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pPS10质粒复制的负调控:通过拉链式结合DNA的RepA单体进行起始点配对

Negative regulation of pPS10 plasmid replication: origin pairing by zipping-up DNA-bound RepA monomers.

作者信息

Gasset-Rosa Fátima, Díaz-López Teresa, Lurz Rudi, Prieto Alicia, Fernández-Tresguerres M Elena, Giraldo Rafael

机构信息

Department of Molecular Microbiology, Centro de Investigaciones Biológicas-CSIC, Madrid, Spain.

出版信息

Mol Microbiol. 2008 May;68(3):560-72. doi: 10.1111/j.1365-2958.2008.06166.x. Epub 2008 Feb 19.

Abstract

In many plasmid replicons of gram-negative bacteria, Rep protein dimers are transcriptional self-repressors of their genes, whereas monomers are initiators of DNA replication. Switching between both functions implies conformational remodelling of Rep, and is promoted by Rep binding to the origin DNA repeats (iterons) or chaperones. Rep proteins play another key role: they bridge together two iteron DNA stretches, found either on the same or on different plasmid molecules. These so-called, respectively, 'looped' and 'handcuffed' complexes are thought to be negative regulators of plasmid replication. Although evidence for Rep-dependent plasmid handcuffing has been found in a number of replicons, the structure of these Rep-DNA assemblies is still unknown. Here, by a combination of proteomics, electron microscopy, genetic analysis and modelling, we provide insight on a possible three-dimensional structure for two handcuffed arrays of the iterons found at the origin of pPS10 replicon. These are brought together in parallel register by zipping-up DNA-bound RepA monomers. We also present evidence for a distinct role of RepA dimers in DNA looping. This work defines a new regulatory interface in Rep proteins.

摘要

在许多革兰氏阴性菌的质粒复制子中,Rep蛋白二聚体是其基因的转录自抑制因子,而单体是DNA复制的起始因子。两种功能之间的转换意味着Rep蛋白构象的重塑,并且由Rep蛋白与起始DNA重复序列(迭代子)或伴侣蛋白的结合所促进。Rep蛋白还发挥着另一个关键作用:它们将位于同一或不同质粒分子上的两个迭代子DNA片段连接在一起。这些分别被称为“环状”和“手铐状”的复合物被认为是质粒复制的负调节因子。尽管在许多复制子中都发现了依赖Rep蛋白的质粒“手铐状”结构的证据,但这些Rep-DNA组装体的结构仍然未知。在这里,通过蛋白质组学、电子显微镜、遗传分析和建模相结合的方法,我们对pPS10复制子起始位点处发现的两个迭代子“手铐状”阵列的可能三维结构有了深入了解。这些阵列通过DNA结合的RepA单体的“拉链式”排列平行对齐在一起。我们还提供了证据证明RepA二聚体在DNA环化中具有独特作用。这项工作定义了Rep蛋白中的一个新的调节界面。

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