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首页> 外文期刊>Molecular Microbiology >Antisense RNA-mediated transcriptional attenuation: an in vitro study of plasmid pT181.
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Antisense RNA-mediated transcriptional attenuation: an in vitro study of plasmid pT181.

机译:反义RNA介导的转录减弱:质粒pT181的体外研究。

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摘要

Antisense RNAs regulate plasmid replication by several different mechanisms. One of these mechanisms, transcriptional attenuation, was first described for the staphylococcal plasmid pT181, and later for the streptococcal plasmids pIP501 and pAMbeta1. Previously, we performed detailed in vitro and in vivo analyses of the pIP501 system. Here, we present an in vitro analysis of the antisense system of plasmid pT181. The secondary structures of antisense and sense RNA species of different lengths were determined. Binding rate constants for sense/antisense RNA pairs were measured, and functional segments required for complex formation were determined. A single-round transcription assay was used for in vitro analysis of transcriptional attenuation. A comparison between pT181 and pIP501 revealed several differences; whereas a truncated derivative of pIP501 antisense RNA was sufficient for stable complex formation, both stem-loop structures of pT181-RNAI were required. In contrast to the sense RNA of pIP501, which showed an intrinsic propensity to terminate (30-50% in the absence of antisense RNA), the sense RNA of pT181 required antisense RNA for induced termination. Rate constants of formation of pT181 sense-antisense RNA complexes were similar to inhibition rate constants, in striking contrast to pIP501, in which inhibition occurred at least 10-fold faster than stable binding.
机译:反义RNA通过几种不同的机制调节质粒复制。首先针对葡萄球菌质粒pT181描述了这些机制之一,即转录衰减,随后针对链球菌质粒pIP501和pAMbeta1进行了描述。以前,我们对pIP501系统进行了详细的体外和体内分析。在这里,我们提出了质粒pT181反义系统的体外分析。确定了不同长度的反义和有义RNA物种的二级结构。测量有义/反义RNA对的结合速率常数,并确定复合物形成所需的功能区段。单轮转录测定用于体外转录衰减分析。 pT181和pIP501的比较显示出一些差异。 pIP501反义RNA的截短衍生物足以稳定形成复合物,而pT181-RNAI的两个茎环结构都是必需的。与pIP501的有义RNA表现出固有的终止倾向(在不存在反义RNA的情况下为30-50%)相反,pT181的有义RNA需要反义RNA才能诱导终止。 pT181有义反义RNA复合物形成的速率常数类似于抑制速率常数,与pIP501形成鲜明对比,在pIP501中,抑制发生的速度至少比稳定结合快10倍。

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