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Resolution of a Holliday junction by vaccinia topoisomerase requires a spacer DNA segment 3′ of the CCCTT↓ cleavage sites

机译:牛痘拓扑异构酶解析霍利迪交界处需要CCCTT↓裂解位点3的间隔DNA片段

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摘要

Vaccinia virus DNA topoisomerase catalyzes reso­lution of synthetic Holliday junctions in vitro. The mechanism entails concerted transesterifications at two recognition sites, 5′-CCCTT↓, that are opposed within a partially mobile four-way junction. Efficient resolution occurs on a junction with a 10 bp segment of branch mobility (5′-GCCCTTATCG) that extends 4 bp 3′ of the scissile phosphate. Here we report that resolution is decreased when branch mobility is limited to an 8 bp segment extending 2 bp 3′ of the cleavage site and then eliminated when branch mobility is confined to the 6 bp GCCCTT sequence 5′ of the scissile phosphate. We surmise that a spacer region 3′ of CCCTT is needed for simultaneous cleavage at two opposing sites at the junction. Branch mobility is not required for reaction chem­i­stry at a junction, because topoisomerase cleaves a single CCCTT site in a non-mobile four-way junction where the scissile phosphate is at the crossover point. The junction resolvase activity of topo­isomerase may be involved in forming the hairpin telomeres of the vaccinia genome.
机译:牛痘病毒DNA拓扑异构酶在体外催化合成的霍利迪接头的溶解。该机制要求在两个识别位点(5'-CCCTT↓)上发生协调的酯交换,这两个位点在部分移动的四向接头中相对。有效的分离发生在具有10 bp分支迁移率片段(5'-GCCCTTATCG)的交界处,该片段延伸了易裂磷酸盐的4 bp 3'。在这里我们报告说,当分支的迁移率限制在一个8 bp的片段,延伸至切割位点3'的3'时分辨率降低,然后,当分支的迁移率被限制在可裂解的磷酸盐的6 bp GCCCTT序列5'时,分辨率就降低了。我们推测,需要CCCTT的间隔区3'同时在连接处的两个相对位点进行裂解。交联处的化学反应不需要支路迁移,因为拓扑异构酶会在不可移动的四向交界处切割单个CCCTT位点,在该处,易裂磷酸盐位于交叉点。拓扑异构酶的连接分辨酶活性可能与牛痘基因组的发夹型端粒形成有关。

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