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Mrs.VINDHYA .V.V
ASST.POFESSOR
Microbiology
IMPORTANCE OF TB DAY
 Tuberculosis is a bacterial disease caused by the
bacteria MYCOBACTERIUM TUBERCULOSIS
 TB day is celebrated to raise the common public health
awareness about the epidemic disease of tuberculosis
its causes,prevention ,and cure ,as well as the efforts
done inorder to totally eradicate this disease.
 As around world 1.7 million of the people are dying of
this disease every year.
 Timely TB identification and treatment are essential
for succesful recovery
MYCOBACTERIA
 Mycobacteria are acid fast bacilli
 They do not stain readly,but once stained they resist
decolorisation due to the presence of mycolic acid in
the cell wall.so they are called as acid fast bacilli
 They appear in filamentous form like fungi,hence
called as Mycobacteria
 They are Obligate aerobes growing most successfully
in tissues with a high oxygen content, mainly in the
lungs
History
 Robert Koch
isolated
Mycobacterium
Tuberculosis in 1882
Classification of Mycobacteria
1.Obligate pathogen
Mycobacterium
tuberculosis complex
a. M.tuberculosis
b. M.bovis
c. M.africanum
d. M.leprae
2.Oppertunistic
pathogens
a. Atypical mycobacteria
-M.kansai
-M.avium
MORPHOLOGY
 Straight, slightly curved
Acid fast Rod shaped 3 x
0.3microns size
 Gram reaction is positive
 May be single, in pairs or
in small clumps
 Non motile
 Non sporing,Non
capsulated
MTB : Cultural characters
 MTB - Obligate aerobe
 Grow slowly. Generation
time 14-15 hrs
 Colonies appear after 2
weeks or at 6-8 weeks
 Grows at 370c
 Ph between 6.4 to 7.0
 Addition of 0.5%glycerol
improves its growth.
Nature of Media Used
 Helps the growth needs
 Solid Medium is
commonly used.
 SOLID MEDIA
1. Lowenstein Jensen’s
medium,Petrangini,Do
rset[contain egg]
2. Tarshis media [blood]
3. Loeffler[serum]
4. Pawlosky[potato]
 Most commonly used
is
 Lowenstein Jensen’s
Medium
 Contain coagulated egg
 Mineral salt solution
 Asparagine's
 Malachite
green[selective agent]
Liquid media
1. Dubos
2. middlebrook’s
3. Proskauer
4. Beck’s
5. Sula’s
On L J Medium
 M.tuberculosis appear
dry, rough raised
irregular colonies
 Appear wrinkled
 They appear creamy
white
 Become yellowish
ON LIQUID MEDIA
 Growth begins at the
bottom,creeps up sides
and forms
prominantsurface
pellicle formation
Resistance of Mycobacterium
 Mycobacterium are
killed at 600c in 15 – 20
mt
 In sputum they survive
for 20 – 30hours
 Relatively resistant to
several chemicals
including Phenol 5 %
 Sensitive to
Glutaraldehyde and
Formaldehyde
 Bacilli survive in
Droplets for 8 – 10 days
Biochemical Tests on
Mycobacterium spp
 Niacin test – positive for Mycobacterium
 Aryl sulphatase test – Negative
 Neutral red test-Positive
 Catalase and peroxidase test – Differentiates Atypical
from Typical
Most Atypical are strongly Catalase positive
Tubercle bacilli are weakly positive
Tubercle bacilli are peroxidase positive – not atypical
• Nitrate reduction test-Positive
Antigenic Characters
 Group specificity due to Polysaccharides
 Type specificity to protein antigens
 Delayed hypersensitivity to proteins
How tuberculosisspreads
 Tuberculosis (TB) is a contagious disease.
 Source of Infection – Open case of Pulmonary
Tuberculosis.
 Coughing , Sneezing, or Talking.
