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GEN1 promotes Holliday junction resolution by a coordinated nick and counter-nick mechanism

机译:GEN1通过协调的缺口和反缺口机制促进霍利迪交界处分离

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Holliday junctions (HJs) that physically link sister chromatids or homologous chromosomes are formed as intermediates during DNA repair by homologous recombination. Persistent recombination intermediates are acted upon by structure-selective endonucleases that are required for proper chromosome segregation at mitosis. Here, we have purified full-length human GEN1 protein and show that it promotes Holliday junction resolution by a mechanism that is analogous to that exhibited by the prototypic HJ resolvase E. coli RuvC. We find that GEN1 cleaves HJs by a nick and counter-nick mechanism involving dual co-ordinated incisions that lead to the formation of ligatable nicked duplex products. As observed with RuvC, cleavage of the first strand is rate limiting, while second strand cleavage is rapid. In contrast to RuvC, however, GEN1 is largely monomeric in solution, but dimerizes on the HJ. Using HJs containing non-cleavable phosphorothioate-containing linkages in one strand, we show that the two incisions can be uncoupled and that the first nick occurs upon GEN1 dimerization at the junction. These results indicate that the mechanism of HJ resolution is largely conserved from bacteria to man, despite a lack of sequence homology between the resolvases.
机译:物理上连接姐妹染色单体或同源染色体的霍利迪结(HJs)在DNA修复过程中通过同源重组形成为中间体。持久的重组中间体受有丝分裂时适当的染色体分离所必需的结构选择性核酸内切酶作用。在这里,我们已经纯化了全长人类GEN1蛋白,并显示它通过类似于原型HJ分离酶大肠杆菌RuvC所展示的机制来促进霍利迪连接解析。我们发现GEN1通过涉及双配位切口的切口和反切口机制切割HJ,导致形成可韧带状切口的双工产物。如用RuvC观察到的,第一条链的切割是速率限制,而第二条链的切割是快速的。与RuvC相反,GEN1在溶液中主要是单体,但在HJ上却二聚。使用在一条链中包含不可裂解的含硫代磷酸酯键的HJ,我们显示两个切口可以解偶联,并且在GEN1二聚化后在连接处出现第一个切口。这些结果表明,尽管在分辨分子之间缺乏序列同源性,HJ分解的机制在细菌与人之间还是很保守的。

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