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通过分子显微镜分析同源重组背景下的重组酶及相关蛋白。

Recombinases and Related Proteins in the Context of Homologous Recombination Analyzed by Molecular Microscopy.

作者信息

Dupaigne Pauline, Tavares Eliana Moreira, Piétrement Olivier, Le Cam Eric

机构信息

Gustave Roussy, CNRS UMR8126, Université Paris-Saclay, Villejuif, France.

出版信息

Methods Mol Biol. 2018;1805:251-270. doi: 10.1007/978-1-4939-8556-2_13.

Abstract

Transmission electron microscopy (TEM) and atomic force microscopy (AFM) are powerful tools to study the behavior of various actors in homologous recombination including molecular motors such as recombinases and helicases/translocases. Here we present specific approaches developed in terms of sample preparation and imaging methods to contribute to the understanding of homologous recombination process and its regulation focusing on the interplay between recombinases and other related proteins such as mediators or antirecombinase actors.Homologous recombination (HR) is a high-fidelity DNA repair pathway since it uses a homologous DNA as template. Recombinases such as RecA in bacteria, RadA in archaea, and Rad51 in eukaryotes are key proteins in the HR pathway: HR is initiated with formation of an ssDNA overhang on which recombinases polymerize and form a dynamic active nucleoprotein filament able to search for homology and to exchange DNA strand in an ATP-dependent manner. We provide practical methods to analyze presynaptic filament formation on ssDNA, its composition and regulation in presence of mediator partners, antirecombinase activity of translocase, and chromatin remodeling events.

摘要

透射电子显微镜(TEM)和原子力显微镜(AFM)是研究同源重组中各种作用因子行为的强大工具,这些作用因子包括诸如重组酶和解旋酶/转位酶等分子马达。在此,我们介绍在样品制备和成像方法方面所开发的特定方法,以促进对同源重组过程及其调控的理解,重点关注重组酶与其他相关蛋白质(如介导因子或抗重组酶作用因子)之间的相互作用。同源重组(HR)是一种高保真的DNA修复途径,因为它使用同源DNA作为模板。细菌中的RecA、古细菌中的RadA以及真核生物中的Rad51等重组酶是HR途径中的关键蛋白质:HR起始于单链DNA突出端的形成,重组酶在该突出端上聚合并形成动态的活性核蛋白丝,该丝能够寻找同源性并以ATP依赖的方式交换DNA链。我们提供了实用方法,用于分析单链DNA上突触前丝的形成、其组成以及在存在介导因子伙伴时的调控、转位酶的抗重组酶活性和染色质重塑事件。

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