (4°C) with the tubes containing filter extracts in
DNA loading station/hood in preparation for PGR analyses (Section 9.7).
9.7 Real-time PGR Analyses
1) Reaction Mixture
Target dsDNA
Reporter Dye
5'l I I III I 3' 3' i i i i i ii i i 5' V _
Forward Reverse Quencher Dye
Primer Primer * W
I I I I I I
Quenched
I
T aqMan®Probe
2) Denature Target dsDNA
5' I I II I I : I I I 1 1 I I 1 I 1 I I I 1 1 : I ' 1 1 I I I I I 1 I I I ' I 3'
3' ' ill mi i i 5'
I 3' 3, ii , 5,
A
T Tl r
3) Anneal Primers and Probe ^
#
S'TTT—m
J_l I I LLJ I I 5'
5' I || j| I I I I I I II || I I || || ! I || I I I I I | I I I I I I ' 1 3'
A
1111 II S'
I
,r
4) Extension, Hydrolysis,
and Detection .
^TTT
3, iiiiimiiniiiniWii,
5'm—m—m—n——r— minimi 3'
< 1 1— 5'
Taq DNA
Polymerase
Figure 1. Real-time PGR Amplification.
23
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Detection of Francisella tularensis in Environmental Samples
As compared to traditional PCR, real-time PCR uses a sequence-specific hybridization probe
sequence internal to the amplification primers, in addition to two target gene-specific
amplification primers. The probe is fluorescently labeled at the 5' end with a reporter
dye/fluorophore and at the 3' end with a quencher dye (usually, Black Hole Quenchers®). The
emission of light/fluorescence by the reporter dye is normally quenched by its proximity to the
quencher dye. At the annealing step in a PCR, along with the amplification primers, depending
upon its orientation, the probe sequence also hybridizes to its target site on the DNA strand
downstream from the binding site of one of the primers. During the enzymatic extension step
when the probe comes in contact with the Taq DNA polymerase enzyme, the 5' exonuclease
activity of the enzyme hydrolyzes the probe sequence by cleaving individual nucleotides from the
5' end. Cleavage of the probe releases the reporter dye from the proximal quencher, allowing
emission of measurable fluorescence. Therefore, this assay is also known as the 5' exonuclease
assay, as it relies on the 5' to 3' exonuclease activity of the Taq DNA polymerase enzyme to
hydrolyze the probe. Thus, the PCR amplification of a specific gene sequence can be detected by
monitoring the increase in fluorescence (Figure 1). As the amplification reaction proceeds, more
amplicons become available for probe binding and hydrolysis, and consequently, the fluorescence
signal intensity per cycle increases. The increase in fluorescence can be detected in real time on
PCRthermocyclers. When the fluorescence level crosses a set threshold value at a certain cycle
number during the PCR, the result indicates the presence of the target gene sequence in the DNA
in the sample, which in turn indicates the presence of a target pathogen in the sample. The PCR
can specifically amplify a single copy of target gene sequence and generate millions of copies in a
matter of minutes.
The TaqMan® fluorogenic probe hydrolysis-based real-time PCR assays are commonly used in
biodetection. Using established computer software (e.g., Primer Express™) and genome sequence
databases, bioagent-specific primers and probe nucleotide sequences for these assays are selected
in such a way that they are present only in a specific location on the unique gene and/or virulence
factor gene of interest for the detection and identification of a specific pathogen. These primers
and probe sequences are absent in any other gene of that pathogen or in the genes of any near
neighbor organisms. The primers generate a PCR product (amplicon) of a definite length/size.
For a high-confidence identification of pathogens, PCR assays for multiple pathogen-specific
genes are usually used. Therefore, in this protocol, two single-plex PCR assays are included.
The Ftl and Ft2 PCR assays target the pathogenicity determinant protein D (pdpD), hypothetical
protein and a junction between ISFtu2 and a flanking 3' region, respectively.
Note: This procedure is to be carried out in an area designated for PCR only. A PCR-
workstation that is equipped with an ultraviolet (UV) light for sterilization must be used
for PCR Master Mix preparation. Micropipets and corresponding sterile, aerosol-
resistant pipet tips are used throughout this procedure for the addition of reagents.
Aseptic technique must be used throughout, and all reagents must be kept at or near
4°C.
9.7.1 Decontaminate the PCR workstation by treating all work surfaces with a 10% pH
amended bleach solution (Section 6.18) or bleach wipes (Section 5.1.3), allowing the
bleach to contact the work surface for a minimum of 15 minutes prior to rinsing with
sterile water. Turn on UV light for 15 minutes. After decontamination, discard gloves in
an autoclavable biohazard bag and replace with a new, clean pair.
Note: If gloves become contaminated, they should be disposed of in an autoclavable
biohazard bag and fresh gloves donned. Only open one tube at a time throughout the
process. At no point should more than one tube be open. Do not allow hands (gloved
24
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Detection of Francisella tularensis in Environmental Samples
or otherwise) to pass over an open tube, PCR plate or any reagent container. All used
pipet tips, gloves and tubes must be discarded in an autoclavable biohazard bag.
9.1.2 Determine the number of reactions that are to be run. Include four replicate reactions
each (for each assay) for an NTC (Section 8.6), PC (Section 8.3) and three replicates of
the PNC (Section 8.8) per run. In addition, include three reactions for each sample
including field blanks (Section 8.7) and two reactions for the EIC (Section 8.5) for each
sample. Prepare a sufficient volume of Master Mix to allow for a minimum of one extra
reaction for every 10 reactions, so that there is enough Master Mix regardless of pipetting
variations. For example, if 10 samples are to be analyzed for each PCR assay, a total of
61 reactions would be required [e.g., 4-NTC, 4-PC, 3-PNC, 30-samples and 20-EICs],
Therefore, the volume of PCR Master Mix prepared should be sufficient for 70 reactions
per PCR assay.
9.7.3 Based on the example provided above (i.e., 10 samples), the amount of Master Mix
required for each assay would be as indicated in Table 4.
Table 4. Example F. tularensis Single-plex PCR Assay Master Mix Preparation for
70 Reactions
Ui'iiiicnl
Volume pei'
reiiclion
(.ill.)
loliil
Volume
(.ill.)
liiiiil
( onceiili'iilioii
TaqMan® 2X Universal Master Mix
12.5
875
IX
Platinum® Taq DNA Polymerase
0.25 (1.25
Units)
17.5
1.25 Units
Forward primer, 10 |_lM
0.5
35
0.20 (iM
Reverse primer, 10 |_lM
0.5
35
0.20 (iM
Probe, 4 |_lM
0.4
28
0.064 (iM
PCR-grade water
5.85
409.5
N/A
Total Volume
20
1400
Note: The PC and NTC controls must be analyzed prior to sample analyses to verify that the
Master Mix works properly and is free of contamination.
9.7.4 In a clean PCR-preparation hood, pipet 20 |_iL of Master Mix to four wells of the PCR
plate. Label two wells as NTC and two as PC.
9.7.5 Add 5 |_iL of PCR-grade water into the NTC wells.
9.7.6 Cover the plate with adhesive plate sealer and transfer the PCR plate to the BSC.
Remove the seal and add 5 |_iL of the PC (/¦'. tularensis DNA [10 pg/(.iL|) to the PC wells.
Note: This step must be performed in the BSC outside the PCR clean room set-up area.
Change gloves.
9.7.7 Seal PCR plate with optical seal, using plate sealer for good contact. Change gloves.
9.7.8 Centrifuge sealed PCR plate for 1 minute at 2000 rpm and 4°C, using the PCR plate
safety cups or mini-plate centrifuge in the BSC.
9.7.9 Open the centrifuge safety cup and transfer PCR plate to the ABI 7500 Fast
thermocycler.
25
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Detection of Francisella tularensis in Environmental Samples
9.7.10 The PCR thermal cycling conditions on the ABI 7500 Fast are provided in Table 5.
Fluorescence is automatically measured at the end of the 60°C annealing-extension
combined step.
Table 5. PCR Thermal Cycling Conditions"'b
Slops
I NC/
Iiicii l>;il i«ui
Ampli 1 :i(| (.old
Acli\;ilion
PCR. 45 Cjck's'1
Hold
Hold
Dciiiilui'iilioii
.\nnc;iliii^/l'A tension
Temperature
50°C
95°C
95°C
60°C
Time
2 minutes
10 minutes
5 seconds
20 seconds6
a Run Mode: Fast 7500
b Reaction volume 25 |iL
0 Uracil-DNA glycosylase
d Fast Ramp: 3.5°C/s up and 3.5°C/s down
e 30 seconds for ABI 7500 Fast Dx instrument
9.7.11 If the Master Mix test results show "True Positive" assay detection for the PC and "True
Negative" assay detection for the NTC, then proceed with analyses of samples. If the
results are not "True" then repeat the PCR Master Mix preparation and testing protocol
and reanalyze.
9.7.12 In a clean PCR-preparation hood, pipet 20 |aL of Master Mix into the required number of
wells of a new PCR plate (as per the number of samples to be analyzed). An eight-
channel micropipettor can be used to add the Master Mix to the plate. Label two wells as
NTC and two as PC. Label the rest of the wells such that there are five wells for each
sample (three wells for actual sample analyses and two wells for EICs for each sample).
9.7.13 Add 5 |_iL of PCR-grade water into the NTC wells.
9.7.14 Cover the plate with adhesive plate sealer and transfer the PCR plate to the BSC.
Remove the seal and add 5 |_iL of the PC (/¦'. tularensis DNA [10 pg/(.iL|) to the PC wells.
Note: These steps must be performed in the BSC outside the PCR clean room set-up area.
Change gloves.
9.7.15 Add 5 |_iL of the PNC extract to the three PNC wells.
9.7.16 Add 5 |_iL of each sample DNA extract to the respective sample wells and EIC wells.
9.7.17 Add 1 (.iL of the PC (/¦'. tularensis DNA [50 pg/jj.L]) to all the EIC wells.
Note: To minimize cross contamination, the EICs should not be placed next to the field
samples when setting up the PCR tray.
9.7.18 Seal PCR plate with optical seal, using a clear Edge Seal for good contact. Change
gloves.
9.7.19 Centrifuge sealed PCR plate for 1 minute at 2000 rpm and 4°C, using the PCR plate
safety cups or mini-plate centrifuge in the BSC.
9.7.20 Transfer PCR plate to the ABI 7500 Fast thermocycler.
9.7.21 Run PCR using the thermocycling conditions as described in Section 9.7.10.
26
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Detection of Francisella tularensis in Environmental Samples
9.7.22 After completion of thermocycling, discard sealed PCR plate in an autoclavable
biohazard bag.
Note: PCR plates with amplified product should not be opened in the laboratory.
9.7.23 Laboratory clean-up procedures
• Dispose of all biological materials in biohazard autoclave bags (double bagged).
• Autoclave all waste materials at the end of the work day.
• Decontaminate counters and equipment with a 10% pH amended bleach solution (Section
6.18) or bleach wipes (Section 5.1.3), followed by 70% isopropyl and a deionized water
final rinse.
9.7.24 Refer to Section 12.1 for Data Analyses and Calculations.
27
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Detection of Francisella tularensis in Environmental Samples
10.0 Culture Method
Acceptable sample types: Gauze wipes (2" * 2" 50% rayon/50% polyester [Kendall™ Versalon™
Cat. No. 8042 or equivalent]), air filters (37 mm Fluoropore™ [Millipore Cat. No. FSLW04700 or
equivalent]), swabs (macrofoam [VWR Cat. No. 89022-994 small swabs or 89022-984 large
swabs, or equivalent]), Sponge-Stick sampling tools, (3M™ Inc. Cat. No. SSL10NB or equivalent)
and drinking water and decontamination waste water.
Media sterility checks (Section 8.2) and positive controls (Section 8.4) should be analyzed every
day that samples are analyzed, to ensure that all media and reagents are performing properly.
10.1 Sample Processing and Plating for Sponge-Sticks and Wipes
Note: All subsequent procedures involving manipulation of Sponge-Sticks and wipes must be carried
out in a BSC using appropriate PPE. Sterile gloves should be used and changed between
samples and as indicated below. The CDC requires BSL-3 handling of this organism. All
wastes should be handled according to the CDC and the BMBL waste management and disposal
requirements.
