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乙型肝炎表面抗原变异体上存在的、可被抗乙型肝炎表面抗原单克隆抗体特异性识别的表位的定位。

Localization of hepatitis B surface antigen epitopes present on variants and specifically recognised by anti-hepatitis B surface antigen monoclonal antibodies.

作者信息

Jolivet-Reynaud C, Lésenéchal M, O'Donnell B, Becquart L, Foussadier A, Forge F, Battail-Poirot N, Lacoux X, Carman W, Jolivet M

机构信息

UMR 2142 bioMérieux/CNRS, CERVI, Lyon, France.

出版信息

J Med Virol. 2001 Oct;65(2):241-9. doi: 10.1002/jmv.2026.

DOI:10.1002/jmv.2026
PMID:11536229
Abstract

Small hepatitis B surface antigen (HBsAg) is considered to be the best marker for the diagnosis of Hepatitis B virus infection. However, HBsAg variants with mutations within the "a" determinant may be poorly or not detected by diagnostic assays. Three anti-HBsAg monoclonal antibodies (6H6B6, 27E7F10, and 2G2G10), directed against conformational epitopes, were tested for their ability to detect the wild-type HBsAg as well as variant forms and their respective epitopes were localised on the HBsAg sequence by using the phage-displayed peptide library technology. Whereas 6H6B6 did not detect mutations T123N, S143L, D144A and G145R, 27E7F10 binding was affected by mutations P120T and G145R. In contrast, 2G2G10 reacted strongly with all tested variants including variant with the G145R mutation. Part of the 6H6B6 epitope was located in the major hydrophilic region (MHR) at residues 101-105, the 27E7F10 epitope (residues 214-219) was located near the C-terminal end of the antigen and the 2G2G10 epitope at residues 199-208, within the theoretical fourth transmembrane helix. The 2G2G10 epitope localisation brings information about the HBsAg structure and the validity of established topological models. Finally, 2G2G10 is a valuable tool for HBsAg variant detection that is used as capture phase in a new bioMérieux diagnostic assay, which is currently in development.

摘要

小分子乙肝表面抗原(HBsAg)被认为是诊断乙肝病毒感染的最佳标志物。然而,“a”决定簇内发生突变的HBsAg变体可能无法被诊断检测方法很好地检测到或根本检测不到。针对构象表位的三种抗HBsAg单克隆抗体(6H6B6、27E7F10和2G2G10),被测试了检测野生型HBsAg以及变体形式的能力,并且利用噬菌体展示肽库技术将它们各自的表位定位在HBsAg序列上。6H6B6不能检测到T123N、S143L、D144A和G145R突变,27E7F10的结合受到P120T和G145R突变的影响。相比之下,2G2G10与所有测试变体包括具有G145R突变的变体都有强烈反应。6H6B6表位的一部分位于主要亲水区(MHR)的101 - 105位残基处,27E7F10表位(214 - 219位残基)位于抗原的C末端附近,而2G2G10表位位于199 - 208位残基处,在理论上的第四个跨膜螺旋内。2G2G10表位的定位为HBsAg结构以及已建立的拓扑模型的有效性提供了信息。最后,2G2G10是一种用于检测HBsAg变体的有价值工具,在目前正在研发的新生物梅里埃诊断检测方法中用作捕获阶段。

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