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BACTERIAL
STAINING
basic methods
Dr. T.V. Rao MD
1
Dr.T.V.Rao MD
Microscopy helps to Measure
and Observe the Bacteria
•Measurement
▫ Microorganisms are very small
▫ Use metric system
▫ Metre (m) : standard unit
▫ Micrometre (m) = 1 x10-6 m
▫ Nanometre (nm) = 1 x10-9 m
▫ Angstrom (Å) = 1 x10-10 m
2
Dr.T.V.Rao MD
Why we should be Stain
Bacteria
Bacteria have nearly the same refractive
index as water, therefore, when they are
observed under a microscope they are
opaque or nearly invisible to the naked eye.
Different types of staining methods are used
to make the cells and their internal
structures more visible under the light
microscope.
.
3
Dr.T.V.Rao MD
Staining helps in observation of
Bacteria
• Microscopes are of
little use unless the
specimens for
viewing are prepared
properly.
Microorganisms must
be fixed & stained to
increase visibility,
accentuate specific
morphological
features, and
preserve them for
future use.
4
Dr.T.V.Rao MD
Stains and Staining
• Bacteria are slightly
negatively charged at
pH 7.0
▫ Basic dye stains
bacteria
▫ Acidic dye stains
background
• Simple stain
▫ Aqueous or alcohol
solution of single basic
dye
5
Dr.T.V.Rao MD
What is a Stain
• A stain is a substance that adheres to a cell,
giving the cell color.
• The presence of color gives the cells significant
contrast so are much more visible.
• Different stains have different affinities for
different organisms, or different parts of
organisms
• They are used to differentiate different types of
organisms or to view specific parts of organisms
6
Dr.T.V.Rao MD
Staining Techniques
• Staining is an auxiliary
technique used in
microscopy to enhance
contrast in the
microscopic image.
Stains and dyes are
frequently used in biology
and medicine to highlight
structures in biological
tissues for viewing, often
with the aid of different
microscopes.
7
Dr.T.V.Rao MD
Smearing out of the
sample
8
Dr.T.V.Rao MD
Fixation
• Fixation–which may
itself consist of
several steps–aims to
preserve the shape of
the cells or tissue
involved as much as
possible. Sometimes
heat fixation is used to
kill, adhere, and alter the
specimen so it will accept
stains
9
Dr.T.V.Rao MD
Simple staining
• simplest, the actual
staining process may
involve immersing the
sample (before or after
fixation and mounting)
in dye solution, followed
by rinsing and
observation.
• The stain can be poured
drop by drop on the slide
10
Dr.T.V.Rao MD
Simple staining
• Methylene blue, Basic fuchsin
• Provide the color contrast but impart the same
color to all the organisms in a smear
• Loffler's ethylene blue: Sat. solution of M. blue
in alcohol - 30mlKoH, 0.01% in water -
100mlDissolve the dye in water, filter. For
smear: stain for 3’. For section: stain
11
Dr.T.V.Rao MD
Simple staining (cont..)
• Dilute Carbol fuchsin:- Made by diluting Z-N
stain with 10- 15 times its volume of water- Stain
for 20-25 seconds, wash with water
Use: To demonstrate the morphology of Vibrio
cholera
Polychrome methylene blue:
Use: M’Fadyean’s reaction - B. anthracis
12
Dr.T.V.Rao MD
Simple Stains
13
Dr.T.V.Rao MD
Bacterial arrangement
- Clusters
(group).
- Chains.
- Pairs (diploids).
- No special
arrangement.
14
Dr.T.V.Rao MD
Simple Staining Easier to Perform
But has Limitations
• Simple easy to use;
single staining agent
used; using basic and
acid dyes.
• Features of dyes: give
coloring of
microorganisms; bind
specifically to various
cell structures
15
Dr.T.V.Rao MD
Differential Stains
Differential Stains use two or more stains
and allow the cells to be categorized into
various groups or types.
Both techniques allow the observation of
cell morphology, or shape, but differential
staining usually provides more
information about the characteristics of
the cell wall (Thickness).
