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Am. J. Biomed. Sci. 2014, 6(1), 20-31; doi: 10.5099/aj140100020 |
Sunil Kumar1, Sandeep Kumar1,
Yash Behl1 , Ravi Kumar Gupta2 |
1
Central Research Institute, Kasauli, H.P. India. |
2 Dept. of Microbiology, Panjab
University, Chandigarh. India |
*Corresponding Author |
Dr. Sunil Kumar |
Central Research Institute, |
Kasauli, Himachal Pradesh, |
India - 173204. |
Abstract In vivo neutralization assay is the only
accepted method for the potency testing of antisnake
venom serum (ASVS), till today. Due to non-availability of any other methods,
this assay is considered as gold standard for potency testing. However, it
requires large number of animals. There is an increasing need over the years to
develop an in vitro alternate method
so as to reduce/abolish the use of animals. Further, newer method may prove
less complicated, sensitive, less expensive and less laborious for potency
testing of antivenom. The present study was planned
to develop, standardize an ELISA assay for the potency testing of ASVS and to
validate its utility as a pre-screen test during commercial production. The
ELISA assay was standardized and validated critically and, was applied to test
the potency of purified anti Cobra venom serum and polyvalent ASVS. Different
variables were tested to determine optimal antigen–antibody concentrations,
antigen-coating conditions and the assay validation as per the WHO recommendations.
The ELISA assay was found to be specific and sensitive with marked
reproducibility. Further comparison of in
vitro and in vivo result
indicated that ELISA method can quantitate the anticobra Ig’s in the serum,
accurately as high degree of correlation >
0.9 was obtained between both the assays. The result suggests that ELISA
can be used as a pre-screen assay to the conventional in vivo assay during initial stages of antivenom
production. Keywords: Antisnake venom serum, ELISA, Cobra venom, Neutralization assay. Download the full article (PDF)
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