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LABORATORY DIAGNOSIS
OF TUBERCULOSIS
CLASSIFICATION OF MYCOBACTERIA
Mycobacterium tuberculosis complex refers to a genetically
related groups of Mycobacterium species that can cause
TUBERCULOSIS [TB] in humans. It includes;
Mycobacterium tuberculosis,
Mycobacterium bovis [M.bovis, subsp bovis, M.bovis subsp.caprae and M.bovis
BCG]
SPECIMEN COLLECTION
In every clinical Microbiology sample collection
“Results are as good as Specimen” Good quality sample
is very important.
Sputum samples of good quality collected in wide mouth
sterile containers.
Quantity sufficient
Extra pulmonary samples collected in sterile containers
/syringes.
Mucoid Sample
Purulent Sample
Bloody Sample
Salivary Sample
DIAGNOSIS OF TUBERCULOSIS
Smear Microscopy
AFB Culture
Manual & Liquid Sensitivity
Molecular Diagnostic
In low income and high tuberculosis prevalence
countries, sputum smear microscopy is the only cost-
effective tool for diagnosing patients with infectious
tuberculosis and to monitor their progress in treatment.
Sputum smear microscopy is a simple, inexpensive,
appropriate technology method which is relatively easy to
perform and to read.
Classical Ziehl-Neelsen stain used-AFB
SMEAR MICROSCOPY
Smear prepared from thick purulent parts of samples.
Size of smear should be 3cmx2cm
At least 300 fields examined
Smear is positive in samples which contain 5000- 10000
bacteria /ml
Sensitivity ranges from 25%-65%
 Sensitivity increases by examination of more than one
smear
SMEAR MICROSCOPY
SIZE OF SMEAR
2 x 3
1 x 2 Uniform Smear
Good Evenness Smear
Uneven Smear
Good Thickness Smear
Too Thick Smear
Too Thin Smear
Smears reported as Positive or
Negative
Quantity of AFB observed
should be noted
Factors influencing smear
sensitivity are type of specimen,
staining technique, experience
of reader
Laboratory Quality Control
important
ZN STAINING
FLUORESCENCE MICROSCOPY
Fluorochrome stain used
Can be examined at lower magnification(40 X)
Rapid but more false positive
LED fluorescence microscopy has been evaluated- rapid
and good results, lower cost
LED attachment to microscope Primo Star iLED from Carl
Zeiss
FLUORESCENCE
MICROSCOPY
DISADVANTAGES OF SMEAR
MICROSCOPY
Needs a large no of bacilli per ml of specimen to be
detected positive
Cannot differentiate between dead and live bacilli
Cannot differentiate between Mtb and NTM
No idea of drug resistance
AFB CULTURE
GOLD STANDARD
Provides definitive diagnosis of TB
Pure growth of mycobacteria to do speciation and drug
sensitivity.
Technically demanding and complex
High level of Biosafety needed
AFB CULTURE BY L.J. MEDIA [SOLID]
Detection of 10-100 viable
bacilli/ml of specimen
Specimens have to be
decontaminated before
inoculation to remove the
normal bacterial flora.
Solid culture – Conventional LJ
method.
Mycobacteria slow growing
and hence take 2-8 weeks to
grow
LOWENSTEIN JENSEN
[L.J. ] MEDIA
LIQUID CULTURE
Many Commercial systems available- BACTEC systems
MGIT960, BacT/ALERT 3D system
Liquid culture yield significantly rapid results than solid
media and isolation rates for mycobacteria are higher
Liquid media- Middle brook 7H9 media used
MGIT system( Mycobacterial growth indicator tubes)
contains a modified Middle brook 7H9 broth with a
fluorescence quenching based oxygen sensor. Growth of
mycobacteria leads to oxygen depletion and indicator
fluoresces brightly
Cultures positive in 10-14 days
LIQUID CULTURE BY BACTEC
DRUG SENSITIVITY FOR AFB
Sensitivity to first and second line drugs available
Expensive
High degree of technical expertise and lab infrastructure
required
Rigorous quality control needed
NON COMMERCIAL METHOD
MODS [Microscopic observed drug susceptibility]
 A micro colony method in liquid culture , based on
inoculation of specimens into drug free and drug
containing media, followed by microscopic examination of
early growth .