16
Dr.T.V.Rao MD
Gram staining
• Named after Hans
Christian Gram,
differentiates
between Gram-
positive purple and
Gram-negative
pink stains and is
used to identify
certain pathogens.
17
Dr.T.V.Rao MD
18
Dr.T.V.Rao MD
Gram staining - Principles
• Gram staining is used to determine gram status to
classify bacteria broadly. It is based on the
composition of their cell wall. Gram staining uses
crystal violet to stain cell walls, iodine as a mordant,
and a fuchsin or safranin counterstain to mark all
bacteria. Gram status is important in medicine; the
presence or absence of a cell wall will change the
bacterium's susceptibility to some antibiotics.
• Gram-positive bacteria stain dark blue or violet.
Their cell wall is typically rich with peptidoglycan
and lacks the secondary membrane and
lipopolysaccharide layer found in Gram-negative
bacteria
19
Dr.T.V.Rao MD
Gram Staining Steps
1. Crystal violet acts as the primary stain. Crystal violet may
also be used as a simple stain because it dyes the cell wall
of any bacteria.
2. Gram’s iodine acts as a mordant (Helps to fix the
primary dye to the cell wall).
3. Decolorizer is used next to remove the primary stain
(crystal violet) from Gram Negative bacteria (those with
LPS imbedded in their cell walls). Decolorizer is
composed of an organic solvent, such as, acetone or
ethanol or a combination of both.)
4. Finally, a counter stain (Safranin), is applied to stain
those cells (Gram Negative) that have lost the primary
stain as a result of decolorization
20
Dr.T.V.Rao MD
Stains differentiates different
groups of Bacteria
• To distinguish
different kinds of
bacteria into
separate groups
based on staining
properties
• Two types: Gram
stain & Acid-fast
stain.
21
Dr.T.V.Rao MD
Differential Stains: Gram Stain
Color of
Gram + cells
Color of
Gram – cells
Primary stain:
Crystal violet
Purple Purple
Mordant:
Iodine
Purple Purple
Decolorizing agent:
Alcohol-acetone
Purple Colorless
Counterstain:
Safranin
Purple Red
22
Dr.T.V.Rao MD
Gram Staining technique
23
Dr.T.V.Rao MD
Gram Staining Procedure 24
Dr.T.V.Rao MD
Gram Staining technique
25
Dr.T.V.Rao MD
Structure and Reactivity to
Gram Staining.
26
Dr.T.V.Rao MD
27
Dr.T.V.Rao MD
Cell structure differentiates Gram
positive from Gram Negative
28
Dr.T.V.Rao MD
Gm+ve cocci & Gm-ve bacilli
29
Dr.T.V.Rao MD
Gram-positive
• Gram-positive bacteria are those that are
stained dark blue or violet by Gram staining.
This is in contrast to Gram-negative bacteria,
which cannot retain the crystal violet stain,
instead taking up the counter stain (safranin or
fuchsine) and appearing red or pink. Gram-
positive organisms are able to retain the crystal
violet stain because of the high amount of
peptidoglycan in the cell wall. Gram-positive cell
walls typically lack the outer membrane found in
Gram-negative bacteria.
30
Dr.T.V.Rao MD
GRAM-POSITIVE BACTERIA
• GRAM-POSITIVE
BACTERIA are
characterized by having as
part of their cell wall
structure peptidoglycan as
well as polysaccharides
and/or teichoic acids. The
peptidoglycans which are
sometimes also called
murein are heteropolymers
of glycan strands, which are
cross-linked through short
peptides.
31
Dr.T.V.Rao MD
What are Gram Negative Bacteria
• Gram-negative bacteria are those bacteria that
do not retain crystal violet dye in the Gram
staining protocol. In a Gram stain test, a counter
stain (commonly safranin) is added after the crystal
violet, coloring all Gram-negative bacteria with a red
or pink color. The test itself is useful in classifying
two distinct types of bacteria based on the structural
differences of their cell walls. On the other
hand, Gram-positive bacteria will retain the crystal
violet dye when washed in a decolorizing solution.
