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Part 2
Performing drug susceptibility testing
on solid media
Module 10
11
Learning objectives
At the end of this module you will be able to:explain the different methods for
performing DST;perform and interpret the proportion
method; record and report DST results;store strains.
22
Content outline
• Drug susceptibility test methods:– direct– Indirect
• Proportion method: technical protocol and interpretation criteria
• Recording and reporting DST results• Storage of strains
33
Direct drug susceptibility method:proportion method
• Sputa with smear grading of 2+ or more can be used as pure cultures after decontamination using standard procedure.
• The neutralized suspension is used for inoculation directly onto drug-containing and drug-free media, according to the proportion method (see below).
• Inoculum size is adjusted according to the number of AFB observed during smear microscopy of concentrated sputum.
• Identification should be performed before results are released.
44
Example of a susceptibility test, proportion method, inoculated directly after decontamination from the sample
(4 AFB/field)
Courtesy of Dr Isabel N. de Kantor, Buenos Aires, Courtesy of Dr Isabel N. de Kantor, Buenos Aires, Argentina55
Direct drug susceptibility method: advantages
• Bacillary populations more representative of those existing in vivo.
• Takes 3–4 weeks less than indirect testing.
66
Direct drug susceptibilitymethod: disadvantages
• Only for highly positive smear.• NOT possible in liquid culture.• High contamination rate.• Difficult to calibrate (live + dead bacilli).• Failure rate: 10–15%
77
Indirect drug susceptibility methods
• Organisms isolated in culture.
• A homogeneous suspension of growth is inoculated onto control and drug-containing egg-based solid media.
88
Indirect drug susceptibility methods
99
Indirect drug susceptibility method:proportion method
• The proportion method is the most widely used method for DST and is currently used as a reference for testing new methods.
• The proportion method determines the percentage of growth (number of colonies) of a defined inoculum on a drug-free control medium vs. growth on culture media containing the critical concentration of an anti-TB drug.
• The critical drug concentration, as well as the critical proportion of resistant colonies, has been evaluated from clinical data.
1010
Indirect proportion method
• A pure culture of tubercle bacilli (test strain) in the active phase of growth (2–4 weeks). In the absence of sufficient growth (<20 colonies, 1+), DST should not be performed unless the culture comes from a patient who has completed anti-TB treatment. From cultures with scarce growth, the bacillary population used for performing DST may not be representative of those existing in vivo.
1111
Proportion method: critical parameters
Use of LJ medium and a critical proportion of 1% of growth for all 4 drugs
Critical drug concentrationDrug Critical conc. (μg/ml) Critical %
Streptomycin 4 1
Isoniazid 0.2 1
Rifampicin 40 1
Ethambutol 2 1
1212
TOUCH ALL COLONIES!
Procedure
5 ml Sterile distilled
water
BEADS
VortexMedia should be from the same batch
Sediment for 15 min and transfer the supernatant to another tube
1313
Calibration of the bacterial suspension
Calibrate the inoculum to 1 MacFarland by comparing with standard 1 MacFarland suspension on a dark background.
Clumps and beads
SN1 MacFarland suspension
1414
Inoculation
• Loop (10 μl, diameter 3 mm)
• Calibrated pipettes
1515
Procedure – inoculum with loop
0.01 ml
2 ml distilled
water
twice
10–2
GC
S
I
R
E
GC
S
I
R
E1616
BEADS
+ inoculum of 2 GC with suspension 10–4
MacFarland 1
Procedure – inoculum with loop ../..
2 ml distilled
water
10–1
GC
S
I
R
E
GC
S
I
R
E
2 ml distilled
water
10–3
1717+ inoculum of 2 GC with suspension 10–5
twice
Procedure – inoculum with pipette
4.5 ml distilled
water
10–1
0.5 ml
4.5 ml distilled
water
10–2
4.5 ml distilled
water
10–3
0.5 ml 0.5 ml
1818
BEADS
10–4 10–5
0.5 ml 0.5 ml 0.5 ml
4.5 ml distilled
water
4.5 ml distilled
water
4.5 ml distilled
water
4.5 ml distilled
water
4.5 ml distilled
water
4.5 ml distilled
water
4.5 ml distilled
water
4.5 ml distilled
water
4.5 ml distilled
water
10–6
0.5 ml
10–3
GC
S
I
R
E
GC
S
I
R
E
0.1 ml
1919
0.1 ml
GC GC
10–5
Inoculum with pipette
10–4
GC
S
I
R
E
GC
S
I
R
E
0.1 ml
2020
0.1 ml
GC GC
10–6
Inoculum with pipette ../
Incubation
• Incubate at 35–37 ºC in slanted position, loose caps.
