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通过将外壳蛋白体外组装到双链RNA噬菌体phi 6的聚合酶复合物上产生感染性核衣壳。

Generation of infectious nucleocapsids by in vitro assembly of the shell protein on to the polymerase complex of the dsRNA bacteriophage phi 6.

作者信息

Olkkonen V M, Ojala P M, Bamford D H

机构信息

Department of Genetics, University of Helsinki, Finland.

出版信息

J Mol Biol. 1991 Apr 5;218(3):569-81. doi: 10.1016/0022-2836(91)90702-8.

Abstract

A method for the in vitro uncoating of the phi 6 nucleocapsid (NC) was developed. The resulting particle, designated as the NC core, containing the genomic double-stranded (ds) RNA segments and the proteins P1, P2, P4 and P7, was not infectious but had a highly enhanced in vitro transcriptase activity compared to that of the intact NC. The NC shell protein P8 was purified by immunoaffinity chromatography, and it was shown to self-assemble to shell-like structures upon addition of calcium ions. The conditions for the self-assembly of the shell were optimized. Shell reassembly on to the NC cores restored the infectivity but resulted in a decrease of transcriptase activity. No reassembly of the shell on to RNA-less cores (procapsids) produced from a cDNA construction in Escherichia coli was observed. Our results suggest that the intracellular uncoating of the NC is the event activating the phi 6 dsRNA transcriptase and that the NC shell is necessary for infectivity, probably for the passage of the NC through the host cytoplasmic membrane. Packaging of the dsRNA segments into the procapsid appears to be a prerequisite for NC shell assembly.

摘要

开发了一种用于体外解开φ6核衣壳(NC)的方法。所得颗粒,命名为NC核心,包含基因组双链(ds)RNA片段以及蛋白质P1、P2、P4和P7,不具有感染性,但与完整的NC相比,其体外转录酶活性显著增强。通过免疫亲和层析纯化了NC壳蛋白P8,结果表明,添加钙离子后,它能自组装成壳状结构。优化了壳自组装的条件。壳重新组装到NC核心上恢复了感染性,但导致转录酶活性降低。未观察到壳重新组装到由大肠杆菌中的cDNA构建产生的无RNA核心(原衣壳)上。我们的结果表明,NC在细胞内的解壳是激活φ6 dsRNA转录酶的事件,并且NC壳对于感染性是必需的,可能是为了使NC穿过宿主细胞质膜。将dsRNA片段包装到原衣壳中似乎是NC壳组装的先决条件。

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