10.1.1 Recover Bacteria from Sponge-Sticks and Wipes
• If the Sponge-Stick sponge/wipe sample is not in a Stomacher® bag, aseptically transfer it
to a Stomacher® bag using sterile forceps.
• Using aseptic technique, remove the plastic stick base holding the sponge together. Place
gloved hands on the outside of the Stomacher® bag, grip the Sponge-Stick head on both
sides and peel the sponge away from the base and unfold the sponge. Be careful not to
puncture bag with edge of stick base. Using sterile forceps remove stick base from bag
and discard into a biohazard autoclave bag. Change forceps between samples.
• Add 90 mL of PBST (0.05% Tween® 20, Section 6.5) to each bag. Set Stomacher®
(Section 5.5.19) to 200 rpm.
• Place a bag containing a sample into the Stomacher® (Section 5.5.19) so the Sponge-
Stick sponge/wipe rests evenly between the paddles and homogenize each sample for 1
minute at 200 rpm.
• Open the door of the Stomacher® (Section 5.5.19) and remove the bag. Grab the
sponge/wipe from the outside of the bag with your gloved hands. With the bag closed,
move the sponge/wipe to the top of the bag while using your hands to squeeze excess
liquid from the sponge/wipe.
• Open the bag and remove sponge/wipe using sterile forceps. Retain the sponge/wipe in a
labeled specimen cup (Section 5.3.5).
• Follow steps described above for each sample, changing forceps between samples.
• Allow bags to sit for 10 minutes to allow elution suspension foam to settle.
• Gently mix the elution suspension in the Stomacher® bag up and down 3 times with a
sterile 50 mL pipet. Remove half of the suspension volume (-47 mL) and place it in a
labeled 50 mL screw cap centrifuge tube. Place the remaining suspension (-47 mL) into
a second 50 mL tube. Adjust the suspension volumes in both the tubes to ensure they are
28
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Detection of Francisella tularensis in Environmental Samples
similar.
• Process elution suspension for each sample as described above.
• Place 50 mL tubes into sealing centrifuge buckets and decontaminate centrifuge buckets
before removing them from the BSC.
• Centrifuge tubes at maximum speed (-3200 x g) with the brake off, for 15 minutes in a
swinging bucket rotor at 4°C.
• Using a sterile 50 mL pipet for each sample, remove approximately 44 mL of the
supernatant from each sample tube and discard it in an autoclavable biohazard container.
The pellet may be easily disturbed and not visible, so keep the pipet tip away from the
bottom of the tube.
• Set the vortexer (Section 5.5.10) to the high setting. Set the sonicator water bath to high.
• Vortex the tubes for 30 seconds and transfer the tubes to the sonicator bath and sonicate
for 30 seconds. Repeat the vortex and sonication cycles two more times.
Note: As an alternative to sonication, tubes may be vortex mixed for two minutes in 10
second bursts using a multi-tube vortexer.
• Remove suspension from one tube with a sterile 5 mL pipet and combine it with the
suspension in the other tube from the same sample. Measure final volume of suspension
with 5 mL pipet and record the result on the tube and data sheet.
• Follow vortexing and sonication steps for each sample.
10.1.2 Serially Dilute the Suspension in PBS
• Vortex the elution suspension on high for 30 seconds.
a. Transfer 1 mL of the suspension from the 50 mL tube to a 15 mL tube containing 9
mL of PBS. Recap the tube and vortex it on high for 30 seconds. This is the
10"1 suspension.
b. Open the cap of the 10"1 suspension tube and transfer 1 mL of this suspension into a
new 15 mL tube containing 9 mL of PBS. Recap the tube and vortex on high for 30
seconds. This is the 10~2 suspension.
c. The above results in 3 cell suspensions: the initial wipe elution suspension (undiluted)
and 2 serial dilutions of the suspension in PBS (101 and 10~2).
• Repeat steps (a) through (b) for each sample.
10.1.3 Culture Cell Suspensions on CHOC with IsoVitaleX and CHAB
To ensure that the agar surface is dry prior to use, plates should be made several days in
advance and stored inverted at room temperature or dried using a laminar-flow hood.
Note: Plating of 0.1 mL results in an additional 1:10 dilution of each of the suspensions.
Each of the following will be conducted in triplicate, resulting in the evaluation of 18
spread plates per sample:
a. After vortexing tubes, pipet 0.1 mL of undiluted suspension onto the surface of pre-
dried CHOC with IsoVitaleX plate and a pre-dried CHAB plate (labeled 101).
29
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Detection ofFrancisella tularensis in Environmental Samples
b. After vortexing tubes, pipet 0.1 mL of 10"1 suspension onto surface of pre-dried
CHOC with IsoVitaleX plate and a pre-dned CHAB plate (labeled 10~2).
c. After vortexing tubes, pipet 0.1 mL of 10"2 suspension onto surface of pre-dried
CHOC with IsoVitaleX plate and a pre-dried CHAB plate (labeled 10"3).
• After pipetting the 6 spread plates for each dilution. Beginning with the 10"3 dilution, use
a stenle L-Shaped spreader to distribute the inoculum over the surface of the medium by
rotating the dish by hand or on a turntable. Ensure that inoculum is evenly distributed
over the entire surface of the plate. Use a different sterile spreader for each plate. Repeat
for the next two dilutions 10"2 and 10_I, in that order.
• Allow inoculum to absorb into the medium completely.
10.1.4 Incubate and Enumerate Colonies
Invert the CHOC with IsoVitaleX and CHAB plates and incubate them at 35°C - 37°C
for a maximum of 7 days. Plates should be examined at 24-hour intervals for a maximum
of 7 days, if necessary.
• CHOC with IsoVitaleX Plates
a. F. tularensis produces gray-white, opaque colonies, usually too small to be seen as
individual colonies at 24 hours. After incubation for 48 hours or more, colonies are
approximately 1-2 mm in diameter, white to gray to bluish-gray, opaque, flat, with an
entire edge, smooth and have a shiny surface (Figure 2).
b. Count the number of F. tularensis colonies on each plate and record results.
• CHAB Plates
a. F. tularensis produces smooth, entire edge, greenish-white, and butyrous (buttery)
with opalescent sheen colonies at 48 to 72 hours. Colonies are usually 2 to 4 mm
after incubation for 48 to 72 hours (Figure 2).
b. Count the number of F. tularensis colonies on each plate and record results.
Figure 2. Francisella tularensis colonies on CHOC (left) and CHAB (right) agar after 48 hours.
(Source: Public Health Image Library, Centers for Disease Control and Prevention)
30
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Detection of Francisella tularensis in Environmental Samples
• Plate Counts
a. If the number of colonies is < 250/plate, record actual number.
b. If the number of colonies is > 250/plate, record as "too numerous to count" (TNTC).
c. If no target colonies are observed, record as "None detected" and proceed to
evaluation of growth on MicroFunnel™ plates (Section 10.1.5).
A minimum of 3 typical colonies should be confirmed using real-time PCR (Section
10.5).
10.1.5 Capture Cells on MicroFunnel™ Filter Membranes and Culture
• Place two 0.45 (.un (pore-size) MicroFunnel™ filter funnels (Section 5.3.4) on the vacuum
manifold and moisten membrane with 5 mL PBS. All filtering should be done with a
vacuum pressure < 10 psi.
• With the vacuum valve closed (and vacuum pressure released), place 10 mL of PBS into
each filter cup. Add 1.0 mL of the undiluted elution suspension (Section 10.1.1) to each
of two MicroFunnel™ cups.
• Open the vacuum valve and filter the suspension. Close the valve and release the vacuum
pressure. Rinse the walls of each MicroFunnel™ cup with 10 mL of PBS and filter. Open
the valve and complete filtration by pouring remaining rinsate through the filter.
• Squeeze the walls of the MicroFunnel™ cup gently and separate the walls from the base
holding the filter. Discard cup in an autoclavable biohazard bag. Remove the
membranes with sterile forceps and place them grid-side up on labeled CHOC with
IsoVitaleX and CHAB plates. Make sure that the filters are in contact with the surface of
the agar. If an air pocket occurs under the filter, use the sterile forceps to lift the edge of
the filter to release the air pocket.
• Record the exact volume of the suspension filtered (e.g., 1.0 mL) on each plate.
• Repeat steps (Section 10.1.5) described above for each sample.
Invert and incubate CHOC with IsoVitaleX and CHAB plates at 35°C - 37°C for a
maximum of 7 days. Plates should be examined daily for growth. Count the number of
colonies and record results.
• Plate Counts
a. If the number of colonies is < 80/plate, record actual number.
b. If the number of colonies is > 80/plate, record as "TNTC."
c. Ideally, plates with 20-80 colonies should be used to calculate the number of colony
forming units (CFUs) per sample, as described in Section 12.2.2.
Confirm 1-3 colonies using real-time PCR (Section 10.5).
Note: For faster sample analysis results during the initial stages of an incident (e.g., incident
characterization) and during post-decontamination/clearance phase, it is
recommended that the remainder of all suspensions (e.g., undiluted, Iff1 and Iff2
dilutions) be filtered using an additional MicroFunnel™ and plated as described above
instead of proceeding with enrichment in trypticase™ soy broth (TSB) with IsoVitaleX.
31
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Detection of Francisella tularensis in Environmental Samples
However, if a problem of background microorganisms overgrowth on a filter is
anticipated, the enrichment culture would be required.
10.1.6 Enrich in TSB with IsoVitaleX
• Add the remainder of the undiluted suspension to the specimen cup containing the
corresponding sponge/wipe. Add 40 mL TSB with IsoVitaleX to the tube. Repeat for
each sample. Incubate the specimen cups at 35°C - 37°C. F. tularensis grows slowly;
the inoculated broth should be incubated and observed for at least 10 days.
• Observe the TSB with IsoVitaleX Enrichment
a. If broth is not cloudy, record as no growth (NG) and incubate for an additional 24
hours.
b. If broth is cloudy, record as positive growth (G+) and proceed to next step.
c. Cap the cup tightly and mix TSB with IsoVitaleX with growth for 30 seconds. Use a
sterile loop to remove a loopfiil of broth with a 10 |_iL loop and streak on a CHAB
plate for isolation. Repeat two times for a total of three CHAB isolation plates.
d. Incubate the CHAB isolation plates and TSB with IsoVitaleX with growth for a
maximum of 10 days at 35°C - 37°C.
e. Examine plates for F. tularensis-suspect colonies. If any colonies are isolated,
proceed to PCR confirmation (Section 10.5).
f. If no suspect colonies are observed, perform PCR on TSB with IsoVitaleX with
growth according to Section 10.5.
10.2 Sample Processing and Plating for Swabs
Note: All subsequent procedures involving manipulation of swabs must be carried out in a BSC
using appropriate PPE. Sterile gloves should be used and changed between samples and as
indicated below. The CDC requires BSL-3 handling of this organism. All wastes should be
handled according to the CDC and the BMBL waste management and disposal requirements.
10.2.1 Recover Bacteria from Swabs
• If the swabs are not in screw cap centrifuge tubes, transfer each swab to sterile, plastic
15 mL screw cap centrifuge tube using sterile forceps.
• If necessary, cut the handle of the swab to fit into the tube using sterile scissors. Use
sterile forceps and scissors for each sample.
• Add 5 mL of PBS to each tube and vortex on high for 2 minutes.
• Using sterile forceps, remove the swab from the 15 mL centrifuge tube. Use the forceps
to press the tip of the swab against the inside of the tube to remove extra liquid from the
foam tip.
• Place the swab into a labeled 50 mL tube with 5 mL TSB with IsoVitaleX and set aside.
• Repeat steps described above for each swab sample.
