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CDK promotes interactions of Sld3 and Drc1 with Cut5 for initiation of DNA replication in fission yeast

机译:CDK促进Sld3和Drc1与Cut5的相互作用,引发裂变酵母中DNA复制的启动

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摘要

Cyclin-dependent kinase (CDK) plays essential roles in the initiation of DNA replication in eukaryotes. Although interactions of CDK-phosphorylated Sld2/Drc1 and Sld3 with Dpb11 have been shown to be essential in budding yeast, it is not known whether the mechanism is conserved. In this study, we investigated how CDK promotes the assembly of replication proteins onto replication origins in fission yeast. Phosphorylation of Sld3 was found to be dependent on CDK in S phase. Alanine substitutions at CDK sites decreased the interaction with Cut5/Dpb11 at the N-terminal BRCT motifs and decreased the loading of Cut5 onto replication origins. This defect was suppressed by overexpression of drc1~+. Phosphorylation of a conserved CDK site, Thr-111, in Drc1 was critical for interaction with Cut5 at the C-terminal BRCT motifs and was required for loading of Cut5. In a yeast three-hybrid assay, Sld3, Cut5, and Drc1 were found to form a ternary complex dependent on the CDK sites of Sld3 and Drc1, and Drc1-Cut5 binding enhanced the Sld3-Cut5 interaction. These results show that the mechanism of CDK-dependent loading of Cut5 is conserved in fission yeast in a manner similar to that elucidated in budding yeast.
机译:细胞周期蛋白依赖性激酶(CDK)在真核生物DNA复制的启动中起着重要作用。尽管已显示CDK磷酸化的Sld2 / Drc1和Sld3与Dpb11的相互作用在发芽酵母中是必不可少的,但尚不清楚该机制是否保守。在这项研究中,我们研究了CDK如何促进复制蛋白在裂殖酵母中复制起点上的组装。发现Sld3的磷酸化依赖于S期的CDK。 CDK位点的丙氨酸取代减少了在N端BRCT基序上与Cut5 / Dpb11的相互作用,并减少了Cut5在复制起点上的负载。 drc1〜+的过量表达抑制了这一缺陷。 Drc1中保守的CDK位点Thr-111的磷酸化对于在C端BRCT基序上与Cut5相互作用至关重要,并且是加载Cut5所必需的。在酵母三杂交试验中,Sld3,Cut5和Drc1被发现形成依赖于Sld3和Drc1的CDK位点的三元复合物,并且Drc1-Cut5的结合增强了Sld3-Cut5的相互作用。这些结果表明,Cut5依赖CDK的加载机制在裂变酵母中得以保守,其方式与在发芽酵母中阐明的相似。

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