GRAM STAINING
AIM
To differentiate two important
groups of bacteria such as Gram positive and Gram negative.
PRINCIPLE
Gram staining technique is a
Differential staining method used to differentiate bacterial species
into two large groups (Gram positive and Gram negative) based on its
cell wall composition Peptidoglycan. The name comes from the Danish
Bacteriologist Hans Christian Gram, who developed the technique in 1884
(originally devised in 1882 but published in 1884). The Crystal violet act as a
Primary stain, Iodine act as a Mordant, 95 % Ethyl alcohol or Acetone act as a
Decolourizing agent and Safranine act as a Counter stain. The Mordant forms the
link between the cell wall of the bacteria and the Primary stain Crystal
violet.
Gram staining is still the
cornerstone of bacterial identification and taxonomic division. Gram positive
bacteria resist decolourization (due to thick Cell wall peptidoglycan) and
appear violet in colour due to the Primary stain Crystal Violet. Gram negative
bacteria undergo decolourization (due to thin Cell wall peptidoglycan) and
takes the Counter stain Safranine and appear pink in colour. Decolourization
step is an important step of Gram staining process because the Decolourization
step distinguishes Gram positive from Gram negative cells. If the decolourizer
95 % Ethyl alcohol or Acetone remains on the sample for too long, it may also
decolorize Gram positive cells.
Based on shape, bacteria are
classified into two types. They are Cocci and Bacilli.
a) Gram positive cocci – Violet colour and Spherical
shape. Example, Staphylococcus sp. (arranged in clusters) and Streptococcus
sp. (arranged in chains).
b) Gram positive bacilli - Violet colour and Rod shape.
Example, Bacillus sp. & Lactobacillus sp.
c) Gram negative cocci – Pink colour and Spherical shape.
Example, Neisseria sp.
d) Gram negative bacilli - Pink colour and Rod shape.
Example, E. coli and Salmonella typhi.
MATERIALS
REQUIRED
i.
Bacterial culture
ii. Microscopic
slide
iii. Inoculation
loop
iv. Crystal
violet
v. Gram’s
Iodine
vi. Gram’s
Decolourizer (95 % Ethyl Alcohol/ Acetone)
vii. Safranine
viii. Bunsen
Burner
ix.
Microscope
PROCEDURE
a) Clean and dry the microscopic slide thoroughly.
b) Prepare thin smear of given bacteria on a clean glass
slide.
c) Allow the smear to air dry and fixed with heat.
d) Flood the smear with Crystal violet and allow it for
one minute.
e) Wash the smear with distilled water for few seconds
using running water.
f) Stain the smear with Iodine solution for one minute.
g) Wash Iodine solution with running water.
h) Add Decolourizer (95 % Ethyl alcohol/Acetone) drop
wise for 10 - 15 seconds, until no more color flows from the smear.
i) Wash the slide with distilled water and drained
properly.
j) Stain the smear finally with counter stain Safranin
for 2 minutes.
k) Wash the slide with running water and dried properly.
l) Observe the slide under Low power objective (10 x or
40 x) and High power objectives (100 x Oil immersion) of the microscope.
OBSERVATION AND RESULTS
a) Gram positive cocci – Violet colour and Spherical
shape.
b) Gram positive bacilli - Violet colour and Rod shape.
c) Gram negative cocci – Pink colour and Spherical shape.
d) Gram negative bacilli - Pink colour and Rod shape.
Figure – 1: Steps
involved in Gram staining (Source: globalindoorhealthnetwork.com)
Figure – 2: Gram
positive cocci
Figure – 3: Gram positive bacilli
Figure – 4: Gram negative cocci
Figure – 5: Gram negative bacilli
Very good for boosting basic understanding
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