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丁型肝炎抗原免疫显性区域的克隆与表达

Cloning and expression of an immunodominant region of the hepatitis delta antigen.

作者信息

Saldanha J, Homer E, Goldin R, Thomas H C, Monjardino J

机构信息

Department of Medicine, St Mary's Hospital Medical School, London, U.K.

出版信息

J Gen Virol. 1990 Feb;71 ( Pt 2):471-5. doi: 10.1099/0022-1317-71-2-471.

Abstract

A cDNA clone prepared from hepatitis delta virus (HDV) RNA extracted from human serum was subcloned in the bacterial expression vector pPL31 to produce a fusion protein consisting of the first 98 amino acids of MS2 polymerase and of 64 amino acids from near the N-terminal region of hepatitis delta antigen (HDAg). The fusion protein was shown to be related to HDAg by a commercial sandwich immunoassay (Abbott) and immunoblotting with human anti-HDAg serum. Antiserum against the fusion protein was raised in rabbits and used to identify HDAg extracted from the serum and liver of an HDV-infected woodchuck and chimpanzee and from the serum of an HDV-infected human, by immunoblotting and immunohistology. A single, major polypeptide of 24K was detected in both serum and liver extracts, with a minor polypeptide of 26K sometimes present. Liver extracts also contained lower Mr polypeptides thought to be degradation products, the major species being 22.5K. The same pattern of staining was obtained with human anti-HDAg serum. Absorption experiments with the expressed protein and cross-competition experiments with the rabbit antiserum suggest that a major immunodominant region of HDAg is present near the N-terminal end of the antigen, between positions 1561 and 1368 on the genome. Both the expressed protein and rabbit antiserum were shown to be good diagnostic reagents.

摘要

从人血清中提取的丁型肝炎病毒(HDV)RNA制备的cDNA克隆,被亚克隆到细菌表达载体pPL31中,以产生一种融合蛋白,该融合蛋白由MS2聚合酶的前98个氨基酸和来自丁型肝炎抗原(HDAg)N端区域附近的64个氨基酸组成。通过商业夹心免疫测定法(雅培)和用人抗HDAg血清进行免疫印迹,显示该融合蛋白与HDAg相关。用该融合蛋白免疫家兔制备抗血清,并通过免疫印迹和免疫组织化学法,用于鉴定从感染HDV的土拨鼠和黑猩猩的血清及肝脏以及感染HDV的人类血清中提取的HDAg。在血清和肝脏提取物中均检测到一条单一的主要24K多肽,有时还存在一条次要的26K多肽。肝脏提取物中还含有较低分子量的多肽,被认为是降解产物,主要种类为22.5K。用人抗HDAg血清也获得了相同的染色模式。用表达的蛋白进行吸收实验以及用兔抗血清进行交叉竞争实验表明,HDAg的一个主要免疫显性区域存在于抗原的N端附近,在基因组上的1561位和1368位之间。表达的蛋白和兔抗血清均被证明是良好的诊断试剂。

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