10.2.2 Serially Dilute the Cell Elution Suspension in PBS
32
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Detection of Francisella tularensis in Environmental Samples
• Vortex the elution suspension on high for 30 seconds.
a. Transfer 1 mL of the suspension from the 50 mL tube to a 15 mL tube containing
9 mL of PBS. Recap the tube and vortex it on high for 30 seconds. This is the 10"1
suspension.
b. Open the cap of the 10"1 suspension tube and transfer 1 mL of this suspension into a
new 15 mL tube containing 9 mL of PBS. Recap the tube and vortex on high for 30
seconds. This is the 10~2 suspension.
c. The above results in 3 cell suspensions: the initial wipe elution suspension
(undiluted) and 2 serial dilutions of the suspension in PBS (10"1 and 10~2).
• Repeat steps (a) through (b) for each sample.
10.2.3 Culture Cell Suspensions on CHOC with IsoVitaleX and CHAB
To ensure that the agar surface is dry prior to use, plates should be made several days in
advance and stored inverted at room temperature or dried using a laminar-flow hood.
Note: Plating of 0.1 mL results in an additional 1:10 dilution of each of the suspensions.
Each of the following will be conducted in triplicate, resulting in the evaluation of 18
spread plates per sample:
a. After vortexing tubes, pipet 0.1 mL of undiluted suspension onto the surface of pre-
dried CHOC with IsoVitaleX plate and a pre-dried CHAB plate (labeled 101).
b. After vortexing tubes, pipet 0.1 mL of 10"1 suspension onto surface of pre-dried
CHOC with IsoVitaleX plate and a pre-dried CHAB plate (labeled 10~2).
c. After vortexing tubes, pipet 0.1 mL of 10"2 suspension onto surface of pre-dried
CHOC with IsoVitaleX plate and a pre-dried CHAB plate (labeled 10~3).
• After pipetting the 6 spread plates for each dilution. Beginning with the 10~3 dilution, use
a sterile L-Shaped spreader to distribute the inoculum over the surface of the medium by
rotating the dish by hand or on a turntable. Ensure that inoculum is evenly distributed
over the entire surface of the plate. Use a different sterile spreader for each plate. Repeat
for the next two dilutions 10~2 and 101, in that order.
• Allow inoculum to absorb into the medium completely.
10.2.4 Incubate and Enumerate Colonies
Invert the CHOC with IsoVitaleX and CHAB plates and incubate them at 35°C - 37°C
for a maximum of 7 days. Plates should be examined at 24-hour intervals for a maximum
of 7 days, if necessary.
• CHOC with IsoVitaleX Plates
a. F. tularensis produces gray-white, opaque colonies, usually too small to be seen as
individual colonies at 24 hours. After incubation for 48 hours or more, colonies are
approximately 1-2 mm in diameter, white to gray to bluish-gray, opaque, flat, with an
entire edge, smooth and have a shiny surface (Figure 2).
b. Count the number of F. tularensis colonies on each plate and record results.
33
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Detection of Francisella tularensis in Environmental Samples
• CHAB Plates
a. F. tularensis produces smooth, entire edge, greenish-white, and butyrous with
opalescent sheen colonies at 48 to 72 hours. Colonies are usually 2 to 4 mm after
incubation for 48 to 72 hours (Figure 2).
b. Count the number of F. tularensis colonies on each plate and record results.
• Plate Counts
a. If the number of colonies is < 250/plate, record actual number.
b. If the number of colonies is > 250/plate, record as "too numerous to count" (TNTC).
c. If no target colonies are observed, record as "None detected" and proceed to
evaluation of growth on MicroFunnel™ plates (10.2.5).
A minimum of 3 typical colonies should be confirmed using real-time PCR (Section
10.5).
10.2.5 Capture Cells on MicroFunnel™ Filter Membranes and Culture
• Place two, 0.45 (.un (pore-size) MicroFunnel™ filter funnels (Section 5.3.4) on the
vacuum manifold and moisten membrane with 5 mL PBS. All filtering should be done
with a vacuum pressure < 10 psi. With the vacuum valve closed (and vacuum pressure
released), place 10 mL of PBS into each filter cup. Add 1.0 mL of the undiluted elution
suspension (Section 10.2.2 [c]) to each of two MicroFunnel™ cups.
• Open the vacuum valve and filter the suspension. Close the valve and release the vacuum
pressure. Rinse the walls of each MicroFunnel™ cup with 10 mL of PBS and filter. Open
the valve and complete filtration.
• Squeeze the walls of the MicroFunnel™ cup gently and separate the walls from the base
holding the filter. Discard cup in an autoclavable biohazard bag. Remove the
membranes with sterile forceps and place them grid-side up on labeled CHOC with
IsoVitaleX and CHAB plates. Ensure that the filter is in contact with the surface of the
agar. If an air pocket occurs under the filter, use the sterile forceps to lift the edge of the
filter to release the air pocket.
• Record the exact volume of the suspension filtered (1.0 mL) on each plate.
• Repeat steps (Section 10.2.5) described above for each sample.
• Invert and incubate CHOC with IsoVitaleX and CHAB plates at 35°C - 37°C for a
maximum of 7 days. Count the number of colonies and record results.
• Plate Counts
a. If the number of colonies is < 80/plate, record actual number.
b. If the number of colonies is > 80/plate, record as "TNTC."
c. Ideally, plates with 20-80 colonies should be used to calculate the number of CFUs
per sample, as described in Section 12.2.2.
Confirm 1-3 colonies using real-time PCR (Section 10.5).
Note: For faster sample analysis results during the initial stages of an incident (e.g., incident
characterization) and during post-decontamination/clearance phase, it is
34
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Detection of Francisella tularensis in Environmental Samples
recommended that the remainder of all suspensions (e.g., undiluted, Iff1 and Iff2
dilutions) be filtered using an additional MicroFunneP' and plated as described above
instead of proceeding with enrichment in TSB with IsoVitaleX. However, if a problem
of background microorganisms overgrowth on a filter is anticipated, the enrichment
culture would be required.
10.2.6 Enrich in TSB with IsoVitaleX
• Add the remainder of the undiluted suspension to the specimen cup containing the
corresponding sponge/wipe. Add 40 mL TSB with IsoVitaleX to the tube. Repeat for
each sample. Incubate the specimen cups at 35°C - 37°C. F. tularensis grows slowly;
the inoculated broth should be incubated and observed for at least 10 days.
• Observe the TSB Enrichment
a. If broth is not cloudy, record as no growth (NG) and incubate for an additional 24
hours.
b. If broth is cloudy, record as positive growth (G+) and proceed to next step.
c. Cap the cup tightly and mix TSB with IsoVitaleX with positive growth for 30
seconds. Use a sterile loop to remove a loopful of broth with a 10 |_iL loop and streak
on a CHAB plate for isolation. Repeat two times for a total of three CHAB isolation
plates.
d. Incubate the CHAB isolation plates and TSB with IsoVitaleX with growth at 35°C -
37°C for a maximum of 10 days.
e. Examine plates for F. tularensis-suspect colonies. If any colonies are isolated,
proceed to PCR confirmation (Section 10.5).
f. If no suspect colonies are observed, perform PCR on TSB with IsoVitaleX with
growth according to Section 10.5.
10.3 Sample Processing and Plating for Air Filters
Note: All subsequent procedures involving manipulation of air filters must be carried out in a BSC
using appropriate PPE. Sterile gloves should be used and changed between samples and as
indicated below. The CDC requires BSL-3 handling of this organism. All wastes should be
handled according to the CDC and the BMBL waste management and disposal requirements.
10.3.1 Recover Bacteria from Air Filters
• If the air filters are not in 50 mL tubes, aseptically transfer each sample to a sterile 50 mL
tube using sterile forceps. Change forceps between samples.
• Add 5 mL of sterile PBS into a leak-proof, 50 mL conical tube containing an air filter and
vortex on high for 2 minutes.
• Transfer liquid to a sterile, labeled 50 mL tube.
• Retain air filter in the initial 50 mL conical tube and set aside.
• Repeat the steps described above for each air filter.
10.3.2 Serially Dilute the Suspension in PBS
• Vortex the elution suspension on high for 30 seconds.
35
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Detection of Francisella tularensis in Environmental Samples
a. Transfer 1 mL of the suspension from the 50 mL tube to a 15 mL tube containing
9 mL of PBS. Recap the tube and vortex it on high for 30 seconds. This is the 10"1
suspension.
b. Open the cap of the 10"1 suspension tube and transfer 1 mL of this suspension into a
new 15 mL tube containing 9 mL of PBS. Recap the tube and vortex on high for 30
seconds. This is the 10~2 suspension.
c. Open cap of the 10~2 suspension tube and transfer 1 mL of this suspension into a new
15 mL tube containing 9 mL of PBS. Recap the PBS tube and vortex on high for 30
seconds. This is the 10~3 suspension.
d. The above results in 4 cell suspensions: the initial stock elution suspension (undiluted)
and three serial dilutions of the suspension in PBS (101, 10~2 and 10~3).
• Repeat steps (a) through (c) for each sample.
10.3.3 Culture Cell Suspensions on CHOC with IsoVitaleX and CHAB
To ensure that the agar surface is dry prior to use, plates should be made several days in
advance and stored inverted at room temperature or dried using a laminar-flow hood.
Note: Plating of 0.1 mL results in an additional 1:10 dilution of each of the suspensions.
Each of the following will be conducted in triplicate, resulting in the evaluation of 24
spread plates per sample:
a. After vortexing tubes, pipet 0.1 mL of undiluted suspension onto the surface of pre-
dried CHOC with IsoVitaleX plate and a pre-dried CHAB plate (labeled 101).
b. After vortexing tubes, pipet 0.1 mL of 10"1 suspension onto surface of pre-dried
CHOC with IsoVitaleX plate and a pre-dried CHAB plate (labeled 10~2).
c. After vortexing tubes, pipet 0.1 mL of 10"2 suspension onto surface of pre-dried
CHOC with IsoVitaleX plate and a pre-dried CHAB plate (labeled 10~3).
d. After vortexing tubes, pipet 0.1 mL of 10-3 suspension onto surface of pre-dried SBA
plate and a pre-dried CIN plate (labeled 10~4).
• After pipetting the 6 spread plates for each dilution. Beginning with the 10"3 dilution, use
a sterile L-Shaped spreader to distribute the inoculum over the surface of the medium by
rotating the dish by hand or on a turntable. Ensure that inoculum is evenly distributed
over the entire surface of the plate. Use a different sterile spreader for each plate. Repeat
for the next two dilutions 10"2 and 10"1, in that order.
• Allow inoculum to absorb into the medium completely.
10.3.4 Incubate and Enumerate Colonies
Invert the CHOC with IsoVitaleX and CHAB plates and incubate them at 35°C - 37°C
for a maximum of 7 days. Plates should be examined at 24-hour intervals for a maximum
of 7 days, if necessary.
• CHOC with IsoVitaleX Plates
a. F. tularensis produces gray-white, opaque colonies, usually too small to be seen as
individual colonies at 24 hours. After incubation for 48 hours or more, colonies are
36
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Detection of Francisella tularensis in Environmental Samples
approximately 1-2 mm in diameter, white to gray to bluish-gray, opaque, flat, with an
entire edge, smooth and have a shiny surface (Figure 2).
b. Count the number of F. tularensis colonies on each plate and record results.
• CHAB Plates
a. F. tularensis produces smooth, entire edge, greenish-white, and butyrous with
opalescent sheen colonies at 48 to 72 hours. Colonies are usually 2 to 4 mm after
incubation for 48 to 72 hours (Figure 2).
b. Count the number of F. tularensis colonies on each plate and record results.
c. Count the number of colonies on each plate and record results.
• Plate Counts
a. If the number of colonies is < 250/plate, record actual number.
b. If the number of colonies is > 250/plate, record as "too numerous to count" (TNTC).
c. If no target colonies are observed, record as "None detected" and proceed to
evaluation of growth on MicroFunnel™ plates (Section 10.3.5).
A minimum of 3 typical colonies should be confirmed using real-time PCR (Section
10.5).
10.3.5 Capture Cells on MicroFunnel™ Filter Membranes and Culture
• Place two, 0.45 (.un (pore-size) MicroFunnel™ filter funnels (Section 5.3.4) on the
vacuum manifold and moisten membrane with 5 mL PBS. All filtering should be done
with a vacuum pressure 10 psi.
