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噬菌体展示技术在鉴定疾病早期被识别的丙型肝炎病毒NS4A表位中的应用。

Usefulness of the phage display technology for the identification of a hepatitis C virus NS4A epitope recognized early in the course of the disease.

作者信息

Ferrieu-Weisbuch Catherine, Bettsworth Florence, Becquart Laurence, Paranhos-Baccala Glaucia, Michel Sandrine, Arnaud Michel, Jolivet-Reynaud Colette

机构信息

Unité Mixte de Recherche UMR 2714 CNRS-bioMérieux, IFR 128 BioSciences Lyon Gerland, 21 avenue Tony Garnier, 69365 Lyon Cedex 07, France.

出版信息

J Virol Methods. 2006 Feb;131(2):175-83. doi: 10.1016/j.jviromet.2005.08.008. Epub 2005 Sep 23.

DOI:10.1016/j.jviromet.2005.08.008
PMID:16183141
Abstract

A dodecapeptide phage-displayed library was screened with the mouse monoclonal antibody (mAb) 2E3C2 which competed with human antibodies for the binding to the HCV c100 recombinant protein. Four mimotopes shared a consensus motif with the HCV 1701-1707 sequence corresponding to the carboxyl-terminal domain of the non-structural protein NS4A. However, these mimotopes reacted with 2E3C2 only, whereas the corresponding NS4 epitope defined at the sequence 1698-1709 and displayed on phage was recognized by both 2E3C2 and sera from HCV infected patients. Using the Spot method of multiple peptide synthesis and alanine replacement analysis, the respective reactivities of mAb 2E3C2 and anti-NS4A human antibodies against NS4 were shown to be directed against two slightly different overlapping minimal linear sequences and to involve different critical residues. The phage clone displaying the NS4 epitope was used to study the specific recognition of this epitope by different individual HCV positive sera as well as by two seroconversion panels of sera from HCV infected patients. Compared with the detection by RIBA of the different HCV antigens and c100 particularly, these results indicated that the antibodies directed against the NS4 (1698-1709) epitope were produced early during the course of the disease and decreased later.

摘要

用与人类抗体竞争结合丙型肝炎病毒(HCV)c100重组蛋白的小鼠单克隆抗体(mAb)2E3C2筛选了一个十二肽噬菌体展示文库。四个模拟表位与HCV 1701 - 1707序列具有共同基序,该序列对应于非结构蛋白NS4A的羧基末端结构域。然而,这些模拟表位仅与2E3C2反应,而在噬菌体上展示的、在序列1698 - 1709处定义的相应NS4表位可被2E3C2和HCV感染患者的血清识别。使用多聚肽合成的斑点法和丙氨酸置换分析,结果显示mAb 2E3C2和抗NS4A人类抗体对NS4的各自反应性针对两个略有不同的重叠最小线性序列,并涉及不同的关键残基。展示NS4表位的噬菌体克隆用于研究不同个体HCV阳性血清以及来自HCV感染患者的两个血清转化组对该表位的特异性识别。特别是与通过重组免疫印迹分析(RIBA)检测不同HCV抗原尤其是c100相比,这些结果表明针对NS4(1698 - 1709)表位的抗体在疾病过程早期产生,随后减少。

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