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质粒pSC101的一个必需复制基因repA受到自身调控。

An essential replication gene, repA, of plasmid pSC101 is autoregulated.

作者信息

Linder P, Churchward G, Xia G X, Yu Y Y, Caro L

出版信息

J Mol Biol. 1985 Feb 5;181(3):383-93. doi: 10.1016/0022-2836(85)90227-x.

Abstract

Measurements of the rate of replication of a mutant pSC101 plasmid, cloned into a ColE1 vector, showed that insertions of the transposon Tn1000 into the repA gene of pSC101 abolished replication activity, but could be complemented in trans, albeit at a low level. The promoter of the repA gene was mapped by the construction of repA-lacZ gene fusions, and one of the fusions was used to demonstrate that repA protein, provided in trans, could repress expression of beta-galactosidase activity. This repression was primarily due to reduction of transcription of the repA-lacZ fusion. The sequence analysis of mutants of the repA-lacZ fusion gene which were no longer sensitive to the presence of repA protein showed that the site of action of repA was a 22 base-pair sequence, present as an inverted repeat, overlapping the repA promoter. The repA gene is thus autoregulated.

摘要

对克隆到ColE1载体中的突变型pSC101质粒复制速率的测量表明,将转座子Tn1000插入pSC101的repA基因会消除复制活性,但可以通过反式互补,尽管水平较低。通过构建repA-lacZ基因融合体来定位repA基因的启动子,并且其中一个融合体用于证明反式提供的repA蛋白可以抑制β-半乳糖苷酶活性的表达。这种抑制主要是由于repA-lacZ融合体转录的减少。对不再对repA蛋白的存在敏感的repA-lacZ融合基因突变体的序列分析表明,repA的作用位点是一个22个碱基对的序列,以反向重复形式存在,与repA启动子重叠。因此,repA基因是自我调节的。

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