32
Dr.T.V.Rao MD
Gram negative bacteria
• On most Gram-stained
preparations, Gram-negative
organisms will appear red or
pink because they are
counterstained. Due to
presence of higher lipid
content, after alcohol-
treatment, the porosity of the
cell wall increases, hence the
CVI complex (Crystal violet -
Iodine) can pass through.
Thus, the primary stain is not
retained.
33
Dr.T.V.Rao MD
Structural Details of Gram –ve
Bacteria
34
Dr.T.V.Rao MD
Gram Negative Bacteria
• Also, in contrast to
most Gram-positive
bacteria, Gram-
negative bacteria have
only a few layers of
peptidoglycan and a
secondary cell
membrane made
primarily of
lipopolysaccharide
35
Dr.T.V.Rao MD
Common Questions
• 1 Principles of Gram Staining and its uses.
• 2 Name common/pathogenic Gram
positive and Gram negative Bacteria
• 3 Why some bacteria are Gram positive
and others Gram negative.
• 4 Why some bacteria cannot be stained by
Gram’s Method of staining.
• 5 What is the Use of Gram staining in your
future clinical practice.
Dr.T.V.Rao MD
36
ACID FAST
STAINING
Dr.T.V.Rao MD
37
Mycobacterium are Acid Fast
Bacilli
• Mycobacterium are Gram-resistant (waxy cell
walls), non-motile, pleomorphic rods, related to the
Actinomyces. Most Mycobacteria are found in
habitats such as water or soil. However, a few are
intracellular pathogens of animals and humans.
Mycobacterium tuberculosis, along with M. bovis,
M. africanum, and M. microti all cause the disease
known as tuberculosis (TB) and are members of the
tuberculosis species complex. Each member of the
TB complex is pathogenic, but M. tuberculosis is
pathogenic for humans while M. bovis is usually
pathogenic for animals.
38
Dr.T.V.Rao MD
Acid-Fast Stain
• Acid-fast cells contain a
large amount of lipids and
waxes in their cell walls
▫ primarily mycolic
acid
• Acid fast bacteria are
usually members of the
genus Mycobacterium or
Nocardia
▫ Therefore, this stain is
important to identify
Mycobacterium or
Nocardia
39
Dr.T.V.Rao MD
Ziehl-Neelsen stain
• Ziehl-Neelsen staining is used to stain
species of Mycobacterium tuberculosis
that do not stain with the standard
laboratory staining procedures like Gram
staining.
• The stains used are the red colored Carbol
fuchsin that stains the bacteria and a
counter stain like Methylene blue or
Malachite green.
40
Dr.T.V.Rao MD
Acid-Fast Organisms
• Primary stain binds cell wall mycolic
acids
• Intense decolorization does not release
primary stain from the cell wall of AFB
• Color of AFB-based on primary stain
• Counterstain provides contrasting
background
41
Dr.T.V.Rao MD
AFB Staining Methods
•Zeihl
Neelsen’s-hot
stain
•Kinyoun’s-cold
stain
•Modifications
42
Dr.T.V.Rao MD
Ziehl- Neelsen Procedure
Make a smear. Air Dry. Heat Fix.
2. Flood smear with Carbol Fuchsin stain
▫ Carbol Fuchsin is a lipid soluble, phenolic compound, which is
able to penetrate the cell wall
3. Cover flooded smear with filter paper
4. Steam for 10 minutes. Add more Carbol Fuchsin stain as
needed
5. Cool slide
6. Rinse with DI water
7. Flood slide with acid alcohol (leave 15 seconds). The acid
alcohol contains 3% HCl and 95% ethanol,
or you can declorase with 20% H2 S04
▫ The waxy cell wall then prevents the stain from being removed
by the acid alcohol (decolorizer) once it has penetrated the cell
wall. The acid alcohol decolorizer will remove the stain from all
other cells.