 Each act can spill 3000 infective nuclei in the air,
 Infective particles are engulfed by Alveolar
Macrophages.
Tuberculosis spread by
Respiratory route
Poverty and Crowded living
spreads Tuberculosis
Generation of Droplet Nuclei
 One cough produces 500
droplets
 The average TB patient
generates 75,000
droplets per day before
therapy
 This falls to 25 infectious
droplets per day within
two weeks of effective
therapy
Dr.T.V.Rao MD 20
Predisposing Factors
 Genetic basis,
 Age
 Stress,
 Nutrition,
 Co existing infections
Eg. HIV
 Ingestion of infected
milk
Pathway of pathogenesis
 Inhalation of bacteria
 Reach lung
 Ingested by alveolar macrophages
 Multiplication in macrophages
 Ghon focus in lower lobe Hilar lymph node
Primary complex formation
 Healing and calcification Haematogenous
 Cause latent infection miliary ,meningeal
disseminated tb
 Reactivation or exogenous infection
 Secondary tb
 Usually pulmonary tb
Extra pulmonary Tuberculosis
 Bacteria on circulation leads to bacteremia leads to
involvement of
GUT, Genito urinary system, Meningitis
Gastro Intestinal system, skin, Lymph nodes Bone
marrow.
Spinal infection Potts spine, Arthritis
Multiorgan Involvement
in Tuberculosis.
Mechanisms of Infection
Mycobacterium do not produce toxins.
Allergy and Immunity plays the major role.
Only 1/10 of the infected will get disease.
Cell Mediated Immunity plays a crucial role.
Humoral Immunity – not Important.
CD4 Cell plays role in Immune Mechanisms.
Lesion –known as Tubercle
 Tubercle is a Avascular granuloma Contain central
zone of giant cells with or without caseation and
peripheral zone of Lymphocytes and Fibroblasts.
 Produce lesions may be
Exudative or Productive
Tubercle with Caseous Necrosis
Dr.T.V.Rao MD 28
Giant cells
Tubercle bacilli
Partially activated
macrophage
Lymphocyte
Fully activated
macrophage
Lesions in Tuberculosis
Exudative – and Productive
 Exudative – Acute inflammatory reaction with
edema fluid – contains Polymorphs-
Lymphocytes – later Mononuclear cells.
Bacilli are virulent .
Productive Type protective Immunity
Dr.T.V.Rao MD 30
Majority of the Tuberculosis
are Pulmonary
Symptoms and Signs of
Tuberculosis
Dr.T.V.Rao MD 31
Clinical Illness with Tuberculosis
 Pulmonary Disease – Major manifestation with
involvement of Lungs
Hemoptysis, Chest pain Fever sweets
Anorexia
Cavity formation in Lungs
Complication of Tuberculosis.
1. Meningitis.
2. Pleurisy,
3. Involvement of Kidney,
4. Spine ( Potts spine )
5. Bone Joints,
6. Miliary tuberculosis
Dr.T.V.Rao MD 34
Tuberculosis - Lymphadenitis
Diagnosis of Tuberculosis
Types of specimens
:
-Sputum.
- BAL.
-Pleural effusions
- Urine
- Stool
-CSF
-Aspiration ( gastric – cold abscess)
- Blood in case of haematogenous TB
METHODS
1. MICROSCOPY
2. CULTURE
3. SEROLOGY
4. MOLECULAR METHODS
5. BACTERIOPHAGE BASED ANALYSIS
6. MYCOLIC ACID CHARACTERISATION
7. ANIMAL INOCULATION
Concentration of specimens
 When AFB not concentrated by direct microscopy
then specimens are concentrated by different
techniques.2methods are there
 1.petroff’s method 2.modified petroff’s
 1.petroff’s method-- equal volumes of sputum sample
and 4%sodium hydroxide are mixed incubated at 370c
for 20-30 minutes and sediment used for microscopy
and culture.
