FOR VIRAL CULTURE CONFIRMATION
The IFA technique is used to identify viral isolates in the cells obtained from shell vials and tube cultures. The indirect method consists of two steps. In the first step, primary antibodies are allowed to react with viral antigens in the cells. These specific complexes are detected in a second step using a species-specific antibody conjugated with a fluorochrome. Viruses which we currently identify by IFA staining include cytomegalovirus immediate early antigen (CMV-IE) and enteroviruses.
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II. Reagents and Materials
Virus-specific antibody
FITC-conjugated antimouse antibody
Phosphate buffered saline (PBS)
Distilled water
Cold acetone (4oC)
Mounting fluid
Sterile pipettes
Cytospin and accessories (for tube cultures)
Humidified chamber
Sterile freezer vial
Glass slides
Coverslips
Paper towels for blotting
Humidified chamber (for tube culture)
III. Procedure
1. Shell Vial
Follow outline in Appendix II to determine if staining should be done in the shell vial itself or if a cytospin needs to be prepared. If the staining is to be done in the shell vial itself, proceed to step i) below.
i. Discard cap. Remove maintenance medium from the shell vial using a clean sterile pipette.
a) Add 1 mL of cold acetone. Cover and fix for 10 minutes.
b) Decant acetone and blot on paper towel.
c) Gently rinse with PBS from squirt bottle, filling vial 3/4 full. Decant PBS.
d) Add 75 ml (2 drops from bottle) of appropriate antibody. Cover.
vi. Incubate at 36oC for 30 minutes.
vii. Gently rinse with PBS from squirt bottle, filling vial 3/4 full. Decant PBS. Repeat.
viii. Add 75ml (2 drops from bottle) of appropriate FITC -conjugated antibodies, cover and repeat steps vi and vii.
x. Remove the coverslip and place cell side down onto a drop of mounting fluid on a glass slide.
xi. Read using fluorescence microscope with the FITC/Evans Blue filter and the 40x objective.
2. Tube Culture (or Shell Vials for CPE)
i. Prepare cytospin preparation from cell culture as outlined in Appendix XX.
ii. Add 20 ml of appropriate antibodies onto the fixed cytospin slide.
iii. Incubate in a humidified chamber for 30 minutes at 36oC.
iv. Wash each slide 3 times with fresh PBS for 2 minutes each in a coplin jar.
v. Wipe excess PBS from the slide without touching the cell spot.
vi. Add 20 ml of appropriate FITC-conjugated antibodies.
vii. Incubate in a humidified chamber at 36oC for 30 minutes.
viii. Wash each slide 3 times with fresh PBS for 2 minutes each in a coplin jar.
ix. Wash with distilled water for 1 minute in a coplin jar.
x. Wipe excess water from the slide without touching the cell spot.
xi. Mount using coverslip and mounting fluid.
xii. Read with fluorescence microscope with the FITC/Evans Blue filter and the 40x objective.
Interpretation of Results
Positive: Enterovirus:
An green fluorescence.
Negative: Red cells with no apple-green fluorescence.
IV. Quality Control
Appropriate positive and negative control slides should be stained with each batch.
V. Reporting
See individual specimen protocols.
VI. Reference
Isenberg, H.D., 1992. Clinical Microbiology Procedures Handbook Vol. 2. ASM Press.
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BAHAN KULIAH DAN MAKALAH KESEHATAN : http://bahankuliahkesehatan.blogspot.com/2011/08/indirect-immunofluorescent-antibody-ifa.html