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在两个不同的噬菌体φ29启动子处转录的激活和抑制是由调节蛋白p4的相同残基与RNA聚合酶的相互作用介导的。

Activation and repression of transcription at two different phage phi29 promoters are mediated by interaction of the same residues of regulatory protein p4 with RNA polymerase.

作者信息

Monsalve M, Mencia M, Rojo F, Salas M

机构信息

Centro de Biología Molecular Severo Ochoa (CSIC- UAM), Universidad Autónoma, Madrid, Spain.

出版信息

EMBO J. 1996 Jan 15;15(2):383-91.

Abstract

Phage phi29 regulatory protein p4 activates transcription from the late A3 promoter and represses the main early promoters, named A2b and A2c. Activation involves stabilization of RNA polymerase (RNAP) at the A3 promoter as a closed complex and is mediated by interaction between RNAP and a small domain of protein p4 in which residue Arg120 plays an essential role. We show that protein p4 represses the A2c promoter by binding to DNA immediately upstream from RNAP in a way that does not hinder RNAP binding; rather, the two proteins bind cooperatively to DNA. In the presence of protein p4, RNAP can form an initiated complex at the A2c promoter that generates short abortive transcripts, but cannot leave the promoter. Mutation of protein p4 residue Arg120, which relieves the contact between the two proteins, leads to a loss of repression. Therefore, the contact between protein p4 and RNAP through the protein p4 domain containing Arg120 can activate or repress transcription, depending on the promoter. The relative position of protein p4 and RNAP, which is different at each promoter, together with the distinct characteristics of the two promoters, may determine whether protein p4 activates or represses transcription.

摘要

噬菌体φ29调控蛋白p4激活晚期A3启动子的转录,并抑制主要的早期启动子,即A2b和A2c。激活过程涉及RNA聚合酶(RNAP)以封闭复合物形式稳定在A3启动子上,并且由RNAP与蛋白p4的一个小结构域之间的相互作用介导,其中精氨酸120残基起着至关重要的作用。我们发现,蛋白p4通过以一种不妨碍RNAP结合的方式结合到RNAP上游紧邻的DNA上来抑制A2c启动子;相反,这两种蛋白协同结合到DNA上。在蛋白p4存在的情况下,RNAP可以在A2c启动子处形成起始复合物,该复合物产生短的流产转录本,但无法离开启动子。蛋白p4精氨酸120残基的突变消除了这两种蛋白之间的接触,导致抑制作用丧失。因此,通过含有精氨酸120的蛋白p4结构域,蛋白p4与RNAP之间的接触可以激活或抑制转录,这取决于启动子。蛋白p4和RNAP在每个启动子处的相对位置不同,再加上两个启动子的不同特性,可能决定蛋白p4是激活还是抑制转录。

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