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同源重组过程中的分支迁移:RuvAB-霍利迪连接体复合物的体外组装

Branch migration during homologous recombination: assembly of a RuvAB-Holliday junction complex in vitro.

作者信息

Hiom K, West S C

机构信息

Imperial Cancer Research Fund, Clare Hall Laboratories, South Mimms, Hertfordshire, England.

出版信息

Cell. 1995 Mar 10;80(5):787-93. doi: 10.1016/0092-8674(95)90357-7.

Abstract

The RuvA and RuvB proteins of E. coli promote the branch migration or movement of Holliday junctions during genetic recombination and DNA repair. Using small synthetic Holliday junctions in which the crossover point is confined near one end of the DNA molecule, we show that RuvAB-mediated branch migration occurs with a defined polarity. The assembly of RuvA and RuvB on the Holliday junction has been investigated by sedimentation analysis and by DNase I footprinting. We find that RuvA protein binds and protects all four strands of DNA at the crossover point, whereas RuvB protein binds the DNA asymmetrically. The polarity of branch migration is defined by the asymmetric assembly of the RuvAB branch migration complex relative to the junction and is consistent with a model in which RuvAB drives branch migration by passing the DNA through the hexameric rings of RuvB.

摘要

大肠杆菌的RuvA和RuvB蛋白在基因重组和DNA修复过程中促进霍利迪连接体的分支迁移或移动。使用交叉点局限于DNA分子一端附近的小型合成霍利迪连接体,我们发现RuvAB介导的分支迁移以确定的极性发生。通过沉降分析和DNase I足迹法研究了RuvA和RuvB在霍利迪连接体上的组装。我们发现,RuvA蛋白在交叉点结合并保护DNA的所有四条链,而RuvB蛋白以不对称方式结合DNA。分支迁移的极性由RuvAB分支迁移复合物相对于连接体的不对称组装所定义,并且与RuvAB通过使DNA穿过RuvB的六聚体环来驱动分支迁移的模型一致。

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