MICROSCOPY
1- Sputum smears stained by Z-N stain
Three morning successive mucopurulent
sputum samples are needed to diagnose
pulmonary TB.
Advantage: - cheap – rapid
- Easy to perform
- High predictive value > 90%
- Specificity of 98%
Disadvantages:
- sputum ( need to contain 5000-10000 AFB/ ml.)
- Young children, elderly & HIV infected persons
may not produce cavities & sputum containing AFB.
GRADING BY RNTCP
Number of bacilli observed Grade
ZERO --
1-2bacilli/300fields --
1-9bacilli/100field --
1-9bacilli/10field --
-
1-9bacilli/field --
>9bacilli/field --
Negative
 Positive
 1+
 2+
• 3+
• 4+
2- Detecting AFB by
fluorochrome stain using
fluorescence microscopy
:
The smear may be stained by aura mine-O dye. In this method the
TB bacilli are stained yellow against dark background & easily
visualized using florescent microscope.
Advantages:
- More sensitive
- Rapid
Disadvantages:
- Hazards of dye toxicity
- more expensive
- must be confirmed by Z-N stain
Acid fast Bacilli seen as in
Florescent Microscope
3- Culture on L J media
Tuberculin Test[mantoux test]
 It is typeIV hypersensitivity reaction
 Purified protein derivative is inoculated intradermally
on forearm
 Site observed after 72hrs for appearance of area of
erythema and induration
 About 10mm indicate positive test
 Below 5mm indicate negative
 Between 5&9 mm indicates doubtful test
Recent Methods for Diagnosis
I – BACTEC 460 ( rapid radiometric culture
system )
specimens are cultured in a liquid medium (Middle brook7H9
broth base )containing C14 – labeled palmitic acid & PANTA
antibiotic mixture.
Growing mycobacteria utilize the acid, releasing radioactive
CO2 which is measured as growth index (GI) in the BACTEC
instrument.
The daily increase in GI output is directly proportional to the
rate & amount of growth in the medium.
III Polymerase Chain Reaction (PCR) & Gene
probe
Other rapid identification methods
are
 MGIT—Mycobacteria Growth Indicator Tube
 BACTEC 9000MB
 BACTEC MGIT 960
 ESP CULTURE SYSTEM 2
 SEPTICHECK AFB SYSTEM[Manual]
Sero diagnosis
ANTIGEN DETECTION
a. Latex particle agglutination
b. Dipstick ELISA
c. Sandwich ELISA
d. Capture ELISA
ANTIBODY DETECTION
a. ELISA
b. INSTA TEST TB
ANIMAL INOCULATION
 The conc.sample is inoculated intra muscularily into
the thigh of 2 healthy Guinea pigs about 12 wks old.
 The animals are weighed b4 inoculation and intervels
thereafter
 Progressive loss of weight is an indication of the
infection
 Positive animal will show a caseous lesion at the site of
inoculation.
Treatment
Drugs used :
1- First line drugs :
- Isoniazid - Rifampicin - Pyrazinamide
- Ethambutol - Streptomycin
2- Second line drugs (more toxic and less effective):
- Kanamycin - capreomycin - Cycloserin
- ethionamide - ciprofloxacin - Ofloxacin
Mycobacteria develops drug resistance.Reason for this is –
improper prescription,delayed initiation of effective
therapy.and HIV infections
So as a control measure DOTS
strategy becomes important
DOTS-Directly Observed
Treatment Short course
‘This ensures that,the patient takes
medicines regularly untill they are
cured’-during the intensive phase a
health worker watches the patient
taking drug in his or her presence.
5 ELEMENTS OF DOTS ARE
1. Government commitment
2. Case detection through quality assured bacteriology
3. Standardised treatment with patient support and
supervision
4. An effective drug supply and management system
5. Monitoring and evaluation system
Immuno-prophylaxis
 BCG
 Intradermal injection of live attenuated vaccine Bacille
Calmette-Guerin (BCG).
