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Acid-fast staining
Anup Muni Bajracharya
Acid-fast staining
ā€¢ is a differential staining
ā€¢ used to differentiate acid fast and non acid fast bacteria.
ā€¢ used to identify acid-fast organisms such as members of
the genus Mycobacterium .
ā€¢ also known as Ziehl-Neelsen method
ā€¢ first introduced by Paul Ehrlich later modified by two
German doctors bacteriologist Franz Ziehl (1859ā€“1926)
and the pathologist Friedrich Neelsen (1854ā€“1898).
A.B
History
ā€¢ In 1882 Robert Koch discovered the etiology of tuberculosis.
ā€¢ Soon after Kochā€™s discovery, Paul Ehrlich developed a stain for
mycobacterium tuberculosis, called the alum hematoxylin stain.
ā€¢ Franz Ziehl then altered Ehrlichā€™s staining technique by using
carbolic acid as the mordant.
ā€¢ Friedrich Neelsen kept Ziehlā€™s choice of mordant but changed the
primary stain to carbol fuchsin.
ā€¢ Ziehl and Neelsenā€™s modifications together have developed the
Ziehl-Neelsen stain.
ā€¢ Another acid-fast satin was developed by Joseph Kinyoun by using
the Ziehl-Neelsen staining technique but removing the heating step
from the procedure.
ā€¢ This new stain from Kinyoun was named the Kinyoun stain.
A.B
What are acid fast bacteria?
ā€¢ those which have a high content of mycolic acids in
their cell walls.
ā€¢ are characterized by
ā€¢ wax-like, nearly impermeable cell walls;
ā€¢ contain mycolic acid and large amounts of fatty acids,
waxes, and complex lipids.
ā€¢ are highly resistant to disinfectants and dry conditions.
ā€¢ Due to their waxy cell wall components,
Mycobacterium are acid fast; that is, they retain the
red dye, carbol fuchsin, after rinsing with acid solvents.
A.B
Acid fast organisms
Acid-fast organisms like
Mycobacterium contain large
amounts of lipid substances,mycolic
acids. which resist staining by
ordinary methods such as a Gram
stain.
Require acid-fast staining that
is used to screen for the
Mycobacterium, Nocardia, and
Legionella species in body
tissues and fluids.
Acid-fastness is an uncommon
characteristic shared by the
genera Mycobacterium and Nocardia
(weakly acid-fast).
Because of this feature, this stain is
extremely helpful in identification in
diseases caused by acid-fast bacteria,
particularly tuberculosis and leprosy.
A.B
Principle
ā€¢ Because the cell wall containing mycolic acid is so waxy and
resistant to most compounds, acid-fast organisms require a
special staining technique.
ā€¢ The primary stain used in acid-fast staining, carbol fuchsin,
is lipid-soluble and contains phenol, which helps the stain
penetrate the cell wall. This is further assisted by the
addition of heat.
ā€¢ The smear is then rinsed with a very strong decolorizer,
which strips the stain from all non-acid-fast cells but does
not permeate the cell wall of acid-fast organisms.
ā€¢ The decolorized non-acid-fast cells then take up the
counterstain.
ā€¢ Acid fast bacteria will be red, while nonacid fast bacteria
will stain green.
A.B
A.B
Requirements
Reagents
ā€¢ Primary Stain: Carbol-fuchsin.
ā€¢ Decoloriser: (HCl+Ethanol)
ā€¢ Counterstain: Methylene blue.
Materials
Slides
Sample
Inoculating loop
Bunsen burner
Cotton
Microscope
A.B
Preparation of reagents
ā€¢ Primary Stain: 0.3% Carbol-fuchsin.
ā€¢ Dissolve 50 g phenol in 100 mL ethanol (95%).
ā€¢ Dissolve 3 g Basic fuchsin in the mixture and add
distilled water to bring the volume to 1 L.
Decolorization Solution: (HCl+Ethanol)
ā€¢ Add 30 mL hydrochloric acid to 1 L of 95% denatured
alcohol.
ā€¢ Cool and mix well before use.
Counterstain: 0.3% Methylene blue.
ā€¢ Dissolve 3 g methylene blue in 1 L distilled water.
A.B
Procedure
ā€¢ Take a clean grease free slide.
ā€¢ Prepare the smear from provided sample.
ā€¢ Air dry and heat fixed the smear.
ā€¢ Place a small strip of filter paper over the top of smear and place the slide
over a boiling hot water bath on a mesh surface.
ā€¢ Cover the filter paper with the primary stain, carbol fuchsin.
ā€¢ Leave the slide on the water bath for 5 minutes or more.
ā€¢ Note- Continue to apply stain if the filter paper begins to dry.
ā€¢ Remove the filter paper and rinse the slide with water until the solution
runs clear.
ā€¢ Run acid-alcohol decolorizer over the slide for approximately 10 to 15
seconds.
ā€¢ Rinse the slide with water.
ā€¢ Cover the smear with the counterstain, methylene blue, for 1 minute.
ā€¢ Gently rinse the slide with water.
ā€¢ Blot the slide dry with bibulous paper.
ā€¢ Observe under microscope. A.B
Procedure
A.B
Observation under Microscope
Acid fast: Red, straight or
slightly curved rods, occurring
singly or in small groups, may
appear beaded
Non-acid fast: Blue color; In
addition, background material
stain blue.
A.B
Organisms stained by acid fast staining
A.B
Kinyoun stain
ā€¢ Unlike the (Z-N stain), the Kinyoun method of staining does
not require heating.
ā€¢ In the ZN stain, heat acts as a physical mordant while
phenol (carbol of carbol fuschin) acts as the chemical
mordant.
ā€¢ Since the Kinyoun stain is a cold method (no heat applied),
the concentration of carbol fuschin used is increased.