43
Dr.T.V.Rao MD
Ziehl- Neelsen Procedure
(continued)
8. Tilt slide 45 degrees over the sink and add acid
alcohol drop wise (drop by drop) until the red
color stops streaming from the smear
9. Rinse with DI water
10. Add Loeffler’s Methylene Blue stain (counter
stain). This stain adds blue color to non-acid fast
cells!! Leave Loeffler’s Blue stain on smear for 1
minute
11. Rinse slide. Blot dry.
12. Use oil immersion objective to view.
44
Dr.T.V.Rao MD
Ziehl-Neelsen
stain
4 5 6
7
1 2 3 45
Dr.T.V.Rao MD
How the Acid fast bacteria
appear
46
Dr.T.V.Rao MD
Fluorochrome AFB Microscopy
* More rapid and
sensitive
* Specificity : same
with sufficient
expĂŠrience
* Equipment cost ,
bulbs, technical
demands
* for busy labs
* External quality
assessment should
be done if this
method is performed
47
Dr.T.V.Rao MD
Fluorescence and Bright-field
Microscopy
48
Dr.T.V.Rao MD
Fluorochrome AFB Microscopy
Primary fluorochrome AFB fluoresces
Auramine O Green
Auramine O-Rhodamine B Yellow/orange
Acridine Orange Yellow/orange
Note: Color of AFB may vary with filter system on microscope
49
Dr.T.V.Rao MD
Staining of M.lepra
• M.lepra are less
acid fast than
M.tuberculosis
group of
organisms,
• The concentration
of H2So4 is
reduced to 5 % for
decolorising
50
Dr.T.V.Rao MD
ALBERT’S STAINING FOR
C.diptheria
Dr.T.V.Rao MD
51
Diphtheria is Serious Disease
When you suspect Diphtheria
• In all cases of suspected
cases of Diphtheria, stain
one of the smears with
Gram stain
• If Gram stained smear
shows morphology
suggestive of C.diptheria,
proceed to do Albert
staining which
demonstrates the
presence or absence of
metachromatic granules.
52
Dr.T.V.Rao MD
Appearance of C.diptheria
• C.diptheria are thin Gram positive bacilli,
straight or slightly curved and often enlarged
(clubbing) at one or both ends and are arranged
at acute angles giving shapes of Chinese letters
or V shape which is characteristic of these
organisms (Fig 1). Present in the body of the
bacillus are numerous metachromatic granules
which give the bacillus beaded or barred
appearance. These granules are best
demonstrated by Albert’s stain.
53
Dr.T.V.Rao MD
Albert staining
• Albert stain I
• Toluidine blue 0.15
gm
Malachite green 0.20
gm
Glacial acetic acid 1.0
ml
Alcohol(95%) 2.0 ml
Distilled water 100 ml
• Albert stain II
•Iodine 2.0 gm
Potassium
iodide 3.0 gm
Distilled water
300 ml
54
Dr.T.V.Rao MD
Albert staining Procedure
• Cover the heat-fixed smear with
Albert stain I. Let it stand for two
minutes.
• Wash with water.
• Cover the smear with Albert stain
II. Let it stand for two minutes.
• Wash with water, blot dry and
examine.
55
Dr.T.V.Rao MD
How the C.diptheria appear
• To demonstrate
metachromatic
granules in
C.diphtheriae. These
granules appear
bluish black whereas
the body of bacilli
appear green or
bluish green.
•
56
Dr.T.V.Rao MD
Flagellar - staining
• Flagella are usually invisible
under light microscopy, but
their identification and
anatomy are important in
determining some pathogens.
Certain chemicals that bind to
the flagella are used in the
staining process. The flagella
color may change or an
increase in contrast should
make them visible.
57
Dr.T.V.Rao MD
Endospore staining
• The cell walls of
endospores are
impermeable to most
chemicals, and being in
the genera Bacillus and
Clostridium, cause
diseases such as anthrax,
teatanus and gangrene.
The staining process
involves both a primary
stain and a counterstain.
58
Dr.T.V.Rao MD
Capsule - Staining
• A stain used to
reveal negatively
charged bacterial
capsules. The
encapsulated
cells will have a
halo appearance
under the
microscope.
