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通过体内雀麦花叶病毒的RNA重组剖析亚基因组启动子序列的需求:转录与重组功能分离的证据

Dissecting the requirement for subgenomic promoter sequences by RNA recombination of brome mosaic virus in vivo: evidence for functional separation of transcription and recombination.

作者信息

Wierzchoslawski Rafal, Dzianott Aleksandra, Bujarski Jozef

机构信息

Plant Molecular Biology Center, Department of Biological Sciences, Northern Illinois University, Montgomery Hall, De Kalb, IL 60115, USA.

出版信息

J Virol. 2004 Aug;78(16):8552-64. doi: 10.1128/JVI.78.16.8552-8564.2004.

Abstract

Previously, we and others mapped an increased homologous recombination activity within the subgenomic promoter (sgp) region in brome mosaic virus (BMV) RNA3. In order to correlate sgp-mediated recombination and transcription, in the present work we used BMV RNA3 constructs that carried altered sgp repeats. We observed that the removal or extension of the poly(U) tract reduced or increased recombination, respectively. Deletion of the sgp core hairpin or its replacement by a different stem-loop structure inhibited recombination activity. Nucleotide substitutions at the +1 or +2 transcription initiation position reduced recombination. The sgp core alone supported only basal recombination activity. The sites of crossovers mapped to the poly(U) region and to the core hairpin. The observed effects on recombination did not parallel those observed for transcription. To explain how both activities operate within the sgp sequence, we propose a dual mechanism whereby recombination is primed at the poly(U) tract by the predetached nascent plus strand, whereas transcription is initiated de novo at the sgp core.

摘要

此前,我们和其他研究人员绘制了雀麦花叶病毒(BMV)RNA3亚基因组启动子(sgp)区域内增强的同源重组活性图谱。为了关联sgp介导的重组和转录,在本研究中,我们使用了携带改变的sgp重复序列的BMV RNA3构建体。我们观察到,聚(U)序列的去除或延长分别降低或增加了重组。sgp核心发夹结构的缺失或被不同的茎环结构取代会抑制重组活性。转录起始位置+1或+2处的核苷酸替换会降低重组。单独的sgp核心仅支持基础重组活性。交叉位点定位于聚(U)区域和核心发夹结构。观察到的对重组的影响与转录中观察到的影响并不平行。为了解释这两种活性如何在sgp序列内发挥作用,我们提出了一种双重机制,即重组由预先分离的新生正链在聚(U)序列处引发,而转录则在sgp核心处从头起始。

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