A.B
Identify Acid-Fast Bacteria Using Staining Techniques

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Identify Acid-Fast Bacteria Using Staining Techniques

  • 2. Acid-fast staining ā€¢ is a differential staining ā€¢ used to differentiate acid fast and non acid fast bacteria. ā€¢ used to identify acid-fast organisms such as members of the genus Mycobacterium . ā€¢ also known as Ziehl-Neelsen method ā€¢ first introduced by Paul Ehrlich later modified by two German doctors bacteriologist Franz Ziehl (1859ā€“1926) and the pathologist Friedrich Neelsen (1854ā€“1898). A.B
  • 3. History ā€¢ In 1882 Robert Koch discovered the etiology of tuberculosis. ā€¢ Soon after Kochā€™s discovery, Paul Ehrlich developed a stain for mycobacterium tuberculosis, called the alum hematoxylin stain. ā€¢ Franz Ziehl then altered Ehrlichā€™s staining technique by using carbolic acid as the mordant. ā€¢ Friedrich Neelsen kept Ziehlā€™s choice of mordant but changed the primary stain to carbol fuchsin. ā€¢ Ziehl and Neelsenā€™s modifications together have developed the Ziehl-Neelsen stain. ā€¢ Another acid-fast satin was developed by Joseph Kinyoun by using the Ziehl-Neelsen staining technique but removing the heating step from the procedure. ā€¢ This new stain from Kinyoun was named the Kinyoun stain. A.B
  • 4. What are acid fast bacteria? ā€¢ those which have a high content of mycolic acids in their cell walls. ā€¢ are characterized by ā€¢ wax-like, nearly impermeable cell walls; ā€¢ contain mycolic acid and large amounts of fatty acids, waxes, and complex lipids. ā€¢ are highly resistant to disinfectants and dry conditions. ā€¢ Due to their waxy cell wall components, Mycobacterium are acid fast; that is, they retain the red dye, carbol fuchsin, after rinsing with acid solvents. A.B
  • 5. Acid fast organisms Acid-fast organisms like Mycobacterium contain large amounts of lipid substances,mycolic acids. which resist staining by ordinary methods such as a Gram stain. Require acid-fast staining that is used to screen for the Mycobacterium, Nocardia, and Legionella species in body tissues and fluids. Acid-fastness is an uncommon characteristic shared by the genera Mycobacterium and Nocardia (weakly acid-fast). Because of this feature, this stain is extremely helpful in identification in diseases caused by acid-fast bacteria, particularly tuberculosis and leprosy. A.B
  • 6. Principle ā€¢ Because the cell wall containing mycolic acid is so waxy and resistant to most compounds, acid-fast organisms require a special staining technique. ā€¢ The primary stain used in acid-fast staining, carbol fuchsin, is lipid-soluble and contains phenol, which helps the stain penetrate the cell wall. This is further assisted by the addition of heat. ā€¢ The smear is then rinsed with a very strong decolorizer, which strips the stain from all non-acid-fast cells but does not permeate the cell wall of acid-fast organisms. ā€¢ The decolorized non-acid-fast cells then take up the counterstain. ā€¢ Acid fast bacteria will be red, while nonacid fast bacteria will stain green. A.B
  • 7. A.B
  • 8. Requirements Reagents ā€¢ Primary Stain: Carbol-fuchsin. ā€¢ Decoloriser: (HCl+Ethanol) ā€¢ Counterstain: Methylene blue. Materials Slides Sample Inoculating loop Bunsen burner Cotton Microscope A.B
  • 9. Preparation of reagents ā€¢ Primary Stain: 0.3% Carbol-fuchsin. ā€¢ Dissolve 50 g phenol in 100 mL ethanol (95%). ā€¢ Dissolve 3 g Basic fuchsin in the mixture and add distilled water to bring the volume to 1 L. Decolorization Solution: (HCl+Ethanol) ā€¢ Add 30 mL hydrochloric acid to 1 L of 95% denatured alcohol. ā€¢ Cool and mix well before use. Counterstain: 0.3% Methylene blue. ā€¢ Dissolve 3 g methylene blue in 1 L distilled water. A.B
  • 10. Procedure ā€¢ Take a clean grease free slide. ā€¢ Prepare the smear from provided sample. ā€¢ Air dry and heat fixed the smear. ā€¢ Place a small strip of filter paper over the top of smear and place the slide over a boiling hot water bath on a mesh surface. ā€¢ Cover the filter paper with the primary stain, carbol fuchsin. ā€¢ Leave the slide on the water bath for 5 minutes or more. ā€¢ Note- Continue to apply stain if the filter paper begins to dry. ā€¢ Remove the filter paper and rinse the slide with water until the solution runs clear. ā€¢ Run acid-alcohol decolorizer over the slide for approximately 10 to 15 seconds. ā€¢ Rinse the slide with water. ā€¢ Cover the smear with the counterstain, methylene blue, for 1 minute. ā€¢ Gently rinse the slide with water. ā€¢ Blot the slide dry with bibulous paper. ā€¢ Observe under microscope. A.B
  • 12. Observation under Microscope Acid fast: Red, straight or slightly curved rods, occurring singly or in small groups, may appear beaded Non-acid fast: Blue color; In addition, background material stain blue. A.B
  • 13. Organisms stained by acid fast staining A.B
  • 14. Kinyoun stain ā€¢ Unlike the (Z-N stain), the Kinyoun method of staining does not require heating. ā€¢ In the ZN stain, heat acts as a physical mordant while phenol (carbol of carbol fuschin) acts as the chemical mordant. ā€¢ Since the Kinyoun stain is a cold method (no heat applied), the concentration of carbol fuschin used is increased. A.B