59
Dr.T.V.Rao MD
Negative staining
• India Ink, Nigrosin
• Organisms are not stained, only the
background is stained
• Unstained organisms stand out in contrast
• Use: To demonstrate the capsule of
Cryptococcus neoformans, Streptococcus
pneumoniae
60
Dr.T.V.Rao MD
61
Dr.T.V.Rao MD
Nigrosin used for Negative
Staining
• The negative stain is
particularly useful for
determining cell size
and arrangement. It
can also be used to
stain cells that are too
delicate to be heat-
fixed.
62
Dr.T.V.Rao MD
Programme designed by
Dr.T.V.Rao MD for “e” learning
in Microbiology for Medical and
Paramedical students in
Developing world
Email
doctortvrao@gmail.com
Dr.T.V.Rao MD
63

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Stainingbacteria 101004225924-phpapp02

  • 2. Microscopy helps to Measure and Observe the Bacteria •Measurement ▫ Microorganisms are very small ▫ Use metric system ▫ Metre (m) : standard unit ▫ Micrometre (m) = 1 x10-6 m ▫ Nanometre (nm) = 1 x10-9 m ▫ Angstrom (Å) = 1 x10-10 m 2 Dr.T.V.Rao MD
  • 3. Why we should be Stain Bacteria Bacteria have nearly the same refractive index as water, therefore, when they are observed under a microscope they are opaque or nearly invisible to the naked eye. Different types of staining methods are used to make the cells and their internal structures more visible under the light microscope. . 3 Dr.T.V.Rao MD
  • 4. Staining helps in observation of Bacteria • Microscopes are of little use unless the specimens for viewing are prepared properly. Microorganisms must be fixed & stained to increase visibility, accentuate specific morphological features, and preserve them for future use. 4 Dr.T.V.Rao MD
  • 5. Stains and Staining • Bacteria are slightly negatively charged at pH 7.0 ▫ Basic dye stains bacteria ▫ Acidic dye stains background • Simple stain ▫ Aqueous or alcohol solution of single basic dye 5 Dr.T.V.Rao MD
  • 6. What is a Stain • A stain is a substance that adheres to a cell, giving the cell color. • The presence of color gives the cells significant contrast so are much more visible. • Different stains have different affinities for different organisms, or different parts of organisms • They are used to differentiate different types of organisms or to view specific parts of organisms 6 Dr.T.V.Rao MD
  • 7. Staining Techniques • Staining is an auxiliary technique used in microscopy to enhance contrast in the microscopic image. Stains and dyes are frequently used in biology and medicine to highlight structures in biological tissues for viewing, often with the aid of different microscopes. 7 Dr.T.V.Rao MD
  • 8. Smearing out of the sample 8 Dr.T.V.Rao MD
  • 9. Fixation • Fixation–which may itself consist of several steps–aims to preserve the shape of the cells or tissue involved as much as possible. Sometimes heat fixation is used to kill, adhere, and alter the specimen so it will accept stains 9 Dr.T.V.Rao MD
  • 10. Simple staining • simplest, the actual staining process may involve immersing the sample (before or after fixation and mounting) in dye solution, followed by rinsing and observation. • The stain can be poured drop by drop on the slide 10 Dr.T.V.Rao MD
  • 11. Simple staining • Methylene blue, Basic fuchsin • Provide the color contrast but impart the same color to all the organisms in a smear • Loffler's ethylene blue: Sat. solution of M. blue in alcohol - 30mlKoH, 0.01% in water - 100mlDissolve the dye in water, filter. For smear: stain for 3’. For section: stain 11 Dr.T.V.Rao MD
  • 12. Simple staining (cont..) • Dilute Carbol fuchsin:- Made by diluting Z-N stain with 10- 15 times its volume of water- Stain for 20-25 seconds, wash with water Use: To demonstrate the morphology of Vibrio cholera Polychrome methylene blue: Use: M’Fadyean’s reaction - B. anthracis 12 Dr.T.V.Rao MD
  • 14. Bacterial arrangement - Clusters (group). - Chains. - Pairs (diploids). - No special arrangement. 14 Dr.T.V.Rao MD
