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戊型肝炎病毒中和表位的鉴定与特性分析

Identification and characterization of the neutralization epitope(s) of the hepatitis E virus.

作者信息

Meng J, Dai X, Chang J C, Lopareva E, Pillot J, Fields H A, Khudyakov Y E

机构信息

Division of Viral Hepatitis, National Center for Infectious Diseases, Centers for Disease Control and Prevention, Atlanta, Georgia 30333, USA.

出版信息

Virology. 2001 Sep 30;288(2):203-11. doi: 10.1006/viro.2001.1093.

DOI:10.1006/viro.2001.1093
PMID:11601892
Abstract

The neutralization epitope(s) of the hepatitis E virus (HEV) was studied by an in vitro neutralization assay using antibodies obtained by immunization of mice with 51 overlapping 30-mer synthetic peptides spanning the region 221-660 amino acids (aa) of the HEV open reading frame 2 encoded protein (pORF2) and 31 overlapping recombinant proteins of different sizes derived from the entire pORF2 of the HEV Burma strain. Antibodies against synthetic peptides and short recombinant proteins of approximately 100 aa did not neutralize HEV, suggesting the HEV neutralization epitope(s) is conformation-dependent. However, one recombinant protein of approximately 400 aa in length comprising the pORF2 sequence at position 274-660 aa as well as all truncated derivatives of this protein containing region 452-617 aa elicited antibodies, demonstrating HEV neutralizing activity. These findings establish for the first time that the minimal size fragment, designated pB166, that can efficiently model the neutralization epitope(s) is 166 aa in length and is located at position 452-617 aa of the HEV pORF2. Additionally, antibodies against pB166 were found to cross-neutralize three different HEV genotypes, suggesting that a common neutralization epitope(s) may exist within the different HEV genotypes. Thus, recombinant proteins constructed in this study may be considered as potential candidates for the development of an HEV subunit vaccine as well as for the development of highly sensitive and specific diagnostic tests.

摘要

通过体外中和试验研究戊型肝炎病毒(HEV)的中和表位,该试验使用的抗体是通过用51个重叠的30肽合成肽免疫小鼠获得的,这些合成肽跨越HEV开放阅读框2编码蛋白(pORF2)的221 - 660个氨基酸(aa)区域,以及31个来自HEV缅甸株整个pORF2的不同大小的重叠重组蛋白。针对合成肽和大约100个aa的短重组蛋白的抗体不能中和HEV,这表明HEV中和表位是构象依赖性的。然而,一种长度约为400个aa的重组蛋白,包含pORF2序列中274 - 660个aa的位置以及该蛋白所有包含452 - 617个aa区域的截短衍生物可引发抗体,证明具有HEV中和活性。这些发现首次确定了能够有效模拟中和表位的最小片段,命名为pB166,其长度为166个aa,位于HEV pORF2的452 - 617个aa位置。此外,发现针对pB166的抗体可交叉中和三种不同的HEV基因型,这表明不同HEV基因型中可能存在共同的中和表位。因此,本研究构建的重组蛋白可被视为开发HEV亚单位疫苗以及高灵敏度和特异性诊断测试的潜在候选物。

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