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利用截短和突变衣壳蛋白的交联二聚体进行辛德毕斯病毒核心样颗粒的体外组装。

In vitro assembly of Sindbis virus core-like particles from cross-linked dimers of truncated and mutant capsid proteins.

作者信息

Tellinghuisen T L, Perera R, Kuhn R J

机构信息

Department of Biological Sciences, Purdue University, West Lafayette, Indiana 47907, USA.

出版信息

J Virol. 2001 Mar;75(6):2810-7. doi: 10.1128/JVI.75.6.2810-2817.2001.

Abstract

A nucleic acid-bound capsid protein dimer was previously identified using a Sindbis virus in vitro nucleocapsid assembly system and cross-linking reagents. Cross-link mapping, in combination with a model of the nucleocapsid core, suggested that this dimer contained one monomer from each of two adjacent capsomeres. This intercapsomere dimer is believed to be the initial intermediate in the nucleocapsid core assembly mechanism. This paper presents the purification of cross-linked dimers of a truncated capsid protein and the partial purification of cross-linked dimers of a full-length assembly-defective mutant. The assembly of core-like particles from these cross-linked capsid protein dimers is demonstrated. Core-like particles generated from cross-linked full-length mutant CP(19-264)L52D were examined by electron microscopy and appeared to have a morphology similar to that of wild-type in vitro-assembled core-like particles, although a slight size difference was often visible. Truncated cross-linked CP(81-264) dimers generated core-like particles as well. These core-like particles could subsequently be disassembled when reversible cross-linking reagents were used to form the dimers. The ability of the covalent intercapsomere cross-link to rescue capsid proteins with assembly defects or truncations in the amino-terminal region of the capsid protein supports the previous model of assembly and suggests a possible role for the amino-terminal region of the protein.

摘要

先前利用辛德毕斯病毒体外核衣壳组装系统和交联试剂鉴定出一种与核酸结合的衣壳蛋白二聚体。交联图谱与核衣壳核心模型相结合,表明这种二聚体包含来自两个相邻衣壳粒的各一个单体。这种衣壳粒间二聚体被认为是核衣壳核心组装机制中的初始中间体。本文介绍了截短衣壳蛋白交联二聚体的纯化以及全长组装缺陷型突变体交联二聚体的部分纯化。证明了由这些交联衣壳蛋白二聚体组装成类核心颗粒。通过电子显微镜检查了由交联的全长突变体CP(19 - 264)L52D产生的类核心颗粒,其形态似乎与野生型体外组装的类核心颗粒相似,尽管通常可见轻微的大小差异。截短的交联CP(81 - 264)二聚体也产生了类核心颗粒。当使用可逆交联试剂形成二聚体时,这些类核心颗粒随后可以被拆解。衣壳粒间共价交联拯救衣壳蛋白中存在组装缺陷或衣壳蛋白氨基末端区域截短的能力支持了先前的组装模型,并表明了该蛋白氨基末端区域可能的作用。

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本文引用的文献

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Cold Spring Harb Symp Quant Biol. 1962;27:1-24. doi: 10.1101/sqb.1962.027.001.005.
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