  • 15. Simple Staining Easier to Perform But has Limitations • Simple easy to use; single staining agent used; using basic and acid dyes. • Features of dyes: give coloring of microorganisms; bind specifically to various cell structures 15 Dr.T.V.Rao MD
  • 16. Differential Stains Differential Stains use two or more stains and allow the cells to be categorized into various groups or types. Both techniques allow the observation of cell morphology, or shape, but differential staining usually provides more information about the characteristics of the cell wall (Thickness). 16 Dr.T.V.Rao MD
  • 17. Gram staining • Named after Hans Christian Gram, differentiates between Gram- positive purple and Gram-negative pink stains and is used to identify certain pathogens. 17 Dr.T.V.Rao MD
  • 19. Gram staining - Principles • Gram staining is used to determine gram status to classify bacteria broadly. It is based on the composition of their cell wall. Gram staining uses crystal violet to stain cell walls, iodine as a mordant, and a fuchsin or safranin counterstain to mark all bacteria. Gram status is important in medicine; the presence or absence of a cell wall will change the bacterium's susceptibility to some antibiotics. • Gram-positive bacteria stain dark blue or violet. Their cell wall is typically rich with peptidoglycan and lacks the secondary membrane and lipopolysaccharide layer found in Gram-negative bacteria 19 Dr.T.V.Rao MD
  • 20. Gram Staining Steps 1. Crystal violet acts as the primary stain. Crystal violet may also be used as a simple stain because it dyes the cell wall of any bacteria. 2. Gram’s iodine acts as a mordant (Helps to fix the primary dye to the cell wall). 3. Decolorizer is used next to remove the primary stain (crystal violet) from Gram Negative bacteria (those with LPS imbedded in their cell walls). Decolorizer is composed of an organic solvent, such as, acetone or ethanol or a combination of both.) 4. Finally, a counter stain (Safranin), is applied to stain those cells (Gram Negative) that have lost the primary stain as a result of decolorization 20 Dr.T.V.Rao MD
  • 21. Stains differentiates different groups of Bacteria • To distinguish different kinds of bacteria into separate groups based on staining properties • Two types: Gram stain & Acid-fast stain. 21 Dr.T.V.Rao MD
  • 22. Differential Stains: Gram Stain Color of Gram + cells Color of Gram – cells Primary stain: Crystal violet Purple Purple Mordant: Iodine Purple Purple Decolorizing agent: Alcohol-acetone Purple Colorless Counterstain: Safranin Purple Red 22 Dr.T.V.Rao MD
  • 24. Gram Staining Procedure 24 Dr.T.V.Rao MD
  • 26. Structure and Reactivity to Gram Staining. 26 Dr.T.V.Rao MD
  • 28. Cell structure differentiates Gram positive from Gram Negative 28 Dr.T.V.Rao MD
  • 29. Gm+ve cocci & Gm-ve bacilli 29 Dr.T.V.Rao MD
  • 30. Gram-positive • Gram-positive bacteria are those that are stained dark blue or violet by Gram staining. This is in contrast to Gram-negative bacteria, which cannot retain the crystal violet stain, instead taking up the counter stain (safranin or fuchsine) and appearing red or pink. Gram- positive organisms are able to retain the crystal violet stain because of the high amount of peptidoglycan in the cell wall. Gram-positive cell walls typically lack the outer membrane found in Gram-negative bacteria. 30 Dr.T.V.Rao MD
  • 31. GRAM-POSITIVE BACTERIA • GRAM-POSITIVE BACTERIA are characterized by having as part of their cell wall structure peptidoglycan as well as polysaccharides and/or teichoic acids. The peptidoglycans which are sometimes also called murein are heteropolymers of glycan strands, which are cross-linked through short peptides. 31 Dr.T.V.Rao MD