• With the vacuum valve closed (and vacuum pressure released), place 10 mL of PBS into
each filter cup. Add 1.0 mL of the undiluted elution suspension (Section 10.3.1 to each
of two MicroFunnel™ cups.
• Open the vacuum valve and filter the suspension. Close the valve and release the vacuum
pressure. Rinse the walls of each MicroFunnel™ cup with 10 mL of PBS and filter. Open
the valve and complete filtration by pouring remaining rinsate through the filter.
• Squeeze the walls of the MicroFunnel™ cup gently and separate the walls from the base
holding the filter. Discard cup in an autoclavable biohazard bag. Remove the
membranes with sterile forceps and place them grid-side up on labeled CHOC with
IsoVitaleX and CHAB plates. Ensure that the filter is in contact with the surface of the
agar. If an air pocket occurs under the filter, use the sterile forceps to lift the edge of the
filter to release the air pocket.
• Record the exact volume of the suspension filtered (1.0 mL) on each plate.
• Repeat steps (Section 10.3.5) described above for each sample.
• Invert and incubate CHOC with IsoVitaleX and CHAB plates at 35°C - 37°C for a
maximum of 7 days. Plates should be examined daily for growth. Count the number of
colonies and record results.
• Plate Counts
a. If the number of colonies is < 80/plate, record actual number.
37
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Detection of Francisella tularensis in Environmental Samples
b. If the number of colonies is > 80/plate, record as "TNTC."
c. Ideally, plates with 20-80 colonies should be used to calculate the number of CFUs
per sample, as described in Section 12.2.2.
Confirm 1-3 colonies using real-time PCR (Section 10.5).
Note: For faster sample analysis results during the initial stages of an incident (e.g., incident
characterization) and during post-decontamination/clearance phase, it is
recommended that the remainder of all suspensions (e.g., undiluted, Iff1 and Iff2
dilutions) be filtered using an additional MicroFunnel™ and plated as described above
instead of proceeding with enrichment in TSB with IsoVitaleX. However, if a problem
of background microorganisms overgrowth on a filter is anticipated, the enrichment
culture would be required.
10.3.6 Enrich in TSB with IsoVitaleX
• Add the remainder of the undiluted suspension to the specimen cup containing the
corresponding sponge/wipe. Add 40 mL TSB with IsoVitaleX to the tube. Repeat for
each sample. Incubate the specimen cups at 35°C - 37°C. F. tularensis grows slowly;
the inoculated broth should be incubated and observed for at least 10 days.
• Observe the TSB with IsoVitaleX Enrichment
a. If broth is not cloudy, record as no growth (NG) and incubate for an additional 24
hours.
b. If broth is cloudy, record as positive growth (G+) and proceed to next step.
c. Cap the cup tightly and mix TSB with IsoVitaleX with positive growth for 30
seconds. Use a sterile loop to remove a loopful of broth with a 10 |_iL loop and streak
on a CHAB plate for isolation. Repeat two times for a total of three CHAB isolation
plates.
d. Incubate the CHAB isolation plates and TSB with IsoVitaleX with growth at 35°C -
37°C for a maximum of 10 days.
e. Examine plates for F. tularensis-suspect colonies. If any colonies are isolated,
proceed to PCR confirmation (Section 10.5).
f. If no suspect colonies are observed, perform PCR on TSB with IsoVitaleX with
10.4 Sample Processing and Plating for Water Samples
It is anticipated that the large volume water sample has undergone primary and secondary
concentration and the resultant concentrated sample has been filtered through a membrane filter.
Therefore, this sub-section describes the procedure for processing of such a membrane filter
received in a 50 mL screw cap tube or other appropriate container.
Note: All subsequent procedures involving manipulation of water samples and membranes must be
carried out in a BSC using appropriate PPE. Sterile gloves should be used and changed
between samples and as indicated below. The CDC requires BSL-3 handling of this organism.
All wastes should be handled according to the CDC and the BMBL waste management and
disposal requirements.
38
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Detection of Francisella tularensis in Environmental Samples
10.4.1 Recover Bacteria from the MicroFunnel™ Membrane
• If the membranes are not in 50 mL tubes, aseptically transfer each sample to a sterile 50
mL tube using sterile forceps. Change forceps between samples.
• Add 5 mL of sterile PBS into a screw cap, 50 mL conical tube containing a membrane
filter and vortex on high for 2 minutes.
• Transfer liquid to a sterile, labeled 50 mL tube.
• Retain membrane filter in the initial 50 mL conical tube and set aside.
• Repeat the steps described above for each membrane.
10.4.2 Serially Dilute the Suspension in PBS
• Vortex the elution suspension on high for 30 seconds.
a. Transfer 1 mL of the suspension from the 50 mL tube to a 15 mL tube containing
9 mL of PBS. Recap the tube and vortex it on high for 30 seconds. This is the 10"1
suspension.
b. Open the cap of the 10"1 suspension tube and transfer 1 mL of this suspension into a
new 15 mL tube containing 9 mL of PBS. Recap the tube and vortex on high for 30
seconds. This is the 10~2 suspension.
c. Open cap of the 10~2 suspension tube and transfer 1 mL of this suspension into a new
15 mL tube containing 9 mL of PBS. Recap the PBS tube and vortex on high for 30
seconds. This is the 10~3 suspension.
d. The above results in 4 cell suspensions: the initial sock elution suspension (undiluted)
and 3 serial dilutions of the suspension in PBS (101, 10"2 and 10"3).
• Repeat steps (a) through (c) for each sample.
10.4.3 Culture Cell Suspensions on CHOC with IsoVitaleX and CHAB
To ensure that the agar surface is dry prior to use, plates should be made several days in
advance and stored inverted at room temperature or dried using a laminar-flow hood.
Note: Plating of 0.1 mL results in an additional 1:10 dilution of each of the suspensions.
Each of the following will be conducted in triplicate, resulting in the evaluation of 24
spread plates per sample:
a. After vortexing tubes, pipet 0.1 mL of undiluted suspension onto the surface of pre-
dried CHOC with IsoVitaleX plate and a pre-dried CHAB plate (labeled 101).
b. After vortexing tubes, pipet 0.1 mL of 10"1 suspension onto surface of pre-dried
CHOC with IsoVitaleX plate and a pre-dried CHAB plate (labeled 10~2).
c. After vortexing tubes, pipet 0.1 mL of 10"2 suspension onto surface of pre-dried
CHOC with IsoVitaleX plate and a pre-dried CHAB plate (labeled 10~3).
d. After vortexing tubes, pipet 0.1 mL of 10"3 suspension onto surface of pre-dried
CHOC with IsoVitaleX plate and a pre-dried CHAB plate (labeled 10~4).
• After pipetting the 6 spread plates for each dilution. Beginning with the 10"4 dilution, use
a sterile L-Shaped spreader to distribute the inoculum over the surface of the medium by
39
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Detection of Francisella tularensis in Environmental Samples
rotating the dish by hand or on a turntable. Ensure that inoculum is evenly distributed
over the entire surface of the plate. Use a different sterile spreader for each plate. Repeat
for the next three dilutions 10"3, 10"2 and 10"1, in that order.
• Allow inoculum to absorb into the medium completely.
10.4.4 Incubate and Enumerate Colonies
Invert the CHOC with IsoVitaleX and CHAB plates and incubate them at 35°C - 37°C
for a maximum of 7 days. Plates should be examined at 24-hour intervals for a maximum
of 7 days, if necessary.
• CHOC with IsoVitaleX Plates
a. F. tularensis produces gray-white, opaque colonies, usually too small to be seen as
individual colonies at 24 hours. After incubation for 48 hours or more, colonies are
approximately 1-2 mm in diameter, white to gray to bluish-gray, opaque, flat, with an
entire edge, smooth and have a shiny surface (Figure 2).
b. Count the number of F. tularensis colonies on each plate and record results.
• CHAB Plates
a. F. tularensis produces smooth, entire edge, greenish-white, and butyrous with
opalescent sheen colonies at 48 to 72 hours. Colonies are usually 2 to 4 mm after
incubation for 48 to 72 hours (Figure 2).
b. Count the number of F. tularensis colonies on each plate and record results.
• Plate Counts
a. If the number of colonies is < 250/plate, record actual number.
b. If the number of colonies is > 250/plate, record as "too numerous to count" (TNTC).
c. If no target colonies are observed, record as "None detected" and proceed to
evaluation of growth on MicroFunnel™ plates (10.4.5).
A minimum of 3 typical colonies should be confirmed using real-time PCR (Section
10.5).
10.4.5 Capture Cells on MicroFunnel™ Filter Membranes and Culture
• Place two, 0.45 (.un (pore-size) MicroFunnel™ filter funnels (Section 5.3.4) on the
vacuum manifold and moisten membrane with 5 mL PBS. All filtering should be done
with a vacuum pressure < 20 mm Hg.
• With the vacuum valve closed (and vacuum pressure released), place 10 mL of PBS into
each filter cup. Add 1.0 mL of the undiluted elution suspension (Section 10.4.2 [d]) to
each of two MicroFunnel™ cups.
• Open the vacuum valve and filter the suspension. Close the valve and release the vacuum
pressure. Rinse the walls of each MicroFunnel™ cup with 10 mL of PBS and filter. Open
the valve and complete filtration.
• Squeeze the walls of the MicroFunnel™ cup gently and separate the walls from the base
holding the filter. Discard cup in an autoclavable biohazard bag. Remove the
membranes with sterile forceps and place them grid-side up on labeled CHOC with
40
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Detection of Francisella tularensis in Environmental Samples
IsoVitaleX and CHAB plates. Ensure that the filter is in contact with the surface of the
agar. If an air pocket occurs under the filter, use the sterile forceps to lift the edge of the
filter to release the air pocket.
• Record the exact volume of the suspension filtered (1.0 mL) on each plate.
• Repeat steps (Section 10.4.5) described above for each sample.
• Invert and incubate CHOC with IsoVitaleX and CHAB plates at 35°C-37°C for a
maximum of 7 days. Plates should be examined daily for growth. Count the number of
colonies and record results.
• Plate Counts
a. If the number of colonies is < 80/plate, record actual number.
b. If the number of colonies is > 80/plate, record as "TNTC."
c. Ideally, plates with 20-80 colonies should be used to calculate the number of CFUs
per sample, as described in Section 12.2.2.
Confirm 1-3 colonies using real-time PCR (Section 10.5).
Note: For faster sample analysis results during the initial stages of an incident (e.g., incident
characterization) and during post-decontamination/clearance phase, it is
recommended that the remainder of all suspensions (e.g., undiluted, Iff1 and Iff2
dilutions) be filtered using an additional MicroFunnel™ and plated as described above
instead of proceeding with enrichment in TSB with IsoVitaleX. However, if a problem
of background microorganisms overgrowth on a filter is anticipated, the enrichment
culture would be required.
10.4.6 Enrich in TSB with IsoVitaleX
• Add the remainder of the undiluted suspension to the specimen cup containing the
corresponding sponge/wipe. Add 40 mL TSB with IsoVitaleX to the tube. Repeat for
each sample. Incubate the specimen cups at 35°C - 37°C. F. tularensis grows slowly;
the inoculated broth should be incubated and observed for at least 10 days.
• Observe the TSB with IsoVitaleX Enrichment
a. If broth is not cloudy, record as no growth (NG) and incubate for an additional 24
hours.
b. If broth is cloudy, record as positive growth (G+) and proceed to next step.
c. Cap the cup tightly and mix TSB with IsoVitaleX with positive growth for 30
seconds. Use a sterile loop to remove a loopful of broth with a 10 (.iL loop and streak
on a CHAB plate for isolation. Repeat two times for a total of three CHAB isolation
plates.
d. Incubate the CHAB isolation plates and TSB with IsoVitaleX with growth at 35°C -
37°C for a maximum of 10 days.
e. Examine plates for F. tularensis-suspect colonies. If any colonies are isolated,
proceed to PCR confirmation (Section 10.5).
f. If no suspect colonies are observed, perform PCR on TSB with IsoVitaleX with
growth according to Section 10.5.