 The strain causes self limited lesion and induces
hypersensitivity & immunity.
 Immunity lasts for 10-15 years. Immunity 60-80%
 Some studies proved BCG is doubtful value in
prevention of Tuberculosis

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Tuberculosis

  • 2. IMPORTANCE OF TB DAY  Tuberculosis is a bacterial disease caused by the bacteria MYCOBACTERIUM TUBERCULOSIS  TB day is celebrated to raise the common public health awareness about the epidemic disease of tuberculosis its causes,prevention ,and cure ,as well as the efforts done inorder to totally eradicate this disease.  As around world 1.7 million of the people are dying of this disease every year.  Timely TB identification and treatment are essential for succesful recovery
  • 3. MYCOBACTERIA  Mycobacteria are acid fast bacilli  They do not stain readly,but once stained they resist decolorisation due to the presence of mycolic acid in the cell wall.so they are called as acid fast bacilli  They appear in filamentous form like fungi,hence called as Mycobacteria  They are Obligate aerobes growing most successfully in tissues with a high oxygen content, mainly in the lungs
  • 5. Classification of Mycobacteria 1.Obligate pathogen Mycobacterium tuberculosis complex a. M.tuberculosis b. M.bovis c. M.africanum d. M.leprae 2.Oppertunistic pathogens a. Atypical mycobacteria -M.kansai -M.avium
  • 6.
  • 7. MORPHOLOGY  Straight, slightly curved Acid fast Rod shaped 3 x 0.3microns size  Gram reaction is positive  May be single, in pairs or in small clumps  Non motile  Non sporing,Non capsulated
  • 8. MTB : Cultural characters  MTB - Obligate aerobe  Grow slowly. Generation time 14-15 hrs  Colonies appear after 2 weeks or at 6-8 weeks  Grows at 370c  Ph between 6.4 to 7.0  Addition of 0.5%glycerol improves its growth.
  • 9. Nature of Media Used  Helps the growth needs  Solid Medium is commonly used.  SOLID MEDIA 1. Lowenstein Jensen’s medium,Petrangini,Do rset[contain egg] 2. Tarshis media [blood] 3. Loeffler[serum] 4. Pawlosky[potato]  Most commonly used is  Lowenstein Jensen’s Medium  Contain coagulated egg  Mineral salt solution  Asparagine's  Malachite green[selective agent]
  • 10. Liquid media 1. Dubos 2. middlebrook’s 3. Proskauer 4. Beck’s 5. Sula’s
  • 11. On L J Medium  M.tuberculosis appear dry, rough raised irregular colonies  Appear wrinkled  They appear creamy white  Become yellowish
  • 12. ON LIQUID MEDIA  Growth begins at the bottom,creeps up sides and forms prominantsurface pellicle formation
  • 13. Resistance of Mycobacterium  Mycobacterium are killed at 600c in 15 – 20 mt  In sputum they survive for 20 – 30hours  Relatively resistant to several chemicals including Phenol 5 %  Sensitive to Glutaraldehyde and Formaldehyde  Bacilli survive in Droplets for 8 – 10 days
  • 14. Biochemical Tests on Mycobacterium spp  Niacin test – positive for Mycobacterium  Aryl sulphatase test – Negative  Neutral red test-Positive  Catalase and peroxidase test – Differentiates Atypical from Typical Most Atypical are strongly Catalase positive Tubercle bacilli are weakly positive Tubercle bacilli are peroxidase positive – not atypical • Nitrate reduction test-Positive
  • 15. Antigenic Characters  Group specificity due to Polysaccharides  Type specificity to protein antigens  Delayed hypersensitivity to proteins
  • 16. How tuberculosisspreads  Tuberculosis (TB) is a contagious disease.  Source of Infection – Open case of Pulmonary Tuberculosis.  Coughing , Sneezing, or Talking.  Each act can spill 3000 infective nuclei in the air,  Infective particles are engulfed by Alveolar Macrophages.
