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雀麦花叶病毒基因间RNA3复制信号与病毒复制蛋白1a共同作用,在体内显著稳定RNA。

A brome mosaic virus intergenic RNA3 replication signal functions with viral replication protein 1a to dramatically stabilize RNA in vivo.

作者信息

Sullivan M L, Ahlquist P

机构信息

Institute for Molecular Virology, University of Wisconsin-Madison, Madison, Wisconsin 53706, USA.

出版信息

J Virol. 1999 Apr;73(4):2622-32. doi: 10.1128/JVI.73.4.2622-2632.1999.

Abstract

Brome mosaic virus (BMV), a positive-strand RNA virus in the alphavirus-like superfamily, encodes two RNA replication proteins. The 1a protein has putative helicase and RNA-capping domains, whereas 2a contains a polymerase-like domain. Saccharomyces cerevisiae expressing 1a and 2a is capable of replicating a BMV RNA3 template produced by in vivo transcription of a DNA copy of RNA3. Although insufficient for RNA3 replication, the expression of 1a protein alone results in a dramatic and specific stabilization of the RNA3 template in yeast. As one step toward understanding 1a-induced stabilization of RNA3, the interactions involved, and its possible relation to RNA replication, we have identified the cis-acting sequences required for this effect. We find that 1a-induced stabilization is mediated by a 150- to 190-base segment of the RNA3 intergenic region corresponding to a previously identified enhancer of RNA3 replication. Moreover, this segment is sufficient to confer 1a-induced stability on a heterologous beta-globin RNA. Within this intergenic segment, partial deletions that inhibited 1a-induced stabilization in yeast expressing 1a alone resulted in parallel decreases in the levels of negative- and positive-strand RNA3 replication products in yeast expressing 1a and 2a. In particular, a small deletion encompassing a motif corresponding to the box B element of RNA polymerase III promoters dramatically reduced the ability of RNAs to respond to 1a or 1a and 2a. These and other findings suggest that 1a-induced stabilization likely reflects an early template selection step in BMV RNA replication.

摘要

雀麦花叶病毒(BMV)是类甲病毒超家族中的一种正链RNA病毒,编码两种RNA复制蛋白。1a蛋白具有推定的解旋酶和RNA加帽结构域,而2a蛋白含有类似聚合酶的结构域。表达1a和2a的酿酒酵母能够复制由RNA3的DNA拷贝经体内转录产生的BMV RNA3模板。虽然单独表达1a蛋白不足以进行RNA3复制,但它能显著且特异性地稳定酵母中的RNA3模板。为了进一步了解1a诱导的RNA3稳定作用、相关的相互作用及其与RNA复制的可能关系,我们确定了产生这种效应所需的顺式作用序列。我们发现,1a诱导的稳定作用是由RNA3基因间隔区150至190个碱基的片段介导的,该片段对应于先前鉴定的RNA3复制增强子。此外,该片段足以赋予异源β-珠蛋白RNA 1a诱导的稳定性。在这个基因间隔区内,单独在表达1a的酵母中抑制1a诱导的稳定作用的部分缺失,会导致在同时表达1a和2a的酵母中负链和正链RNA3复制产物水平的平行下降。特别是,一个包含与RNA聚合酶III启动子的B框元件相对应基序的小缺失显著降低了RNA对1a或1a和2a的反应能力。这些以及其他发现表明,1a诱导的稳定作用可能反映了BMV RNA复制中早期的模板选择步骤。

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