41
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Detection of Francisella tularensis in Environmental Samples
10.5 Confirm F. tularensis Colonies by Real-time PCR Analysis
10.5.1 DNA Preparation from Cultured Cells
• Cells grown on solid culture medium
a. Pipet 100 |_iL of PCR-grade water into a 1.5 mL Eppendorf microcentrifuge tube
(Section 5.1.20).
b. Use a disposable 1 (.iL inoculating loop or pre-wetted swab to remove bacterial
growth from a typical F. tularensis colony grown on CHOC with IsoVitaleX or
CHAB plates.
Note: In some cases, it may be difficult to remove the bacterial growth with a loop. If this
happens, use a sterile applicator swab. Pre-wet the swab with PCR-grade water before
removing the bacterial growth.
c. Insert the loop or swab into the tube containing the PCR-grade water and immerse
the bacterial growth in the liquid.
d. Gently spin the loop or swab in the liquid to remove and resuspend the bacterial
growth in the water. Press the tip of the swab against the tube to remove the liquid
from the tip prior to discarding the swab or the loop in an autoclavable biohazard
bag. Proceed to Section 10.5.2.
• Cells grown in liquid culture medium
a. Transfer 50 |_iL of broth with growth to a microcentrifuge tube.
b. Place tube into a refrigerated microcentrifuge and spin at 12,000 x g for 2 minutes.
c. Remove and discard the supernatant in an autoclavable biohazard bag. Add 100 |_iL
of PCR grade water to the tube containing the bacterial pellet.
d. Resuspend the pellet by flicking the tube. Proceed to Section 10.5.2.
10.5.2 Preparation of Lysate
• Cap the microcentrifuge tubes containing the bacterial suspension with cap-holding tabs
to prevent the tubes from popping open during heating, and vortex mix for 3-5 sees.
• Place the capped tubes in a floating rack if using the water bath. Otherwise, place the
capped tube in the heat block at 95°C-98°C.
• Heat the sample for 20 minutes. Heating for 20 minutes will ensure all organisms are
killed; this allows the sample to be handled outside of the BSL3 laboratory.
• Remove the tubes from the water bath or heat block and place them directly in a cold
block (4°C). Chill for a minimum of two minutes.
• Remove the cap-holding tabs and place the microcentrifuge tubes in the refrigerated
microcentrifuge. Centrifuge at 12,000 rpm for two minutes.
10.5.3 Filtration of Lysate using a 0.1 Centrifugal Filter Device (Section 5.1.30)
Centrifugal filtration with 0.1 -|im Ultrafree®-MC filter devices (Section 5.1.30;
Millipore® Cat. No. UFC30VV00). following extraction of DNA will remove F.
42
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Detection of Francisella tularensis in Environmental Samples
tularensis cells that might contaminate DNA preparations, making the samples safe
without compromising the sensitivity of the real-time PCR assay (Reference 16.12).
• Remove top cap from the 0.1 |_im Ultrafree®-MC filter device (Section 5.1.30; Millipore®
Cat. No. UFC30VV00).
• Hold each filter device vertical with the filter cup opening facing up. Using a
micropipettor tip, transfer the supernatant from each microcentrifuge tube into the
corresponding 0.1 |_im Ultrafree®-MC filter device (Section 5.1.30; Millipore® Cat. No.
UFC30VV00). Do not allow the micropipettor tip to touch the filter membrane. Avoid
transferring any particulate matter that may be evident at the bottom of the tube. Close
the cap. Discard the microcentrifuge tube in an autoclavable biohazard bag.
• Place the Ultrafree®-MC filter devices into a centrifuge (Section 5.5.6; Eppendorf
5415R/5424R).
• Centrifuge at 8000 x g (approximately, 9200 rpm) for 2 minutes at 4°C.
Note: If the supernatant has not passed completely through the filter, centrifuge for an
additional two minutes. Repeat as necessary until all the supernatant has passed
through the filter.
• Carefully open the caps and remove the Ultrafree®-MC filter inserts (Section 5.1.30;
Millipore® Cat. No. UFC30VV00) using disposable forceps (gripping only the sides),
close the caps of the collection tubes and dispose of the Ultrafree®-MC inserts and the
forceps in an autoclavable biohazard bag.
• If there is concern regarding the biosafety of the filtered material, it is recommended that
the laboratory perform a sterility check on the filtered material according to internal
laboratory procedures.
• Wipe the outside of the tubes containing lysates with 10% pH amended bleach (Section
6.18) or bleach wipes (Section 5.1.3). Samples lysates are safe to remove from the BSL-
3 after filtration and disinfection of the tube.
• Using clean gloves, place the cold block (4°C) with the tubes containing the lysates in
DNA loading station/hood in preparation for PCR analyses (Section 9.7)
• If PCR analysis will not be completed the same day the lysates are prepared, aliquot
lysates and freeze them at -20°C.
Note: DNA extracted by this procedure should not be stored for more than lweek.
10.5.4 Use 5 |_iL of the lysate as the DNA template to run the PCR analysis in triplicate using the
Ftl and Ft2 assays.
Note: DNA obtained from cell lysates should be diluted (e.g., 1:10 or 1:100) prior to testing to
avoid excess DNA template, which can cause false negative results.
10.5.5 For real-time PCR, follow instructions provided in Sections 9.7.1-9.7.23 with the
following exceptions and changes:
• No PNC and EIC controls are required for the samples.
• For each batch of sample colonies, PCR Master Mix should be made for 4 PCs, 4 NTCs
and 3 replicates for DNA extracts per colony.
10.5.6 Refer to Sections 12.1 and 12.2.3 for Data Analyses and Calculations.
43
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Detection ofFrancisella tularensis in Environmental Samples
11.0 Rapid Viability-Polymerase Chain Reaction (RV-PCR) Method
Acceptable sample types: Drinking water and decontamination waste water
11.1 RV-PCR
The RV-PCR method (Figures 3 and 4) serves as an alternative to the traditional culture-based
methods for detection of viable pathogens. The RV-PCR method integrates high-throughput
sample processing, short-incubation broth culture, and highly sensitive and specific real-time
PCR assays to detect low concentrations of viable F. tularensis. This section includes a RV-PCR
method with appropriate sample processing procedures for detection of F. tularensis in water
samples.
The RV-PCR method not only generates rapid results, but also may provide a higher throughput
capability compared to the traditional culture-based methods, and hence, increases the laboratory
capacity for sample analysis. In place of multiple dilutions, plates, and enrichment culture per
sample used by the culture method, the RV-PCR method (16.5) uses a single well on a 48-well
plate per sample for /<'. tularensis (Figure 3).
• RV-PCR is based on DNA analyses before
(T0) and after (Tf) incubation of sample
• Algorithm for detection of viable
F. tularensis:
- A CT [CT (To) - CT (Tt)] > 6.0
• CT (Tf) value <39.0
• Ct(T0) value <45.0
(If no CT forT0, it is set to 45 to calculate A CT)
• A shift in PCR CT value indicates an increase
in DNA, which is itself due to an increase in
cell number
• The method accurately distinguishes live
cells from dead based on CT (T0), CT (Tf) and
ACX
Endpoint
response,
CT (T,)
500
0
1 400
o
M
| 300
"" 200
response,
Ct(T0)
30
PCR Cycle
Time 0
Figure 3. Example real-time PCR amplification curves for the initial To aliquot and the Tr(final)
endpoint aliquot.
The RV-PCR protocol steps and some of the equipment for F. tularensis are shown in Figure 3.
After mixing the water sample with growth medium, an aliquot is withdrawn for baseline (time 0)
analysis before incubating the broth culture in the 48-well plate at 37°C for 30 hours. This is the
44
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Detection ofFrancisella tularensis in Environmental Samples
To aliquot and is stored at 4°C for immediate processing or at -20°C for an extended period until
analysis. After the broth culture is incubated at 37°C for 30 hours or more, another aliquot is
withdrawn. This is the Tjo or Tf aliquot. Both the To and T30 or Tf aliquots are then processed to
extract and purify F. tularensis total DNA. The To and T30 or Tf DNA extracts are then analyzed,
in triplicate, using real-time PCR to detect the presence of F. tularensis DNA. The Ct values for
both the To and T30 or Tf DNA extracts are recorded and compared. A change in Ct for the Tse or
Tf aliquot relative to the Ct for the To aliquot is calculated as follows: ACt = (Ct [To] - Ct [Tjo or
Tf]). A ACt > 6 (i.e., the endpoint PCR Ct of < 39 for the Tjo or Tf DNA extract in a 45-cycle
PCR) is set as a cut-off value for a positive detection of viable F. tularensis in the sample. The
ACt > 6 criterion represents an approximate two log increase in DN A concentration at Tp or Tf
relative to To. The increase in DNA concentration at T30 or Tf is as a result of the presence of
viable F. tularensis bacteria in the sample that grew during the 30 or more hours of incubation in
growth medium. Incubation time could be extended to 36-48 hours to greatly eliminate the
possibility of a false negative result, especially for very dirty and/or post-decontamination
clearance samples. The current protocol provides qualitative (presence or absence) results.
As stated in Section 9, for a high-confidence identification of pathogens, PCR assays for multiple
pathogen-specific genes are usually used. Therefore, in this protocol, two single-plex PCR assays
(See Section 6.9, Ftl and Ft2) are included. However, for sample analysis during a confirmed
tularemia incident for which the F. tularensis strain has already been identified and characterized,
only the Type A (Ftl) or B (Ft2) specific real-time PCR assay targeting a strain-specific gene
may be performed.
Experimentally-
determined
endpoint of 30 hr
Water
Sample
Add 3 mL to
48-well plate
Mix; Take T0
aliquot for PCR
Incubate @ 37°C
30 hr
Mix; Take T30
aliquot for PCR
48 water samples
(~3 mL) can be processed per plate;
multiple plates can be processed for
throughput of 100s of samples
Add 6X growth
medium
Concentrated growth medium used
DNA extraction
& purification
T0 aliquot
PCR analysis
Automated or
manual
DNA extraction
Viable cells
present based on
ACt > 6
DNA extraction
& purification
T30 aliquot
PCR analysis
Figure 4. Flow Chart for RV-PCR Analysis of Francisella tularensis Cells from Water Samples.
45
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Detection of Francisella tularensis in Environmental Samples
11.2 RV-PCR: Sample Processing for Water Samples
Note: All subsequent procedures involving manipulation of water samples and membranes must be
carried out in a BSC using appropriate PPE). Sterile gloves should be used and changed
between samples and as indicated below. The CDC requires BSL-3 handling of this organism.
All wastes should be handled according to the CDC and the BMBL waste management and
disposal requirements.
11.2.1 Concentrate Water Sample by Centrifugation
Note: If the water sample has not been previously stabilized by buffer addition to maintain
cell viability, add 4.5 mL of 1 OX PBS to 40 mL water sample (final ~ IX PBS
concentration). If the sample volume is greater than 40 mL, adjust the PBS volume to
achieve a final concentration of ~1X PBS.
• Using a 50-mL serological pipet, transfer 40 mL of sample to a 50 mL screw cap
centrifuge tube. If the sample volume is greater than 40 mL, divide the final volume into
equal volumes and dispense into multiple tubes.
• Repeat the step above for each sample.
• Ensure tubes are balanced and place tubes into sealing centrifuge buckets. Decontaminate
centrifuge buckets with a 10% pH amended bleach solution (Section 6.18) or bleach
wipes (Section 5.1.3) before removing them from the BSC.
• Centrifuge tubes at 3500 / g. with the brake off, for 15 minutes in a swinging bucket
rotor.
• Remove the supernatant from each tube with a sterile 50 mL serological pipet and
discard, leaving approximately 3 mL in each tube (or 3 mL total if combining pellets
from multiple tubes per sample). The pellet may be easily disturbed and not visible, so
keep the pipet tip away from the tube bottom.
• Vortex mix the remaining 3 mL and the pellet.
• Remove suspension (or combined suspension) from one tube with a sterile 5 mL pipet
(recording the volume) and transfer to one well of the 48-well plate.
• Repeat for each sample.