  • 32. What are Gram Negative Bacteria • Gram-negative bacteria are those bacteria that do not retain crystal violet dye in the Gram staining protocol. In a Gram stain test, a counter stain (commonly safranin) is added after the crystal violet, coloring all Gram-negative bacteria with a red or pink color. The test itself is useful in classifying two distinct types of bacteria based on the structural differences of their cell walls. On the other hand, Gram-positive bacteria will retain the crystal violet dye when washed in a decolorizing solution. 32 Dr.T.V.Rao MD
  • 33. Gram negative bacteria • On most Gram-stained preparations, Gram-negative organisms will appear red or pink because they are counterstained. Due to presence of higher lipid content, after alcohol- treatment, the porosity of the cell wall increases, hence the CVI complex (Crystal violet - Iodine) can pass through. Thus, the primary stain is not retained. 33 Dr.T.V.Rao MD
  • 34. Structural Details of Gram –ve Bacteria 34 Dr.T.V.Rao MD
  • 35. Gram Negative Bacteria • Also, in contrast to most Gram-positive bacteria, Gram- negative bacteria have only a few layers of peptidoglycan and a secondary cell membrane made primarily of lipopolysaccharide 35 Dr.T.V.Rao MD
  • 36. Common Questions • 1 Principles of Gram Staining and its uses. • 2 Name common/pathogenic Gram positive and Gram negative Bacteria • 3 Why some bacteria are Gram positive and others Gram negative. • 4 Why some bacteria cannot be stained by Gram’s Method of staining. • 5 What is the Use of Gram staining in your future clinical practice. Dr.T.V.Rao MD 36
  • 38. Mycobacterium are Acid Fast Bacilli • Mycobacterium are Gram-resistant (waxy cell walls), non-motile, pleomorphic rods, related to the Actinomyces. Most Mycobacteria are found in habitats such as water or soil. However, a few are intracellular pathogens of animals and humans. Mycobacterium tuberculosis, along with M. bovis, M. africanum, and M. microti all cause the disease known as tuberculosis (TB) and are members of the tuberculosis species complex. Each member of the TB complex is pathogenic, but M. tuberculosis is pathogenic for humans while M. bovis is usually pathogenic for animals. 38 Dr.T.V.Rao MD
  • 39. Acid-Fast Stain • Acid-fast cells contain a large amount of lipids and waxes in their cell walls ▫ primarily mycolic acid • Acid fast bacteria are usually members of the genus Mycobacterium or Nocardia ▫ Therefore, this stain is important to identify Mycobacterium or Nocardia 39 Dr.T.V.Rao MD
  • 40. Ziehl-Neelsen stain • Ziehl-Neelsen staining is used to stain species of Mycobacterium tuberculosis that do not stain with the standard laboratory staining procedures like Gram staining. • The stains used are the red colored Carbol fuchsin that stains the bacteria and a counter stain like Methylene blue or Malachite green. 40 Dr.T.V.Rao MD
  • 41. Acid-Fast Organisms • Primary stain binds cell wall mycolic acids • Intense decolorization does not release primary stain from the cell wall of AFB • Color of AFB-based on primary stain • Counterstain provides contrasting background 41 Dr.T.V.Rao MD
  • 43. Ziehl- Neelsen Procedure Make a smear. Air Dry. Heat Fix. 2. Flood smear with Carbol Fuchsin stain ▫ Carbol Fuchsin is a lipid soluble, phenolic compound, which is able to penetrate the cell wall 3. Cover flooded smear with filter paper 4. Steam for 10 minutes. Add more Carbol Fuchsin stain as needed 5. Cool slide 6. Rinse with DI water 7. Flood slide with acid alcohol (leave 15 seconds). The acid alcohol contains 3% HCl and 95% ethanol, or you can declorase with 20% H2 S04 ▫ The waxy cell wall then prevents the stain from being removed by the acid alcohol (decolorizer) once it has penetrated the cell wall. The acid alcohol decolorizer will remove the stain from all other cells. 43 Dr.T.V.Rao MD
  • 44. Ziehl- Neelsen Procedure (continued) 8. Tilt slide 45 degrees over the sink and add acid alcohol drop wise (drop by drop) until the red color stops streaming from the smear 9. Rinse with DI water 10. Add Loeffler’s Methylene Blue stain (counter stain). This stain adds blue color to non-acid fast cells!! Leave Loeffler’s Blue stain on smear for 1 minute 11. Rinse slide. Blot dry. 12. Use oil immersion objective to view. 44 Dr.T.V.Rao MD
