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首页> 外文期刊>Molecular and Cellular Biology >Mechanistic Insights into Replication Termination as Revealed by Investigations of the Reb1-Ter3 Complex of Schizosaccharomyces pombe
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Mechanistic Insights into Replication Termination as Revealed by Investigations of the Reb1-Ter3 Complex of Schizosaccharomyces pombe

机译:通过对粟酒裂殖酵母Reb1-Ter3复合物的研究揭示了对复制终止的机理性认识。

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摘要

Relatively little is known about the interaction of eukaryotic replication terminator proteins with the cognate termini and the replication termination mechanism. Here, we report a biochemical analysis of the interaction of the Reb1 terminator protein of Schizosaccharomyces pombe, which binds to the Ter3 site present in the nontranscribed spacers of ribosomal DNA, located in chromosome III. We show that Reb1 is a dimeric protein and that the N-terminal dimerization domain of the protein is dispensable for replication termination. Unlike its mammalian counterpart Ttf1, Reb1 did not need an accessory protein to bind to Ter3. The two myb/SANT domains and an adjacent, N-terminal 154-amino-acid-long segment (called the myb-associated domain) were both necessary and sufficient for optimal DNA binding in vitro and fork arrest in vivo. The protein and its binding site Ter3 were unable to arrest forks initiated in vivo from ars of Saccharomyces cerevisiae in the cell milieu of the latter despite the facts that the protein retained the proper affinity of binding, was located in vivo at the Ter site, and apparently was not displaced by the “sweepase” Rrm3. These observations suggest that replication fork arrest is not an intrinsic property of the Reb1-Ter3 complex.
机译:关于真核复制终止子蛋白与同源末端和复制终止机制的相互作用的了解相对较少。在这里,我们报告了生化裂殖酵母Reb1终止蛋白相互作用的生化分析,该蛋白与位于核糖体DNA非转录间隔区中的 Ter3 位点结合。染色体III。我们显示Reb1是一种二聚体蛋白质,该蛋白质的N端二聚结构域可用于复制终止。与哺乳动物的Ttf1不同,Reb1不需要辅助蛋白即可与 Ter3 结合。两个myb / SANT结构域和一个相邻的N端154个氨基酸长的片段(称为myb相关结构域)对于在体外实现最佳的DNA结合以及在体内进行分叉阻滞都是必要和充分的。该蛋白及其结合位点 Ter3 在其细胞环境中不能阻止由酿酒酵母 ars 体内启动的叉子。蛋白质保留了适当的结合亲和力的事实,该蛋白质位于体内的 Ter 位点,并且显然没有被“清除酶” Rrm3取代。这些观察结果表明复制叉阻滞不是Reb1- Ter3 复合物的固有特性。

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