摘要
In order to enhance the sensitivity of diagnosis, a recombinant clone containing domain I of HCV core (amino acid residues 1 to 123) was subjected to random mutagenesis. Five mutants with higher sensitivity were obtained by colony screening of 616 mutants using reverse ELISA. Sequence analysis of these mutants revealed alterations focusing on W 84, P 95, P 110, or V 129. The inclusion bodies of these recombinant proteins overexpressed in E. coli BL21(DE3) were subsequently dissolved using 6 M urea and then refolded by stepwise dialysis. Compared to the unfolded wild-type antigen, the refolded M3b antigen (W 84S, P 110S and V 129L) exhibited an increase of 66% antigenicity with binding capacity of 0.96 and affinity of 113 μM -1. Moreover, the 33% decrease of the production demand suggests that M3b is a potential substitute for anti-HCV antibody detection.
原文 | 英語 |
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文章編號 | 359042 |
期刊 | Journal of Biomedicine and Biotechnology |
卷 | 2011 |
DOIs | |
出版狀態 | 已出版 - 2011 |
對外發佈 | 是 |