  • 45. Ziehl-Neelsen stain 4 5 6 7 1 2 3 45 Dr.T.V.Rao MD
  • 46. How the Acid fast bacteria appear 46 Dr.T.V.Rao MD
  • 47. Fluorochrome AFB Microscopy * More rapid and sensitive * Specificity : same with sufficient expĂŠrience * Equipment cost , bulbs, technical demands * for busy labs * External quality assessment should be done if this method is performed 47 Dr.T.V.Rao MD
  • 49. Fluorochrome AFB Microscopy Primary fluorochrome AFB fluoresces Auramine O Green Auramine O-Rhodamine B Yellow/orange Acridine Orange Yellow/orange Note: Color of AFB may vary with filter system on microscope 49 Dr.T.V.Rao MD
  • 50. Staining of M.lepra • M.lepra are less acid fast than M.tuberculosis group of organisms, • The concentration of H2So4 is reduced to 5 % for decolorising 50 Dr.T.V.Rao MD
  • 52. Diphtheria is Serious Disease When you suspect Diphtheria • In all cases of suspected cases of Diphtheria, stain one of the smears with Gram stain • If Gram stained smear shows morphology suggestive of C.diptheria, proceed to do Albert staining which demonstrates the presence or absence of metachromatic granules. 52 Dr.T.V.Rao MD
  • 53. Appearance of C.diptheria • C.diptheria are thin Gram positive bacilli, straight or slightly curved and often enlarged (clubbing) at one or both ends and are arranged at acute angles giving shapes of Chinese letters or V shape which is characteristic of these organisms (Fig 1). Present in the body of the bacillus are numerous metachromatic granules which give the bacillus beaded or barred appearance. These granules are best demonstrated by Albert’s stain. 53 Dr.T.V.Rao MD
  • 54. Albert staining • Albert stain I • Toluidine blue 0.15 gm Malachite green 0.20 gm Glacial acetic acid 1.0 ml Alcohol(95%) 2.0 ml Distilled water 100 ml • Albert stain II •Iodine 2.0 gm Potassium iodide 3.0 gm Distilled water 300 ml 54 Dr.T.V.Rao MD
  • 55. Albert staining Procedure • Cover the heat-fixed smear with Albert stain I. Let it stand for two minutes. • Wash with water. • Cover the smear with Albert stain II. Let it stand for two minutes. • Wash with water, blot dry and examine. 55 Dr.T.V.Rao MD
  • 56. How the C.diptheria appear • To demonstrate metachromatic granules in C.diphtheriae. These granules appear bluish black whereas the body of bacilli appear green or bluish green. • 56 Dr.T.V.Rao MD
  • 57. Flagellar - staining • Flagella are usually invisible under light microscopy, but their identification and anatomy are important in determining some pathogens. Certain chemicals that bind to the flagella are used in the staining process. The flagella color may change or an increase in contrast should make them visible. 57 Dr.T.V.Rao MD
  • 58. Endospore staining • The cell walls of endospores are impermeable to most chemicals, and being in the genera Bacillus and Clostridium, cause diseases such as anthrax, teatanus and gangrene. The staining process involves both a primary stain and a counterstain. 58 Dr.T.V.Rao MD
  • 59. Capsule - Staining • A stain used to reveal negatively charged bacterial capsules. The encapsulated cells will have a halo appearance under the microscope. 59 Dr.T.V.Rao MD
  • 60. Negative staining • India Ink, Nigrosin • Organisms are not stained, only the background is stained • Unstained organisms stand out in contrast • Use: To demonstrate the capsule of Cryptococcus neoformans, Streptococcus pneumoniae 60 Dr.T.V.Rao MD
  • 62. Nigrosin used for Negative Staining • The negative stain is particularly useful for determining cell size and arrangement. It can also be used to stain cells that are too delicate to be heat- fixed. 62 Dr.T.V.Rao MD
  • 63. Programme designed by Dr.T.V.Rao MD for “e” learning in Microbiology for Medical and Paramedical students in Developing world Email doctortvrao@gmail.com Dr.T.V.Rao MD 63