Recommended as direct or indirect tests for rapid
screening of patients suspected of having MDR TB
CRI
( Colorimetric redox indicator)
Indirect testing methods based on the reduction of a
coloured indicator added to liquid culture medium on a
microtitre plate after exposure of M. tb strains to anti TB
drugs in vitro
NRA
(Nitrate reductase assay)
 A direct or indirect method on solid culture based on the
ability of M. tuberculosis to reduce nitrate, which is
detected by a colour reaction
SEROLOGICAL TESTS
NEGATIVE RECOMMENDATION from WHO in 2011
SHOULD NOT BE ORDERED
MOLECULAR TEST
Genotypic methods have considerable advantage of
speed, standardization of testing and reduced requirement
for Biosafety
1. LINE PROBE ASSAY
( HAINS TEST)
2. GENEXPERT
1. LINE PROBE ASSAY ( HAINS TEST)
Simultaneous identification for M.tuberculosis complex
Molecular assay for the detection of resistance to INH &
RIF of M.tuberculosis complex
By detection of most significant mutations to – inhA,
RpoB and the katG genes
Based on DNA strip technology
Can be done from positive cultures (from MGIT,
BacT/ALERT bottles or LJ)
Pulmonary samples which are smear +ve can be done
directly
Detection of multiple genes responsible for the antibiotic
resistance &
Simultaneous recognition of missing wild type gene
Also Available for Second secondline
and identification of some strain of NTM
Limitations of Genotype MTBDRplus
Needs preprocessing of samples.
Needs a PCR set up
Technically demanding
Panic of contamination
Special infrastructure required
Needs dedicated staff and space.
2. GENEXPERT [CBNAAT]
The Xpert MTB/RIF is a cartridge based nucleic acid
amplification test , automated diagnostic test that can
identify Mycobacterium tuberculosis (MTB) DNA and
resistance to Rifampicin (RIF) by Nucleic Acid
Amplification Test(NAAT).
SAMPLES;
Pulmonary samples( Sputum, BAL )
Extra pulmonary samples [Lymph node tissue and
aspirates, CSF, Pus , Gastric lavage and aspirates ( in
children) & Other Tissues]
Pulmonary samples - Xpert MTB/ Rif Sensitivity
Status Sensitivity %
Smear +ve culture +ve 98
Smear –ve culture +ve 68
People with HIV 79
People without HIV 86
Extra pulmonary samples Xpert MTB/Rif - sensitivity and specificity
Samples Sensitivity % Specificity %
Lymphnode tissue and
aspirate
84.9 92.5
CSF 79.5 98.6
Pleural fluid 43.7 98.1
Gastric lavage and
aspirations
83.8 98.1
Other tissue 81.2 98.1
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LaboratorydiagnosisofTB.pptx

  • 2. CLASSIFICATION OF MYCOBACTERIA Mycobacterium tuberculosis complex refers to a genetically related groups of Mycobacterium species that can cause TUBERCULOSIS [TB] in humans. It includes; Mycobacterium tuberculosis, Mycobacterium bovis [M.bovis, subsp bovis, M.bovis subsp.caprae and M.bovis BCG]
  • 3. SPECIMEN COLLECTION In every clinical Microbiology sample collection “Results are as good as Specimen” Good quality sample is very important. Sputum samples of good quality collected in wide mouth sterile containers. Quantity sufficient Extra pulmonary samples collected in sterile containers /syringes.
  • 4. Mucoid Sample Purulent Sample Bloody Sample Salivary Sample
  • 5. DIAGNOSIS OF TUBERCULOSIS Smear Microscopy AFB Culture Manual & Liquid Sensitivity Molecular Diagnostic
  • 6. In low income and high tuberculosis prevalence countries, sputum smear microscopy is the only cost- effective tool for diagnosing patients with infectious tuberculosis and to monitor their progress in treatment. Sputum smear microscopy is a simple, inexpensive, appropriate technology method which is relatively easy to perform and to read. Classical Ziehl-Neelsen stain used-AFB SMEAR MICROSCOPY
  • 7. Smear prepared from thick purulent parts of samples. Size of smear should be 3cmx2cm At least 300 fields examined Smear is positive in samples which contain 5000- 10000 bacteria /ml Sensitivity ranges from 25%-65%  Sensitivity increases by examination of more than one smear SMEAR MICROSCOPY
  • 8. SIZE OF SMEAR 2 x 3 1 x 2 Uniform Smear
  • 9. Good Evenness Smear Uneven Smear Good Thickness Smear Too Thick Smear Too Thin Smear
  • 10. Smears reported as Positive or Negative Quantity of AFB observed should be noted Factors influencing smear sensitivity are type of specimen, staining technique, experience of reader Laboratory Quality Control important ZN STAINING
