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天然和重组人着丝粒蛋白A自身抗原的分离与比较。

Isolation and comparison of natural and recombinant human CENP-A autoantigen.

作者信息

Martinez A, Sun D, Billings P B, Swiderek K M, Sullivan K F, Hoch S O

机构信息

The Agouron Institute, La Jolla, CA, 92037, USA.

出版信息

J Autoimmun. 1998 Dec;11(6):611-9. doi: 10.1006/jaut.1998.0249.

Abstract

Anticentromere antibodies (ACA) are associated with systemic sclerosis (scleroderma) patients exhibiting the more benign or so called limited manifestation of the disease (lSSc). ACA reactivity is directed against multiple polypeptide targets, the smallest of which is designated CENP-A. CENP-A is not an abundant cellular constituent; therefore to maximize recovery, we developed a protocol with a minimum of steps to isolate CENP-A from a human cell line. The trace cellular amount of this protein clearly dictated the production of its recombinant counterpart to facilitate determination of the role of the CENP-A antigen in scleroderma pathogenesis. Here we describe the eukaryotic expression of CENP-A cDNA using baculovirus-mediated infection of insect cells. The non-fusion recombinant protein spans the natural residues of the human CENP-A protein and rCENP-A followed the same chromotographic sequence for purification as did the natural source. The availability of the bona fide antigen provided a critical standard upon which to document authenticity of the recombinant polypeptide. The two forms of this antigen have been compared and shown to exhibit similar physical and antigenic properties.

摘要

抗着丝点抗体(ACA)与系统性硬化症(硬皮病)患者相关,这些患者表现出该疾病较为良性或所谓的局限性表现(局限性系统性硬化症,lSSc)。ACA反应针对多种多肽靶点,其中最小的被命名为着丝粒蛋白A(CENP - A)。CENP - A并非细胞中的丰富成分;因此,为了最大程度地提高回收率,我们开发了一种步骤最少的方案,用于从人细胞系中分离CENP - A。这种蛋白质在细胞中的微量存在明确决定了其重组对应物的产生,以促进确定CENP - A抗原在硬皮病发病机制中的作用。在此,我们描述了使用杆状病毒介导的昆虫细胞感染来真核表达CENP - A cDNA。非融合重组蛋白涵盖了人CENP - A蛋白的天然残基,并且重组CENP - A(rCENP - A)的纯化色谱序列与天然来源相同。这种真正抗原的可得性为证明重组多肽的真实性提供了关键标准。已对该抗原的两种形式进行了比较,并显示出相似的物理和抗原特性。

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