11.2.2 Add Concentrated Growth Medium and Process for RV-PCR analysis
• Add 600 |_iL of 6X BVFH to each well of the 48-well plate using a 1000 |_iL pipettor.
(Final BVFH ~ IX). Mix the sample and growth medium well.
• Transfer 500 |_iL from each well of the 48-well plate to an appropriately labeled screw
cap tube. This is a To aliquot for each sample. Repeat for each sample.
• Store aliquots on ice or in cold block (4°C).
11.2.3 Seal and Incubate 48-well Plate
• Seal the 48-well plate with a sterile, breathable seal.
• Place in ziplock bag and seal bag.
• Incubate the 48-well plate at 37°C for 30 hours in a shaker incubator at 180 rpm.
46
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Detection of Francisella tularensis in Environmental Samples
Note: The incubation time could be extended to 36-48 hours to minimize the possibility of
false negative results due to dirty and/or post-decontamination clearance samples.
11.2.4 Process To Aliquots for DNA Extraction
• Centrifuge tubes at 14,000 rpm (20,800 relative centrifugal force [RCF]) for 10 minutes
at 4°C.
• Remove 300 |a,L of supernatant and dispose to waste. Store pellets on ice or in cold block
(4°C). Alternatively, the pellet may be stored at -20°C until it is ready to be processed for
DNA extraction.
11.2.5 Process T30 or Tf Aliquots for DNA Extraction
Note: For dirty and post-decontamination samples the incubation time could be extended to
36-48 hours.
• After 30-hour or longer incubation, transfer 500 |_iL from each well to an appropriately
labeled 2-mL screw cap tube. Ensure that the T30 aliquot for each sample is taken from
the same well from which the TO aliquot for the corresponding sample was taken. This is
a T30 or Tf aliquot for each sample.
• Centrifuge tubes at 14,000 rpm (20,800 RCF) for 10 minutes at 4°C.
• Remove 300 |a,L of supernatant and dispose to waste. Store pellets on ice or in cold block
(4°C). Alternatively, the pellet may be stored at -20°C until it is ready to be processed for
DNA extraction.
11.3 RV-PCR: Manual DNA Extraction/Purification Procedure Using the Promega MagneSil®
Kit Reagents
11.3.1 Thaw To and T30 or Tf aliquots if they were stored at -20°C.
11.3.2 Add 800 (.iL of Lysis Buffer (VWR, Cat. No. PAMD1392 or equivalent) using a 1000 (.iL
pipettor with a new tip for each sample. Cap the tubes and mix by vortexing on high
(-1800 rpm) for 30 seconds and place in 96-well tube rack at room temperature. Change
gloves as necessary between samples.
11.3.3 Vortex each screw cap tube briefly (low speed, 5-10 seconds) and transfer the sample
volume to a 2 mL Eppendorf tube (ensure the tubes are labeled correctly during transfer).
Change gloves in between each sample. Incubate the To and T30 lysate tubes hereafter
referred to as "To and T30 or Tf tubes" at room temperature for five minutes.
11.3.4 Vortex the paramagnetic particles (PMPs) on high (-1800 rpm) for 30-60 seconds, or
until they are uniformly resuspended. Keep PMPs in suspension by briefly vortexing
(3-5 seconds) before adding to each To and T30 or Tf lysate tube.
11.3.5 Uncap one tube at a time and add 600 (.iL of PMPs using a new tip for each sample, to
each To and T30 tubes (containing 1 mL sample-Lysis Buffer mix). Discard used tips in a
sharps container. Mix by vortexing for 3-5 seconds.
11.3.6 Repeat Section 11.3.5 for all To and T3oor Tf tubes, vortexing the PMPs suspension
between each To and T30 or Tf tube.
11.3.7 Vortex each To and T30 or Tf tube for 5-10 seconds (high), incubate at room temperature
for five minutes, briefly vortex, and then place on the DynaMag magnetic stand with
hinged-side of the tube facing toward the magnet. After all the tubes are in the stand,
47
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Detection of Francisella tularensis in Environmental Samples
invert tubes 180 degrees (upside-down) turning away from you, then right side-up, then
upside down toward you, then right side-up (caps up) position. This step allows all PMPs
to contact the magnet. Check to see if any beads are in the caps and if so, repeat the tube
inversion cycle again. Let the tubes sit for 5-10 seconds before opening. Maintain the
tube layout when transferring tubes between the magnetic stand and the 96-well tube
rack. Alternatively, tubes may be vortexed while in removable rack that interfaces with
magnetic stand.
11.3.8 Uncap each tube one at a time and withdraw all liquid using a 1000 |_iL pipettor with the
pipet tip placed in the bottom of 2 mL tube, taking care not to disturb the PMPs. Ensure
that all the liquid is removed. Use a new pipet tip to remove any residual liquid, if
necessary. If liquid remains in the tube cap, remove by pipetting. Dispose tip and liquid
in a sharps container. Recap tube. Change gloves as necessary.
Note: Section 11.3.8 can be combined with Section 11.3.9. After withdrawing the liquid in
Section 11.3.8, add 360 [iL of Lysis Buffer using a separate pipettor and a new tip.
11.3.9 Uncap each To and T30 or Tf tube one at a time and add 360 |_iL of Lysis Buffer using a
1000 |_iL pipettor. Use a new tip for each sample and discard used tips in a sharps
container. Cap and vortex on low setting for 5-10 seconds, then transfer to 96-well tube
rack.
11.3.10 After adding Lysis Buffer to all of the To and T30 or Tf tubes, vortex each tube for 5-10
seconds (low) and place back on the magnetic stand. After all tubes are in the stand,
follow tube inversion cycle, as described in Section 11.3.7.
11.3.11 Remove all the liquid as described in Section 11.3.8, except that a glove change between
samples is not required. Use a new tip for each To and T30 or Tf tube (discard used tips in
a sharps container). Recap the tube.
11.3.12 Repeat Sections 11.3.9-11.3.11 for all tubes.
Note: Section 11.3.11 can be combined with Section 11.3.13. After withdrawing the liquid in
Section 11.3.11, add 360 [iL of Salt Wash solution using a separate pipettor and new
tip. If the steps are combined, cap the tube after the Salt Wash addition.
11.3.13 1st Salt Wash: Uncap each To and T30 tube one at a time and add 360 uI * of Salt Wash
solution (Section 6.12). Use a new tip for each To and T30 or Tf tube and discard used tips
in a sharps container. Cap and transfer to 96-well tube rack.
11.3.14 After adding the Salt Wash solution to all of the To and T30 or Tf tubes, vortex each tube
for 5-10 seconds (low) and place on the magnetic stand. After all tubes are in the stand,
follow tube inversion cycle, as described in Section 11.3.7.
11.3.15 Remove liquid as described in Section 11.3.8, except that a glove change between To and
T30 tubes is not required. Use a new tip for each To and T30 or Tf tube and discard used
tips in a sharps container. Recap the tube. Repeat for all To and T30 or Tf tubes.
Note: Section 11.3.15 can be combined with Section 11.3.16. After withdrawing the liquid in
Section 11.3.15, add 360 [iL of Salt Wash solution using a separate pipettor and new
tip. If the steps are combined, cap the tube after the Salt Wash addition.
11.3.16 2nd Salt Wash: Repeat Sections 11.3.13-11.3.15 for all To and T30 or Tf tubes.
Note: Section 11.3.16 can be combined with Section 11.3.17. After withdrawing the liquid in
Section 11.3.16, add 500 [iL of Alcohol Wash buffer using a separate pipettor and new
48
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Detection of Francisella tularensis in Environmental Samples
tip. If the steps are combined, cap the tube after the Alcohol Wash addition.
11.3.17 1st Alcohol Wash: Uncap each To and T30 or Tf tube, one at a time, and add 500 |_iL of
Alcohol Wash (Section 6.12). Use a new tip for each sample and discard used tips in a
sharps container. Cap and transfer to 96-well tube rack.
11.3.18 After adding the Alcohol Wash (Section 6.12) to all of the To and T30 or Tf tubes, vortex
each tube for 5-10 seconds (low speed) and place on the magnetic stand. After all, To
and T30 or Tf tubes are in the stand, follow the tube inversion cycle, as described in
Section 11.3.7.
11.3.19 Remove liquid as described in Section 11.3.8, except that a glove change between To and
T30 or Tf tubes is not required. Use a new tip for each To and T30 or Tf tube and discard
used tips in a sharps container. Recap the tube.
Note: Section 11.3.19 can be combined with Section 11.3.20. After withdrawing the liquid in
Section 11.3.19, add 500 [iL of Alcohol Wash using a separate pipettor and new tip. If
the steps are combined, cap the tube after the Alcohol Wash addition.
11.3.20 2nd Alcohol Wash: Repeat Sections 11.3.17-11.3.19. After the liquid is removed, recap
the tube and transfer to the 96-well tube rack.
Note: Section 11.3.20 can be combined with Section 11.3.21. After withdrawing the liquid in
Section 11.3.20, add 500 [iL of Alcohol Wash using a separate pipettor and new tip. If
the steps are combined, cap the tube after the ethanol wash addition.
11.3.21 3rd Alcohol Wash: Repeat Sections 11.3.17-11.3.19 for all To and T30 or Tf tubes except
use 70% ethanol wash solution. After the liquid is removed, recap the tube and transfer
to the 96-well tube rack.
11.3.22 Open all To and T30 or Tf tubes and air dry for two minutes.
11.3.23 Heat the open To and T30 or Tf tubes in the heat block (placed in the BSC) at 80°C until
the PMPs are dry (-20 minutes). Allow all the alcohol solution to evaporate, since
alcohol may interfere with analysis.
11.3.24 DNA elution: While they are in the heating block add 200 |aL of Elution Buffer to each
To and T30 or Tf tube, and close tube.
11.3.25 Vortex for 10 seconds and let the tubes sit in the heating block for 80 seconds.
11.3.26 Briefly vortex the tubes (5-10 seconds), taking care to prevent the liquid from entering
the tube cap. Let the tube sit in the heating block for 1 minute.
11.3.27 Repeat Section 11.3.26 four more times.
11.3.28 Remove the tubes from the heating block, place them in a 96-tube rack in the BSC, and
let them sit at room temperature for at least five minutes.
11.3.29 Briefly vortex each tube (5-10 seconds) on low speed. Optional: Centrifuge at 2000 rpm
at 4°C for 1 minute. Place tube in 96-well tube rack.
11.3.30 Briefly vortex each tube (5-10 seconds) and place on the magnetic stand for at least 30
seconds. Bring the cold block (4°C) to the BSC.
11.3.31 Collect elution liquid from each To and T30 or Tf tube with a micropipettor and transfer to
a clean, labeled, 1.5 mL tube (-80-90 (iL) on a cold block at 4°C (check tube labels to
ensure the correct order). Use a new tip for each tube and discard tips in a sharps
49
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Detection of Francisella tularensis in Environmental Samples
container. Visually verify absence of PMP carryover during final transfer. If magnetic
bead carryover occurred, place the 1.5 mL tube on magnet, collect liquid, and transfer to
a clean, labeled, 1.5 mL tube (ensure the tubes are labeled correctly during transfer).
Centrifuge tubes at 14,000 rpm at 4°C for five minutes to pellet any particles remaining
with the eluted DNA; carefully remove supernatant and transfer to a new 1.5 mL tube
using a new tip for each tube (ensure the tubes are labeled correctly during transfer).
If analyses need to be conducted outside of a BSL-3, the DNA extract may be filtered
using a 0.1 [im Ultrafree ' -MCfilter insert, as described in Section 9.6.10.
Store To and T30 or Tf DNA extract tubes at 4°C until PCR analysis (use photo-tray to
transport 1.5 mL tubes in a rack).
If PCR cannot be performed within 24 hours, freeze DNA extracts at -20°C.
Laboratory cleanup procedures
Dispose of all biological materials in autoclavable biohazard bags (double bagged).
Autoclave all waste materials at the end of the work day.
Decontaminate counters and equipment with fresh 10% pH amended bleach (Section
6.18), followed by 70% isopropyl alcohol, and a deionized water final rinse.
