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首页> 外文期刊>Nucleic Acids Research >Meiotic association between Spo11 regulated by Rec102, Rec104 and Rec114
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Meiotic association between Spo11 regulated by Rec102, Rec104 and Rec114

机译:Rec102,Rec104和Rec114调控的Spo11之间的减数分裂关联

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摘要

Meiotic recombination is initiated by DNA double-stranded break (DSB) formation catalyzed by Spo11, a type-II topoisomerase-like transesterificase, presumably via a dimerization-mediated mechanism. We demonstrate the existence of in vivo interactions between Spo11 proteins carrying distinct tags, and the chromatin-binding and DSB activity of tagged Spo11 at innate and targeted DSB sites upon fusion to the Gal4 DNA-binding domain. First we identified the interaction between Spo11-3FLAG and Gal4BD-Spo11 proteins, and established that this interaction specifically occurs at the time of DSB formation. We then observed that presence of the Gal4BD-spo11Y135F (nuclease-deficient) protein allows Spo11-3FLAG recruitment at the GAL2 locus, indicative of the formation of a hetero-complex near the GAL2 UAS sites, but no formation of double- or single-strand breaks. Spo11 self-interaction around the GAL2 DSB site depends on other proteins for DSB formation, in particular Rec102, Rec104 and Rec114. Together, these results suggest that in vivo self-association of Spo11 during meiosis is genetically regulated. The results are discussed in relation to possible roles of Spo11 self-interaction in the control of the cleavage activity.
机译:减数分裂重组是由Spo11(一种II型拓扑异构酶样酯交换酶)催化的DNA双链断裂(DSB)形成开始的,大概是通过二聚化介导的机制。我们证明了带有独特标签的Spo11蛋白之间的体内相互作用的存在,以及与Gal4 DNA结合结构域融合后在先天和目标DSB位点上标记的Spo11的染色质结合和DSB活性。首先,我们确定了Spo11-3FLAG与Gal4BD-Spo11蛋白之间的相互作用,并确定这种相互作用在DSB形成时特别发生。然后,我们观察到Gal4BD-spo11Y135F(核酸酶缺陷)蛋白的存在使Spo11-3FLAG可以在GAL2位点募集,这表明在GAL2 UAS位点附近形成了一个复杂的杂物,但没有形成双或单链断裂。 GAL2 DSB位点周围的Spo11自相互作用取决于形成DSB的其他蛋白质,特别是Rec102,Rec104和Rec114。总之,这些结果表明减数分裂过程中Spo11的体内自缔合是遗传调控的。讨论了有关Spo11自我相互作用在控制卵裂活性中可能发挥的作用的结果。

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