dc.contributor.author |
Athapaththu, A.M.M.H. |
|
dc.contributor.author |
Khanna, N. |
|
dc.contributor.author |
Inouve, S. |
|
dc.contributor.author |
Gunasena, S. |
|
dc.contributor.author |
Abeyewickreme, W. |
|
dc.contributor.author |
Hapugoda, M. |
|
dc.date.accessioned |
2016-05-31T05:14:59Z |
|
dc.date.available |
2016-05-31T05:14:59Z |
|
dc.date.issued |
2013 |
|
dc.identifier.citation |
The Bulletin of the Sri Lanka College of Microbiologists. 2013; 11(1): 15 |
en_US |
dc.identifier.issn |
1391-930x |
|
dc.identifier.uri |
http://repository.kln.ac.lk/handle/123456789/13311 |
|
dc.description |
Oral Presentation (OP 13) The bulletin of the Sri Lanka College of Microbiologists, 24rd-26th July 2013, Colombo |
en_US |
dc.description.abstract |
INTRODUCTION AND OBJECTIVE: Laboratory confirmation of Chikungunya (CHIK) virus is very useful as clinical symptoms of CHIK can overlap with other diseases. Chikungunya virus specific antigen, which shows high specificity, sensitivity and low cross reactivity with other related diseases, is required for laboratory confirmation. Objective of this study was to develop and compare two recombinant protein antigens for detection of anti-CHIK antibodies. DESIGN, SETTING AND METHODS: Recombinant CHIK protein antigens were prepared using Envelope (E1 and E2) regions of the CHIK virus. The genes were custom designed and chemically synthesized with a 6X His tag. Bacterial expression systems [BL21 (DE3)] were used to clone and express the recombinant proteins. The recombinant proteins were purified with >95% of purity per liter of culture using Ni-NTA columns under denature conditions. In this study, two antigens were evaluated for detection of anti-CHIK antibody by using novel optimized in-house IgM and IgG ELISAs, using a panel of well characterized serum samples obtained from the Dept. of Virology (WHO Reference Center for Viral Reference and Research) Institute of Tropical Medicine, Nagasaki University, Japan. RESULTS: Atotal of 55 serum samples confirmed as positives and 186 confirmed as negatives by HA! test, IgM capture ELISA and indirect IgG ELISA using the purified CHIK antigen were used to evaluate the antigens using novel IgM ELISA. A total of 78 serum samples confirmed as positives and 148 (E1) or 227 (E2) (148 + extra 79) confirmed ac negatives were used to evaluate the antigens using novel IgG ELISA. The E1 recombinant protein showed 5% (3/ 55) sensitivity and 99% (184/186) specificity for IgM ELISA and 60% (47/78) sensitivity and 63% (94/148) specificity for IgG ELISA. The E2 recombinant protein showed 65% (36/55) sensitivity and 70% (131/186) specificity for IgM ELISA and 83% (65/78) sensitivity and 86% (195/227) specificity for IgG ELISA. CONCLUSION: Recombinant CHIK-E2 protein antigen showed higher specificity and sensitivity in detection of both IgM and IgG antibodies. Thus the E2 recombinant protein antigen used in this study could be expressed in an eukaryotic expression system to achieve much higher results. ACKNOWLEDGMENT: International Center for Genetic Engineering and Biotechnology (ICGEB CRP SRL 08/02), National Science Foundation (NSF/RG/2009/BT/01) and International Atomic Energy Authority (lAEA/SRL/5/042) are gratefully acknowledged. |
en_US |
dc.language.iso |
en_US |
en_US |
dc.publisher |
Sri Lanka College of Microbiologists |
en_US |
dc.subject |
protein antigens |
en_US |
dc.title |
Development of recombinant protein antigens using a bacterial expression system for the detection of anti-Chikungunya (CHIK) antibodies |
en_US |
dc.type |
Article |
en_US |