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与单个RuvA四聚体复合的霍利迪连接体DNA的晶体结构。

Crystal structure of the holliday junction DNA in complex with a single RuvA tetramer.

作者信息

Ariyoshi M, Nishino T, Iwasaki H, Shinagawa H, Morikawa K

机构信息

Department of Structural Biology, Biomolecular Engineering Research Institute (BERI), 6-2-3 Furuedai, Suita, Osaka 565-0874, Japan.

出版信息

Proc Natl Acad Sci U S A. 2000 Jul 18;97(15):8257-62. doi: 10.1073/pnas.140212997.

Abstract

In the major pathway of homologous DNA recombination in prokaryotic cells, the Holliday junction intermediate is processed through its association with RuvA, RuvB, and RuvC proteins. Specific binding of the RuvA tetramer to the Holliday junction is required for the RuvB motor protein to be loaded onto the junction DNA, and the RuvAB complex drives the ATP-dependent branch migration. We solved the crystal structure of the Holliday junction bound to a single Escherichia coli RuvA tetramer at 3.1-A resolution. In this complex, one side of DNA is accessible for cleavage by RuvC resolvase at the junction center. The refined junction DNA structure revealed an open concave architecture with a four-fold symmetry. Each arm, with B-form DNA, in the Holliday junction is predominantly recognized in the minor groove through hydrogen bonds with two repeated helix-hairpin-helix motifs of each RuvA subunit. The local conformation near the crossover point, where two base pairs are disrupted, suggests a possible scheme for successive base pair rearrangements, which may account for smooth Holliday junction movement without segmental unwinding.

摘要

在原核细胞中同源DNA重组的主要途径中,霍利迪连接体中间体通过与RuvA、RuvB和RuvC蛋白结合来进行加工。RuvA四聚体与霍利迪连接体的特异性结合是RuvB运动蛋白加载到连接体DNA上所必需的,并且RuvAB复合物驱动ATP依赖的分支迁移。我们以3.1埃的分辨率解析了与单个大肠杆菌RuvA四聚体结合的霍利迪连接体的晶体结构。在这个复合物中,DNA的一侧在连接体中心可被RuvC解离酶切割。优化后的连接体DNA结构显示出具有四重对称性的开放凹面结构。霍利迪连接体中每条具有B型DNA的臂主要通过与每个RuvA亚基的两个重复螺旋-发夹-螺旋基序形成氢键,在小沟中被识别。在两个碱基对被破坏的交叉点附近的局部构象,提示了一个连续碱基对重排的可能方案,这可能解释了霍利迪连接体的平滑移动而无需片段解旋。

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