11.4 RV-PCR: Automated DNA Extraction/Purification Procedure (Roche MagNA Pure
Compact kit)
11.4.1 When ready to proceed with inactivation, thaw pellet and heat lyse sample tubes by
incubating at 70°C ± 2°C for 10 min. Allow sample tubes to cool briefly (2-3 min).
11.4.2 Add 300 |iL lysis/binding buffer (MagNA Pure® LC Total Nucleic Acid Isolation Kit
Lysis/Binding Buffer-Refill; Roche, Cat. No. 03 246 779 001) to each sample tube and
close sample tube cap. Vortex on single tube vortexer for 5 sec at 1800-2000 rpm (VWR,
IKA Model MV1 or equivalent).
11.4.3 Add 300 |iL phosphate-buffered saline (PBS; IX PBS, Teknova, Cat. No. P0261) to each
PC Tube.
11.4.4 Vortex tubes for 10 sec on single tube vortexer at 1800-2000 rpm (VWR, IKA Model
MV1 or equivalent).
11.4.5 Incubate tubes for 30 min at room temperature (in BSC). Every 5 min invert tubes 5
times to mix.
11.4.6 Adapt the Reagent Cartridge to room temperature (15 to 25°C) before use. The kit may
not work well at temperatures outside the recommended range.
11.4.7 Use the MagNA Pure® Compact Nucleic Acid Isolation Kit I and select the
DNA_Blood_external_lysis purification protocol (supplied with the MagNA Pure®
Compact instrument). The sample and elution volumes must be chosen from the software
menu.
11.4.8 Samples will be lysed and filtered manually using 0.2-micron Ultrafree-MC filter units
(Millipore Cat. No. UFC30GV0S) following manufacturer's instructions, outside the
MagNA Pure® Compact instrument. Filtered lysates are then transferred to the instrument
and purification is carried out automatically. This procedure allows for physical
11.3.32
Note:
11.3.33
Note:
11.3.34
50
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Detection of Francisella tularensis in Environmental Samples
separation of the initial lysis/inactivation step(s) from the purification steps and enables
use of inactivated sample material on the MagNA Pure® Compact instrument (e.g., when
using potentially infectious sample material).
11.4.9 Turn on the instrument; ensure that the Tube Rack is seated correctly in the instrument.
11.4.10 Remove the Elution Tube Rack from the instrument.
11.4.11 Click the Run button on the Main Menu Screen to access Sample Ordering Screen 1.
11.4.12 Follow the software-guided workflow.
11.4.13 Remove a prefilled Reagent Cartridge from the blister pack. Handle each Reagent
Cartridge as follows:
• Always wear gloves when handling the cartridge.
• Hold the cartridge only at the barcode imprinted area and the opposite side.
• Avoid touching the sealing foil covering the cartridge wells.
• Avoid touching the two single open wells and do not use them as handles.
• Avoid any foam formation and let the fluid within the cartridge wells settle again
completely. If fluid remains under the sealing foil, knock the cartridge bottom gently on a
flat lab bench surface. This is especially important for well 1 which contains a small
volume of Proteinase K.
11.4.14 Check the cartridge integrity and filling volumes of the wells. Do not use cartridges that
have a different pattern of filling or that are damaged.
11.4.15 Scan the cartridge barcode using the barcode scanner supplied with the instrument.
11.4.16 With the two isolated wells pointing away from you, insert all the wells on the Reagent
Cartridge into the holes in the Cartridge Rack.
11.4.17 Use the guide slots on the rack to help position the cartridge.
11.4.18 Repeat the steps above for the desired numbers of samples (1 to 8).
11.4.19 Proceed to Sample Ordering Screen 2.
11.4.20 Select the appropriate purification protocol from the Protocol menu
(DNA_Blood_external_lysis).
11.4.21 Select the elution volume (100 |iL).
11.4.22 Optional: Select the Internal Control Volume (0 |iL).
11.4.23 Insert the appropriate number of Tip Trays (one per sample) into the assigned position in
the instrument Tip Rack.
11.4.24 Check if the Tip Tray holds a disposable tip or piercing tool in each position. Do not use
tip trays that are not assembled accordingly.
11.4.25 Handle Tip Trays with care to prevent tips or piercing tool from falling out of the tray.
Should this happen, discard the respective tip tray and tips. Use the Tip Tray Kit to
replace missing Tip Trays.
11.4.26 Proceed to Sample Ordering Screen 3.
11.4.27 Scan the sample barcode from the primary sample tube or enter the sample ID.
51
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Detection of Francisella tularensis in Environmental Samples
11.4.28 One at a time, uncap and arrange the Sample Tubes in row 1 of the Tube Rack. Make
sure, the brim of the tubes seats solidly on the rack. Discard caps to waste.
11.4.29 Scan the bar codes of the Elution Tubes.
11.4.30 Place the Elution Tubes into the Elution Tube Rack. Ensure the brim of the tubes seats
solidly on the rack.
11.4.31 On the Confirmation Screen, check the information display.
11.4.32 If the information is correct, confirm it by touching the "Confirm Data" button, close the
front cover, and start the run.
11.4.33 After the purification run has ended, the Result Screen appears showing the result of the
isolation process for each channel.
11.4.34 The result will be PASS if the isolation run was completed without any warning or error.
11.4.35 The result will be FAIL if any interruption of the process or error occurred during the
run. For each FAIL result, the result screen will show a brief error or warning messages
to help you decide whether the error or warning can be ignored. Refer to the
troubleshooting section of the MagNA Pure® Compact Operator's Manual.
11.4.36 Close the Elution Tubes with the supplied tube caps and remove the Elution Tube Rack
or the Elution Tubes immediately after the end of the purification run.
11.4.37 If not proceeding directly to your downstream application, store DNA eluates at -20°C.
DNA is stable for at least 6 to 12 months if stored properly.
11.4.38 Optional: Start the automated liquid waste discard.
11.4.39 Always empty the MagNA Pure® Compact Waste Tank after every purification run.
11.4.40 Treat liquid waste as potentially infectious (depending on sample material), and
hazardous, since lysis buffers are present (see Safety Information in instrument manual
and/or SDS for the lysis buffer).
11.4.41 Store DNA extract tubes "referred to as TO or T30 DNA extracts" at 4°C until PCR
analysis (use photo-tray to transport 1.5 mL tubes in a rack).
Note: If PCR cannot be performed within 24 hours, freeze DNA extracts at -20°C.
11.5 RV-PCR: Real-time PCR Analysis of To and T30 or Tf DNA Extracts
Note: PCR Master Mix for 6 reactions per sample is required to accommodate the To and T30 or Tf
DNA extracts. For each batch of samples, PCR Master Mix should be made for 4 PCs, 4 NTCs,
3 PNCs and 6 DNA extracts per sample (3 for To and 3 for T30 or Tf DNA extracts). No EIC
control is required for the samples.
11.5.1 Prepare PCR Mix according to the Table 6.
11.5.2 Set up 96-well PCR plate with PCR mix according to plate layout in PCR-preparation
hood, seal, and transfer to BSC.
11.5.3 Analyze To and T30 or Tf DNA extracts on same PCR plate.
11.5.4 If DNA extracts were frozen, transfer them to BSC and let them thaw to room
temperature.
52
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Detection of Francisella tularensis in Environmental Samples
11.5.5 Perform 1:10 dilution of DNA extracts. Alternatively, only run samples undiluted (5 |_iL
plus 20 |_iL PCR Master Mix).
11.5.6 Add 90 (iL of PCR-grade water to wells of a sterile 96-well plate. Note: 10-fold dilutions
may also be made in screw cap tubes or 1.5 mL Eppendorf tubes.
11.5.7 Mix DNA extracts by vortexing (5 seconds at low speed) and transfer 10 (.iL to the plate
wells, following the plate layout.
11.5.8 Mix diluted DNA extracts by vortexing (5 seconds at low speed) and transfer 5 (.iL from
each plate well or tube to the PCR plate (with PCR Mix). Seal PCR plate with optical
seal using a clear Edge Seal.
11.5.9 Centrifuge sealed PCR plate for 1 minute at 2000 rpm.
11.5.10 Open the centrifuge safety cup in BSC, place plate on photo-tray, change gloves, transfer
PCR plate to ABI® thermocycler.
11.5.11 The PCR cycling conditions on the ABI® 7500 Fast are provided in Table 7.
Fluorescence is automatically measured at the end of the 60°C annealing-extension
combined step.
11.5.12 After cycle completion, discard sealed PCR plate to waste and autoclave. PCR plates
with amplified product are never to be opened in the laboratory.
11.5.13 Follow laboratory cleanup procedure (11.3.34).
11.5.14 10.5.6 Refer to Sections 12.3 for Data Analyses and Calculations.
Table 6. Master Mix for Ftl and Ft2 Francisella tularensis PCR Assays
Reagent
Volume
(ill.)
Final Concentration
l aq Man 2\ lni\ ersal Masler Mix
12.5
IX
Platinum® Taq DNA Polymerase
0.25
1.25 U
Forward primer, 10 |iM
0.5
0.20 viM
Reverse primer, 10 |iM
0.5
0.20 uM
Probe, 4 |iM
0.4
0.064 [iM
Molecular Biology grade water
5.85
N/A
Template DNA
5
Variable
TOTAL
25
Table 7. PCR1
"hernial Cycling Conditions a'b
Slops
i \c;*
1 iicii l>;i lion
Ampli 1 :i(| (.old
Acli\;ilion
Hold
Hold
Dciiiilui'iilioii
.\nnc;iling/l'.\lcnsion
Temperature
50°C
95°C
95°C
60°C
Time
2 minutes
10 minutes
5 seconds
20 seconds6
a Run Mode: Fast 7500
b Reaction volume 25 |iL
0 Uracil-DNA glycosylase
d Fast Ramp: 3.5°C/s up and 3.5°C/s down
e 30 seconds for ABI® 7500 Fast Dx instrument
53
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Detection ofFrancisella tularensis in Environmental Samples
12.0 Data Analysis and Calculations
12.1 Real-time PCR Analysis
Calculate the average Ct from the replicate reactions for each sample DNA extract, PC and the
EIC, where applicable. Most instruments will perform this calculation for the user, but an
equation is provided below should manual calculation be needed.
Sy=iCT(y)
= Average CT,
N
where N is the number of replicate reactions
Example:
Where 3 replicate reactions produce CT values of 20,25, and 24,
£y=i CT(l)+CT(2)+CT(3) £20+25+24 67 . _
— = • = — = 23 Average CT
Tlie average Ct < 40 and the presence of a logarithmic curve in the real-time graph for the sample
DNA extract indicates a positive result suggesting the presence of F. tularensis in the sample. A
minimum of two out of three replicates must show Ct < 40 for a sample result to be considered
positive. If only one out of three PCR replicates for any sample DNA extract gives Ct < 40, the
PCR analysis of the DNA extract for that sample must be repeated.
Amplification Plot
BA Assay 2: Sensitivity of Detection
l§4.800 E+3
¦4
DNA
- 10 pg
¦ 1 Pg
- 100 fg
- 20 fg
" 10 fg
¦NTC
Detector: |B A *" ] Plot:JnRri vs '"ycle ^ Threshold:] 199.1 7773
Figure 5. Example logarithmic curve for Fluorogenic PCR for Bacillus anthracis.
If the EIC for a sample results in a Ct value (> 3) compared to the Ct value for the positive
control, there may be matrix inhibition. If the corresponding sample is negative (Ct > 40) for
F. tularensis, the sample DNA extract should be diluted 1:4 and 1:10 and the PCR assay should
be repeated for that sample along with the EIC with diluted sample DNA extracts. Negative
54
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Detection of Francisella tularensis in Environmental Samples
controls should not yield any measurable Ct values; if Ct values are obtained, check for potential
cross-contamination and repeat analysis. In addition, field blank samples should not yield any
measurable Ct values. If Ct values are obtained as a result of a possible contamination or cross-
contamination, depending upon the Ct value, a careful interpretation of the Ct values for the
sample DNA extracts must be done for the final result or the PCR analyses must be repeated.
