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质粒R1复制的控制:反义RNA CopA与其靶标CopT之间体外相互作用的动力学

Control of replication of plasmid R1: kinetics of in vitro interaction between the antisense RNA, CopA, and its target, CopT.

作者信息

Persson C, Wagner E G, Nordström K

机构信息

Department of Microbiology, University of Uppsala, Sweden.

出版信息

EMBO J. 1988 Oct;7(10):3279-88. doi: 10.1002/j.1460-2075.1988.tb03195.x.

Abstract

The frequency of replication of IncFII plasmids is regulated by the availability of a rate-limiting protein, RepA. This protein acts to promote initiation of replication and its synthesis is negatively controlled both at the transcriptional and translational level. The translational control is exerted by the binding of a small antisense RNA, CopA RNA, to its target, CopT, which is located in the leader region of the RepA mRNA. As a consequence, formation of RepA is inhibited. Here we demonstrate the binding of CopA RNA to CopT RNA in vitro; the rate constant of binding was determined to be approximately 1 X 10(6) M-1 s-1 at 37 degrees C. We have also shown that in vitro synthesized RepA mRNA molecules differing in length, but which contain the whole CopT region, are able to bind CopA RNA with similar rates. Analysis of the binding of CopA/CopT molecules derived from a copy-number mutant plasmid showed that the effect of the mutation on the rate of in vitro binding correlates well with its phenotypic effect in vivo, i.e. the binding rate constant is lowered in proportion to the increase in copy number. Likewise, the result of an in vitro incompatibility test is in agreement with in vivo data.

摘要

IncFII质粒的复制频率受一种限速蛋白RepA可用性的调节。该蛋白促进复制起始,其合成在转录和翻译水平均受到负调控。翻译控制是通过一种小反义RNA(CopA RNA)与其靶标CopT结合来实现的,CopT位于RepA mRNA的前导区。结果,RepA的形成受到抑制。在此我们证明了CopA RNA在体外与CopT RNA的结合;在37℃下,结合速率常数测定约为1×10⁶ M⁻¹ s⁻¹。我们还表明,体外合成的长度不同但包含整个CopT区域的RepA mRNA分子,能够以相似速率结合CopA RNA。对来自拷贝数突变体质粒的CopA/CopT分子结合情况的分析表明,突变对体外结合速率的影响与其在体内的表型效应密切相关,即结合速率常数随拷贝数增加而成比例降低。同样,体外不相容性测试结果与体内数据一致。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/ed37/454754/f5e70e0e83ca/emboj00147-0322-a.jpg

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