| 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.D. |
|
| dc.date.accessioned |
2016-05-24T04:31:34Z |
|
| dc.date.available |
2016-05-24T04:31:34Z |
|
| dc.date.issued |
2011 |
|
| dc.identifier.citation |
The Bulletin of the Sri Lanka College of Microbiologists. 2011; 09(1): 16 |
en_US |
| dc.identifier.issn |
1391-930x |
|
| dc.identifier.uri |
http://repository.kln.ac.lk/handle/123456789/13184 |
|
| dc.description |
Oral Presentation (OP 6) The bulletin of the Sri Lanka College of Microbiologists, 04th-16th September 2011, Colombo |
en_US |
| dc.description.abstract |
INTRODUCTION: Chikungunya (CHIK) virus specific antigen which has high specificity and low cross reactivity with other related diseases is required for laboratory confirmation. OBJECTIVE: To compare two antigens for detection of anti-CHIK antibody. DESIGN, SETTING AND METHODS: In this study, two antigens {viral cell lysate and recombinant protein) were evaluated for detection of anti-1 CH IK antibody by using IgM ELISA. A novel recombinant | protein antigen was designed based on envelope domain, a critical antigenic region of the major structural protein, I This protein was expressed in Escherichia coli and resultant protein was affinity purified and ~10mg with >95% of purity per liter of culture was obtained. Cell lysate antigen was prepared using a crude culture fluid. Two antigens were evaluated separately using a panel of well characterized serum samples obtained from the Dept. of Virology (WHO Reference Centre for Viral Reference and Research), Institute of Tropical Medicine,] Nagasaki University. RESULTS: Atotal of 64 serum samples confirmed as positives andl 22 confirmed as negatives were used to evaluate the antigens. Specificity and sensitivity of the recombinant protein antigen was 48% and 90% respectively. Specificity and sensitivity of the viral lysate antigen was] 17% and 100% respectively. Conclusion Viral lysate antigens can cause biohazard risk, high production cost and cross reactivity with other organisms of the same genus/family. Recombinant protein antigen which shows high specificity and sensitivity used in this study is important to overcome problems associated with viral lysate antigen. Testing of a large number of samples is needed to reconfirm this finding. ACKNOWLEDGMENT: Financial assistance and technical co-operation by 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 (IAEA/SRL/5/042) is acknowledged. |
en_US |
| dc.language.iso |
en_US |
en_US |
| dc.publisher |
Sri Lanka College of Microbiologists |
en_US |
| dc.subject |
chikungunya |
en_US |
| dc.title |
Comparison of recombinant protein and cell lysate antigens for detection of anti-chikungunya (CHIK) IgM antibody |
en_US |
| dc.type |
Article |
en_US |