  • 18. Poverty and Crowded living spreads Tuberculosis
  • 19. Generation of Droplet Nuclei  One cough produces 500 droplets  The average TB patient generates 75,000 droplets per day before therapy  This falls to 25 infectious droplets per day within two weeks of effective therapy
  • 21. Predisposing Factors  Genetic basis,  Age  Stress,  Nutrition,  Co existing infections Eg. HIV  Ingestion of infected milk
  • 22. Pathway of pathogenesis  Inhalation of bacteria  Reach lung  Ingested by alveolar macrophages  Multiplication in macrophages  Ghon focus in lower lobe Hilar lymph node
  • 23. Primary complex formation  Healing and calcification Haematogenous  Cause latent infection miliary ,meningeal disseminated tb  Reactivation or exogenous infection  Secondary tb  Usually pulmonary tb
  • 24. Extra pulmonary Tuberculosis  Bacteria on circulation leads to bacteremia leads to involvement of GUT, Genito urinary system, Meningitis Gastro Intestinal system, skin, Lymph nodes Bone marrow. Spinal infection Potts spine, Arthritis
  • 26. Mechanisms of Infection Mycobacterium do not produce toxins. Allergy and Immunity plays the major role. Only 1/10 of the infected will get disease. Cell Mediated Immunity plays a crucial role. Humoral Immunity – not Important. CD4 Cell plays role in Immune Mechanisms.
  • 27. Lesion –known as Tubercle  Tubercle is a Avascular granuloma Contain central zone of giant cells with or without caseation and peripheral zone of Lymphocytes and Fibroblasts.  Produce lesions may be Exudative or Productive
  • 28. Tubercle with Caseous Necrosis Dr.T.V.Rao MD 28 Giant cells Tubercle bacilli Partially activated macrophage Lymphocyte Fully activated macrophage
  • 29. Lesions in Tuberculosis Exudative – and Productive  Exudative – Acute inflammatory reaction with edema fluid – contains Polymorphs- Lymphocytes – later Mononuclear cells. Bacilli are virulent . Productive Type protective Immunity
  • 30. Dr.T.V.Rao MD 30 Majority of the Tuberculosis are Pulmonary
  • 31. Symptoms and Signs of Tuberculosis Dr.T.V.Rao MD 31
  • 32. Clinical Illness with Tuberculosis  Pulmonary Disease – Major manifestation with involvement of Lungs Hemoptysis, Chest pain Fever sweets Anorexia Cavity formation in Lungs
  • 33. Complication of Tuberculosis. 1. Meningitis. 2. Pleurisy, 3. Involvement of Kidney, 4. Spine ( Potts spine ) 5. Bone Joints, 6. Miliary tuberculosis
  • 34. Dr.T.V.Rao MD 34 Tuberculosis - Lymphadenitis
  • 36. Types of specimens : -Sputum. - BAL. -Pleural effusions - Urine - Stool -CSF -Aspiration ( gastric – cold abscess) - Blood in case of haematogenous TB
  • 37. METHODS 1. MICROSCOPY 2. CULTURE 3. SEROLOGY 4. MOLECULAR METHODS 5. BACTERIOPHAGE BASED ANALYSIS 6. MYCOLIC ACID CHARACTERISATION 7. ANIMAL INOCULATION
  • 38. Concentration of specimens  When AFB not concentrated by direct microscopy then specimens are concentrated by different techniques.2methods are there  1.petroff’s method 2.modified petroff’s  1.petroff’s method-- equal volumes of sputum sample and 4%sodium hydroxide are mixed incubated at 370c for 20-30 minutes and sediment used for microscopy and culture.