  • 11. FLUORESCENCE MICROSCOPY Fluorochrome stain used Can be examined at lower magnification(40 X) Rapid but more false positive LED fluorescence microscopy has been evaluated- rapid and good results, lower cost LED attachment to microscope Primo Star iLED from Carl Zeiss
  • 13. DISADVANTAGES OF SMEAR MICROSCOPY Needs a large no of bacilli per ml of specimen to be detected positive Cannot differentiate between dead and live bacilli Cannot differentiate between Mtb and NTM No idea of drug resistance
  • 14. AFB CULTURE GOLD STANDARD Provides definitive diagnosis of TB Pure growth of mycobacteria to do speciation and drug sensitivity. Technically demanding and complex High level of Biosafety needed
  • 15. AFB CULTURE BY L.J. MEDIA [SOLID] Detection of 10-100 viable bacilli/ml of specimen Specimens have to be decontaminated before inoculation to remove the normal bacterial flora. Solid culture – Conventional LJ method. Mycobacteria slow growing and hence take 2-8 weeks to grow LOWENSTEIN JENSEN [L.J. ] MEDIA
  • 16. LIQUID CULTURE Many Commercial systems available- BACTEC systems MGIT960, BacT/ALERT 3D system Liquid culture yield significantly rapid results than solid media and isolation rates for mycobacteria are higher Liquid media- Middle brook 7H9 media used MGIT system( Mycobacterial growth indicator tubes) contains a modified Middle brook 7H9 broth with a fluorescence quenching based oxygen sensor. Growth of mycobacteria leads to oxygen depletion and indicator fluoresces brightly Cultures positive in 10-14 days
  • 18. DRUG SENSITIVITY FOR AFB Sensitivity to first and second line drugs available Expensive High degree of technical expertise and lab infrastructure required Rigorous quality control needed
  • 19. NON COMMERCIAL METHOD MODS [Microscopic observed drug susceptibility]  A micro colony method in liquid culture , based on inoculation of specimens into drug free and drug containing media, followed by microscopic examination of early growth . Recommended as direct or indirect tests for rapid screening of patients suspected of having MDR TB
  • 20. CRI ( Colorimetric redox indicator) Indirect testing methods based on the reduction of a coloured indicator added to liquid culture medium on a microtitre plate after exposure of M. tb strains to anti TB drugs in vitro
  • 21. NRA (Nitrate reductase assay)  A direct or indirect method on solid culture based on the ability of M. tuberculosis to reduce nitrate, which is detected by a colour reaction
  • 22. SEROLOGICAL TESTS NEGATIVE RECOMMENDATION from WHO in 2011 SHOULD NOT BE ORDERED
  • 23. MOLECULAR TEST Genotypic methods have considerable advantage of speed, standardization of testing and reduced requirement for Biosafety 1. LINE PROBE ASSAY ( HAINS TEST) 2. GENEXPERT
  • 24. 1. LINE PROBE ASSAY ( HAINS TEST) Simultaneous identification for M.tuberculosis complex Molecular assay for the detection of resistance to INH & RIF of M.tuberculosis complex By detection of most significant mutations to – inhA, RpoB and the katG genes Based on DNA strip technology Can be done from positive cultures (from MGIT, BacT/ALERT bottles or LJ) Pulmonary samples which are smear +ve can be done directly
  • 25. Detection of multiple genes responsible for the antibiotic resistance & Simultaneous recognition of missing wild type gene Also Available for Second secondline and identification of some strain of NTM Limitations of Genotype MTBDRplus Needs preprocessing of samples. Needs a PCR set up Technically demanding Panic of contamination Special infrastructure required Needs dedicated staff and space.
  • 26. 2. GENEXPERT [CBNAAT] The Xpert MTB/RIF is a cartridge based nucleic acid amplification test , automated diagnostic test that can identify Mycobacterium tuberculosis (MTB) DNA and resistance to Rifampicin (RIF) by Nucleic Acid Amplification Test(NAAT). SAMPLES; Pulmonary samples( Sputum, BAL ) Extra pulmonary samples [Lymph node tissue and aspirates, CSF, Pus , Gastric lavage and aspirates ( in children) & Other Tissues]
  • 27. Pulmonary samples - Xpert MTB/ Rif Sensitivity Status Sensitivity % Smear +ve culture +ve 98 Smear –ve culture +ve 68 People with HIV 79 People without HIV 86 Extra pulmonary samples Xpert MTB/Rif - sensitivity and specificity Samples Sensitivity % Specificity % Lymphnode tissue and aspirate 84.9 92.5 CSF 79.5 98.6 Pleural fluid 43.7 98.1 Gastric lavage and aspirations 83.8 98.1 Other tissue 81.2 98.1