12.2 Culture Analysis
12.2.1 Serial Dilution Plating
Count the number of typical colonies (Figure 2) on replicate culture plates and calculate
the average number of colonies per plate. Apply the following guidelines (a-e) when
counting the colonies and report results based on the number of characteristic F.
tularensis colonies.
Media sterility checks should not exhibit growth. Growth should also not be present on
CHOC/CHAB plates from field blank samples. If growth is observed on plates, colony
morphology should be evaluated to determine if contamination is due to the target
organism and potential source of contamination. Depending on the situation, results
should be qualified if QC plates are contaminated with F. tularensis.
a. If the number of colonies is < 250/plate, record actual number.
b. If the number of colonies is > 250/plate, record as "TNTC."
c. Ideally, plates with 25-250 colonies should be used to calculate the number of colony
forming units (CFU) per sample as described below.
d. If there are no plates with 25-250 colonies, choose the plates with the counts closest
to the acceptable range of 25-250 colonies. For example, if all plate counts are
greater than 250 choose the plates that have counts closest to 250. Likewise, if all of
the plate counts are less than 25, the plates with counts closet to 25 would be used to
calculate the number of CFUs per sample.
e. If no target colonies are observed, record as "None detected."
To determine the number of CFUs per sample, average the number of colonies in the
dilution series that produced <250 cells/plate. In this case assume the colony counts
were 210, 193, and 200 for the 10"1 dilution series and 25, 19, and 26 for the 10~2. Divide
the total number of colonies on plates with 25-250 colonies by the total volume plated to
obtain the number of colonies in 1 mL, and then multiply by the total suspension volume
(in this example, 5mL), as in the following equation:
Xy=i CFU (/)
TJJ=i Volume (/)
x Total Suspension Volume = CFUs per sample,
where N is the number of plates for which the CFU Count is between 25 and 250
Example:
210 + 193 + 200 + 25 + 26
AO.1 + 0.1 + 0.1 + 0.01 + 0.01
x 5
= 10,220 CFUs per sample
55
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Detection of Francisella tularensis in Environmental Samples
12.2.2 MicroFunnel™ Filter Plating
Count the number of typical colonies (Figure 2) on each filter and record. Apply the
following (a-c) when counting the colonies and report results based on the number of
characteristic F. tularensis colonies.
Media sterility checks should not exhibit growth. Growth should also not be present on
CHOC/CHAB plates from field blank samples. If growth is observed on filters, colony
morphology should be evaluated to determine if contamination is due to the target
organism and potential source of contamination. Depending on the situation, results
should be qualified if QC plates are contaminated with F. tularensis.
a. If the number of colonies is < 80/plate, record actual number.
b. If the number of colonies is > 80/plate, record as "TNTC."
c. Ideally, plates with 20-80 colonies should be used to calculate the number of CFUs
per sample, as described below.
d. If there are no plates with 20-80 colonies, choose the plates with the counts closest to
the acceptable range of 20-80 colonies. For example, if all plate counts are greater
than 80 choose the plates that have counts closest to 80. Likewise, if all of the plate
counts are less than 20, the plates with counts closet to 20 would be used to calculate
the number of CFUs per sample.
e. If no target colonies are observed, record as "None detected".
To determine the number of CFUs per sample, average the number of colonies on the
duplicate filters which produced 20-80 colonies/plate. In this case assume the colony
counts were 57 colonies/filter and 63 colonies/filter on the 2 respective filters. Since
each filter received 1.0 mL of the suspension, then the average colony count for the filters
would then be 60 colonies/mL. Multiply by the average colony count per mL by the total
suspension volume per sample, as in the following equation:
60 x 5 —^— = 300 CFUs per sample
mL sample
12.2.3 Enrichment in TSB with IsoVitaleX
Evaluate post-enrichment streaked CHOC/CHAB plates for the presence of F. tularensis
colonies (Figure 2). If no suspect colonies are observed, broth should be evaluated for the
presence of F. tularensis. Typical isolates or TSB with IsoVitaleX with growth must be
confirmed using real-time PCR prior to reporting results. Since the sample was enriched,
only qualitative (presence/absence) results can be reported.
Media sterility checks should not exhibit growth. Growth should also not be present in
TSB with IsoVitaleX from field blank samples. If growth is observed on plates, colony
morphology should be evaluated to determine if contamination is due to the target
organism and the potential source of contamination. Depending on the situation, results
should be qualified if QC samples are contaminated with F. tularensis.
12.2.4 Confirmation of Colonies by Real-time PCR
Presence of F. tularensis typical colonies on the culture plate indicates the presence of
56
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Detection of Francisella tularensis in Environmental Samples
viable F. tularensis cells in the sample. A minimum of three typical colonies should be
confirmed using real-time PCR and the either the Ftl (For F. tularensis Type A strain) or
Ft2 (For F. tularensis Type B strain) real-time PCR assay depending upon the type strain
identified to be involved in an incident. Optionally, both Ftl and Ft2 PCR assays can be
used. The Ct < 40 and the presence of a logarithmic curve in the real time graph (Figure
5) for the sample indicates a positive result suggesting the presence of F. tularensis in the
respective sample. Report the results based on the number of confirmed colonies.
Negative controls should not yield any measurable Ct values above the background level.
If Ct values are obtained as a result of a possible contamination or cross-contamination,
prepare fresh PCR Master Mix and repeat the analysis.
12.3 RV-PCR Analysis
Calculate an average Ct from the replicate reactions for To and T30 or Tf DNA extracts of each
sample. Subtract the average Ct of the T30 or Tf DNA extract from the average Ct of the To DNA
extract. If there is no Ct for the To DNA extract (i.e., the To is non-detect), use 45 (total number
of PCR cycles used) as the Ct to calculate the ACt for the sample. The change (decrease) in the
average Ct value from To to T30 or Tf (ACt) > 6 indicates a positive result suggesting the presence
of viable F. tularensis cell in the sample. A ACt criterion of > 6 (an approximate two log
difference in DNA concentration) and a corresponding T30 or Tf Ct of < 39, was set. If an
incubation time longer than 30 hours was used for the RV-PCR, instead of T30, appropriate Tf
(incubation time) should be used (i.e., 36-40 hours for post-decontamination, field samples with
high concentrations of dead F. tularensis cells). However, (ACt) > 6 algorithm should still be
used for a positive result. A minimum of two out of three To PCR replicates must result in Ct
values < 44 (in a 45-cycle PCR) to calculate the average To Ct. A minimum of two out of three
T30 or Tf PCR replicates must result in Ct values < 39 to calculate the average Ct for a sample
result to be considered positive. Negative controls (No Template Controls, NTCs) should not
yield any measurable Ct values above the background level. If Ct values are obtained as a result
of a possible contamination or cross-contamination, prepare fresh PCR Master Mix and repeat
analysis. In addition, field blank samples should not yield any measurable Ct values. If Ct
values are observed as a result of a possible contamination or cross-contamination, a careful
interpretation of the Ct values for the sample DNA extracts and field blanks must be done to
determine if the data is considered valid or if the PCR analyses must be repeated.
13.0 Method Performance
To be completed upon protocol verification and/or validation.
14.0 Pollution Prevention
14.1 The solutions and reagents used in this method pose little threat to the environment when
recycled and managed properly.
14.2 Solutions and reagents should be prepared in volumes consistent with laboratory use to minimize
the volume of expired materials to be discarded in an autoclavable biohazard bag. If there is any
57
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Detection of Francisella tularensis in Environmental Samples
possibility of the materials having been contaminated, they must be disposed of according to
CDC BSL-3 procedure (in an autoclavable biohazard container).
15.0 Waste Management
15.1 It is the laboratory's responsibility to comply with all federal, state and local regulations
governing waste management, especially the biohazard and hazardous waste rules and land
disposal restrictions. Following these regulations protects the air, water and land by minimizing
and controlling all releases from fume hoods and bench operations. Compliance with all sewage
discharge permits and regulations is also required.
15.2 Samples, reference materials and equipment known or suspected to be contaminated with or to
contain viable F. tularensis must be decontaminated prior to disposal.
15.3 Large volume water filtrates should be decontaminated using bleach (10% final concentration) for
a minimum of 30 minutes prior to disposing to the sanitary sewer (e.g., pouring down the drain).
15.4 For further information on waste management, consult The Waste Management Manual for
Laboratory Personnel (Reference 16.13) and Less Is Better: Laboratory Chemical Management
for Waste Reduction (Reference 16.14), both authored by the American Chemical Society.
16.0 References
16.1 McClendon MK, Apicella MA, and Allen LA. 2006. Francisella tularensis: Taxonomy, genetics,
and immunopathogenesis of a potential agent of biowarfare. Annu Rev Microbiol. 60:167-185.
16.2 Dennis DT, Inglesby TV, Henderson DA, Bartlett JG, Ascher MS, Eitzen E, Fine AD,
Friedlander AM, Hauer J, Layton M, Lillibridge SR, McDade JE, Osterholm MT, O'Toole T,
Parker G, Perl TM, Russell PK, and Tonat K. 2001. Tularemia as a biological weapon: medical
and public health management. JAMA. 285(21): 2763-2773.
16.3 Christopher LGW, Cieslak TJ, Pavlin JA, and Eitzen EM. 1997. Biological warfare: A historical
perspective. JAMA. 278(5): 412-417.
16.4 Sinclair R, Boone SA, Greenberg D, Keim P, and Gerba CP. 2008. Persistence of Category A
Select Agents in the environment. Appl Environ Microbiol. 74(3): 555-563.
16.5 Kane SR, Shah SR, and Alfaro TM. 2019. Rapid viability polymerase chain reaction method for
detection of Francisella tularensis. J Microbiol Methods. 166: 105738.
16.6 ASM (American Society for Microbiology). 2016. Sentinel level clinical laboratory guidelines
for suspected agents ofbioterrorism and emerging infectious diseases - Francisella tularensis.
Washington, DC: American Society for Microbiology.
https://www.asm.org/ASM/media/Policv-and-Advocacv/LRN/Sentinel%20Files/tularemia.pdf
[Last Accessed September 17, 2019]
16.7 U.S. Department of Health and Human Services, Centers for Disease Control and Prevention and
National Institutes of Health. 2009. Biosafety in Microbiological and Biomedical Laboratories
(BMBL), 5th Edition. Atlanta, Georgia: The Centers for Disease Control and Prevention.
http://www.cdc.gov/biosafetv/publications/bmbl5/index.htm [Last Accessed September 17, 2019]
58
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Detection of Francisella tularensis in Environmental Samples
16.8 American Chemical Society (ACS). 2006. Reagent Chemicals: Specifications and Procedures,
10th Edition. New York: Oxford University Press (USA).
16.9 Bucknell DJ, AnalaR Standards Ltd. 1984. AnalaR Standards for Laboratory Chemicals. 8th
Edition. Poole, Dorset, U.K.: BDH Ltd.
16.10 United States Pharmacopeia. 2005. United States Pharmacopeia and National Formulary 24.
Rockville, MD: United States Pharmacopeial Convention.
16.11 Kugeler KJ, Pappert R, Zhou Y, and Petersen JM. 2006. Real-time PCR for Francisella
tularensis Types A and B. Emerg Infect Dis. 12(11): 1799-1801.
16.12 Dauphin LA, and Bowen MD. 2009. A simple method for the rapid removal of Bacillus anthracis
spores from DNA preparations. J Microbiol Methods. 76(2009): 212-214.
16.13 American Chemical Society (ACS) 1990. The Waste Management Manual for Laboratory
Personnel. Washington, DC: American Chemical Society Department of Government Relations
and Science Policy.
16.14 Fermor PL. 2002. Less Is Better: Laboratory Chemical Management for Waste Reduction.
Washington, DC: American Chemical Society Taskforce on RCRA (Resource Conservation and
Recovery Act of 1976). http://goo.gl/2vlHPr [Last Accessed September 17, 2019]
59
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Detection of Francisella tularensis in Environmental Samples
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vvEPA
United States
Environmental Protection
Agency
PRESORTED STANDARD
POSTAGE & FEES PAID
EPA
PERMIT NO. G-35
Office of Research and Development (8101R)
Washington, DC 20460
Official Business
Penalty for Private Use
$300
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