Department of Biochemistry, University of Oxford, Oxford OX1 3QU, UK.
Mol Cell. 2011 Oct 7;44(1):97-107. doi: 10.1016/j.molcel.2011.07.034.
The contribution of DNA catenation to sister chromatid cohesion is unclear partly because it has never been observed directly within mitotic chromosomes. Differential sedimentation-velocity and gel electrophoresis reveal that sisters of 26 kb circular minichromosomes are held together by catenation as well as by cohesin. The finding that chemical crosslinking of cohesin's three subunit interfaces entraps sister DNAs of circular but not linear minichromosomes implies that cohesin functions using a topological principle. Importantly, cohesin holds both catenated and uncatenated DNAs together in this manner. In the vicinity of centromeres, catenanes are resolved by spindle forces, but linkages mediated directly by cohesin resist these forces even after complete decatenation. Crucially, persistence of catenation after S phase depends on cohesin. We conclude that by retarding Topo II-driven decatenation, cohesin mediates sister chromatid cohesion by an indirect mechanism as well as one involving entrapment of sister DNAs inside its tripartite ring.
DNA 连环化对姐妹染色单体黏合的贡献尚不清楚,部分原因是它从未在有丝分裂染色体中被直接观察到。差速沉降速度和凝胶电泳显示,26kb 圆形微小染色体的姐妹染色单体通过连环化以及黏连蛋白结合在一起。化学交联黏连蛋白的三个亚基界面可以捕获圆形但不是线性微小染色体的姐妹 DNA,这表明黏连蛋白的功能是基于拓扑学原理。重要的是,黏连蛋白以这种方式将连环化和非连环化的 DNA 结合在一起。在着丝粒附近,连环体被纺锤体力解开,但直接由黏连蛋白介导的连接即使在完全去连环化后也能抵抗这些力。至关重要的是,S 期后连环化的持续存在取决于黏连蛋白。我们的结论是,通过减缓拓扑异构酶 II 驱动的去连环化,黏连蛋白通过间接机制以及将姐妹 DNA 困在其三聚体环内的机制介导姐妹染色单体黏合。
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