  • 39. MICROSCOPY 1- Sputum smears stained by Z-N stain Three morning successive mucopurulent sputum samples are needed to diagnose pulmonary TB. Advantage: - cheap – rapid - Easy to perform - High predictive value > 90% - Specificity of 98% Disadvantages: - sputum ( need to contain 5000-10000 AFB/ ml.) - Young children, elderly & HIV infected persons may not produce cavities & sputum containing AFB.
  • 40. GRADING BY RNTCP Number of bacilli observed Grade ZERO -- 1-2bacilli/300fields -- 1-9bacilli/100field -- 1-9bacilli/10field -- - 1-9bacilli/field -- >9bacilli/field -- Negative  Positive  1+  2+ • 3+ • 4+
  • 41. 2- Detecting AFB by fluorochrome stain using fluorescence microscopy : The smear may be stained by aura mine-O dye. In this method the TB bacilli are stained yellow against dark background & easily visualized using florescent microscope. Advantages: - More sensitive - Rapid Disadvantages: - Hazards of dye toxicity - more expensive - must be confirmed by Z-N stain
  • 42. Acid fast Bacilli seen as in Florescent Microscope
  • 43. 3- Culture on L J media
  • 44. Tuberculin Test[mantoux test]  It is typeIV hypersensitivity reaction  Purified protein derivative is inoculated intradermally on forearm  Site observed after 72hrs for appearance of area of erythema and induration  About 10mm indicate positive test  Below 5mm indicate negative  Between 5&9 mm indicates doubtful test
  • 45. Recent Methods for Diagnosis I – BACTEC 460 ( rapid radiometric culture system ) specimens are cultured in a liquid medium (Middle brook7H9 broth base )containing C14 – labeled palmitic acid & PANTA antibiotic mixture. Growing mycobacteria utilize the acid, releasing radioactive CO2 which is measured as growth index (GI) in the BACTEC instrument. The daily increase in GI output is directly proportional to the rate & amount of growth in the medium.
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  • 48. III Polymerase Chain Reaction (PCR) & Gene probe
  • 49. Other rapid identification methods are  MGIT—Mycobacteria Growth Indicator Tube  BACTEC 9000MB  BACTEC MGIT 960  ESP CULTURE SYSTEM 2  SEPTICHECK AFB SYSTEM[Manual]
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  • 52. Sero diagnosis ANTIGEN DETECTION a. Latex particle agglutination b. Dipstick ELISA c. Sandwich ELISA d. Capture ELISA
  • 54. ANIMAL INOCULATION  The conc.sample is inoculated intra muscularily into the thigh of 2 healthy Guinea pigs about 12 wks old.  The animals are weighed b4 inoculation and intervels thereafter  Progressive loss of weight is an indication of the infection  Positive animal will show a caseous lesion at the site of inoculation.
  • 55. Treatment Drugs used : 1- First line drugs : - Isoniazid - Rifampicin - Pyrazinamide - Ethambutol - Streptomycin 2- Second line drugs (more toxic and less effective): - Kanamycin - capreomycin - Cycloserin - ethionamide - ciprofloxacin - Ofloxacin Mycobacteria develops drug resistance.Reason for this is – improper prescription,delayed initiation of effective therapy.and HIV infections
  • 56. So as a control measure DOTS strategy becomes important DOTS-Directly Observed Treatment Short course ‘This ensures that,the patient takes medicines regularly untill they are cured’-during the intensive phase a health worker watches the patient taking drug in his or her presence.
  • 57. 5 ELEMENTS OF DOTS ARE 1. Government commitment 2. Case detection through quality assured bacteriology 3. Standardised treatment with patient support and supervision 4. An effective drug supply and management system 5. Monitoring and evaluation system
  • 58. Immuno-prophylaxis  BCG  Intradermal injection of live attenuated vaccine Bacille Calmette-Guerin (BCG).  The strain causes self limited lesion and induces hypersensitivity & immunity.  Immunity lasts for 10-15 years. Immunity 60-80%  Some studies proved BCG is doubtful value in prevention of Tuberculosis