• At 48 hours: • tighten caps• check for contaminants• move to upright position
2121
Reading results• Read after 4 weeks as a provisional result and after 6 weeks for the
definitive interpretation of result. • The growth on GC tube 1/100 should allow easy counting of 30–100
colonies.• If fewer than 20 colonies have grown on this control, report only if resistant
(repeat if susceptible).
• A strain is resistant if the medium containing the critical concentration of the corresponding drug shows more colonies than the GC with the 1% inoculum .
• “Borderline cases” (about 1% growth on drug-containing medium) should be reported as resistant and retested.
• If the criteria described above are met and quality control of the batch meets the standards, the result is interpreted and reported as “susceptible” or “resistant” using the report form sheet.
2222
Growth on control tubes (>20 colonies on GC) and no growth on drug tubes
Interpretation
SENSITIVE TO ALL DRUGS2323
Growth on control tubes (>20 colonies)
and number of colonies on isoniazid tube
≥ number of colonies on control tube 1/100
Interpretation
RESISTANT TO ISONIAZID
2424
Growth on control tubes (>20 colonies) and number of colonies on isoniazid tube < number of colonies on control tube 1/100
Interpretation
SENSITIVE TO ISONIAZID
2525
Growth on control tubes (>20 colonies) and number of colonies on rifampicin tube ≥ number of colonies on control tube 1/100
Interpretation
RESISTANT TO RIFAMPICIN
2626
Growth on control tubes (>20 colonies) and number of colonies on rifampicin tube < number of colonies on control tube 1/100
Interpretation
SENSITIVE TO RIFAMPICIN
2727
Growth on control tubes (>20 colonies) and number of colonies on streptomycin tube ≥ number of colonies on control tube 1/100
Interpretation
RESISTANT TO STREPTOMYCIN
2828
Growth on control tubes (>20 colonies) and number of colonies on streptomycin tube < number of colonies on control tube 1/100
Interpretation
SENSITIVE TO STREPTOMYCIN
2929
Growth on control tubes (>20 colonies) and number of colonies on ethambutol tube ≥ number of colonies on control tube 1/100
Interpretation
RESISTANT TO ETHAMBUTOL
3030
Growth on control tubes (>20 colonies) and number of colonies on iethambutol tube < number of colonies on control tube 1/100
Interpretation
SENSITIVE TO ETHAMBUTOL
3131
Growth on control tubes (>20 colonies) and number of colonies on isoniazid tube and on rifampicin≥ number of colonies on control tube 1/100
Interpretation
MULTIDRUG-RESISTANT (MDR)
3232
No growth on control tubes (or <20 colonies on GC) and no growth on
drug tubes
Interpretation
INVALID RESULT – REPEAT
3333
Proportion method ‒ advantages and disadvantages
Advantages: • Standardization of
the size inoculum is not critical
• Simple
Disadvantages:• Influenced by degree
of dispersion of the inoculum suspension
3434
Possible errors• Related to drug concentrations and stability:
– preparation of drug solutions and drug-containing media;– excessive or prolonged heat during inspissation – steaming of media;– improper storage of drug solutions and drug-containing media.
Related to media quality:– excessive moisture on the surface of the medium;– excessive dehydration of the medium.
Related to the inoculum:– use of an inoculum not representative of the bacterial population;– use of too little inoculum;– presence of large aggregates of bacteria.
Related to NTM contamination:– failure to recognize the simultaneous presence of MTB complex and
other mycobacteria. Use only pure M. tuberculosis cultures.3535
Quality assurance issues
• Every new batch of drug-containing media prepared for DST must be quality-controlled.
• For each drug, a slant of the critical concentration and media with lower drug concentrations are tested with H37Rv strain.
