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原发性胆汁性肝硬化患者自身抗体主要识别的一种人类核抗原的cDNA的分离与鉴定

Isolation and characterization of cDNA encoding a human nuclear antigen predominantly recognized by autoantibodies from patients with primary biliary cirrhosis.

作者信息

Szostecki C, Guldner H H, Netter H J, Will H

机构信息

Max-Planck-Institut für Biochemie, Martinsried, Federal Republic of Germany.

出版信息

J Immunol. 1990 Dec 15;145(12):4338-47.

PMID:2258622
Abstract

Autoantibodies to a novel nuclear Ag, Sp100, have recently been described that recognize a nuclear protein with an apparent molecular mass of 95 to 100 kDa and a dot-like distribution within cell nuclei. By immunoscreening of a lambda gt11 cDNA expression library derived from HeLa cells with an anti-Sp100 autoimmune serum a 0.7-kb cDNA (Sp26) coding for a fragment of Sp100 was isolated. Expression of this cDNA and use of the recombinant protein in ELISA revealed that the fragment carries major Sp100 autoepitopes and that anti-Sp100 autoantibodies predominantly occur in patients suffering from primary biliary cirrhosis (50/184). The Sp26 cDNA was used as hybridization probe for isolation of longer cDNA from human liver- and placenta-derived lambda gt10 cDNA libraries. Overlapping fragments were assembled to generate a full length cDNA coding for a protein with a molecular mass of 53 kDa and an isoelectric point of 4.7. The Sp100 autoantigen expressed in vitro from this cDNA and authenticated by a capture immunoblot assay, comigrated in SDS-PAGE with the authentic HeLa autoantigen of 95 to 100 kDa and thus showed an aberrant electrophoretic mobility. Computer based protein sequence analysis of the Sp100 autoantigen revealed regions of striking sequence similarities to the alpha 1 and alpha 2 domains of various human and non-human MHC class I Ag and to several transacting transcriptional regulatory proteins.

摘要

最近发现了针对一种新型核抗原Sp100的自身抗体,该抗体可识别一种表观分子量为95至100 kDa的核蛋白,其在细胞核内呈点状分布。用抗Sp100自身免疫血清对来自HeLa细胞的λgt11 cDNA表达文库进行免疫筛选,分离出一个编码Sp100片段的0.7 kb cDNA(Sp26)。该cDNA的表达以及重组蛋白在ELISA中的应用表明,该片段携带主要的Sp100自身抗原表位,且抗Sp100自身抗体主要出现在原发性胆汁性肝硬化患者中(50/184)。Sp26 cDNA用作杂交探针,从人肝脏和胎盘来源的λgt10 cDNA文库中分离出更长的cDNA。将重叠片段组装起来,生成一个编码分子量为53 kDa、等电点为4.7的蛋白质的全长cDNA。从该cDNA体外表达并经捕获免疫印迹分析鉴定的Sp100自身抗原,在SDS-PAGE中与95至100 kDa的HeLa真实自身抗原共迁移,因此显示出异常的电泳迁移率。对Sp100自身抗原进行基于计算机的蛋白质序列分析,发现其与多种人类和非人类MHC I类抗原的α1和α2结构域以及几种反式作用转录调节蛋白存在显著的序列相似区域。

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