• Compare results with the MIC of H37Rv.• External quality control should be organized and
supervised annually by the national research laboratory, using a panel of 20 test strains provided by the SRL network.
3636
Recording and reporting form
3737
Request and reporting form for TB culture and Drug Susceptibility Test (DST)
Patient identification (ID):
TB register number:____________ Previous TB register number:____________ MDR register number:_____________
Surname and first name of patient:________________________________ Age (yrs):_____ Sex:____
Ward / Department: __________________ Address: _________________________________
*HIV-status: Pos / Neg / Unknown _________________________________ TB Disease type and treatment history Site: pulmonary History: new (never treated before for ?1 month) extrapulmonary (specify):_______________ relapse failure Previous treatment: Cat.1 return after default Cat.2 chronic excretor Cat.4 (second-line drugs) MDR contact Other _________________ uncertain Origin of request:
Region ID:_______________ District ID:_______________ Local laboratory ID:________________
Date specimen was collected: ____/____/20____ Specimen ID number:_______________
Local laboratory: smear result: 1st ____ 2nd ____ 3rd ____ specimen microscopy technique used: hot Ziehl-Neelsen direct smear cold staining concentrated smear fluorescence
Request for testing at the reference laboratory: Reason: diagnosis Specimen: sputum follow-up at …. months during treatment sputum in preservative, type …………… follow-up at …. months after treatment other specify):__________________
Requested tests: microscopy (type _______ ) culture DST (first / second line)
Person requesting examination: Name:_________________________ Position:________________
* Information that can be disclosed optionally ID = identification number or code
Date: _____/______/20_____ Signature:________________
Iso
nia
zid
-2
Iso
nia
zid
-4
Rif
am
pic
in-2
Rif
am
pic
in-4
Str
ep
tom
yc
in-2
Str
ep
tom
yc
in-4
Eth
am
bu
tol-
2
Eth
am
bu
tol-
4
1 week
4 weeks
6 weeks
1 week
4 weeks
6 weeks
ID t
es
t 2
**
Ide
nti
fic
ati
on
ID t
es
t 3
**
Re
sis
tan
ce
pro
file
Quantified results of growth / reactions
Drug concentrations in µg/ml*
Co
ntr
ol
-4
Co
ntr
ol
-2
Re
ad
ing
tim
e
PN
B
ID t
es
t 1
**
Final results
Da
te r
ep
ort
ed
ID # ____________ Legend: S = susceptible; R = resistant; C = contaminated; ND = not done
INH Rifampicin Ethambutol Streptomycin Pyrazinamide Ofloxacin Kanamycin
µg/ml
result
Date: _____/______/20_____ Signature:________________
Storage of strains
• As part of good laboratory practice, cultures should be stored in appropriate conditions:– to preserve viability;– for safety reasons.
• Viability will decline over time if bacteria are stored at room temperature or at 4 ºC. (Check national policy on strain storage.)
3838
Storage of strains
• Short-term storage:– 4 ºC (1 year solid)– 20 ºC (2 weeks)– liquid cultures – no more than 1 month.
Long-term storage of patient cultures:– –20 ºC.
Long-term storage of reference cultures:– –20 ºC.
3939
Storage of strains
• Liquid media • Skim milk
4040
True and false exercise
1. DST is considered to be a procedure that risks generating aerosols.
2. Misidentification of a strain can lead to clinically irrelevant DST results.
3. Modified proportion method on LJ is currently considered as the reference method for DST of first-line drugs
4. Results should be reported only if quality assurance criteria are satisfied.
4141
Module review: take-home messages The proportion method is valid for susceptibility testing of M.
tuberculosis complex with anti-TB drugs. The proportion method is considered to be a reference standard,
against which other routine methods should be assessed. The proportion method determines the percentage of growth of a
defined inoculum on a drug-free control medium vs. growth on culture media containing the critical concentration of an anti-TB drug.
Slants must be read after 4 weeks of incubation for a provisional result and after 6 weeks of incubation for the definitive interpretation of results.
The critical concentration to define a resistant strain is 1% of the inoculum.
Test with invalid growth control should be repeated.4242
Self-assessment
• Explain the differences between direct and indirect DST methods.
• List the possible errors in performing the proportion method.
• List the consequences of a false resistance.• List the consequences of a false sensitivity.
4343
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