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首页> 外文期刊>Molecular and Cellular Biology >Meiotic DNA Double-Strand Break Repair Requires Two Nucleases, MRN and Ctp1, To Produce a Single Size Class of Rec12 (Spo11)-Oligonucleotide Complexes
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Meiotic DNA Double-Strand Break Repair Requires Two Nucleases, MRN and Ctp1, To Produce a Single Size Class of Rec12 (Spo11)-Oligonucleotide Complexes

机译:减数分裂DNA双链断裂修复需要两个核酸酶MRN和Ctp1,以产生单一大小的Rec12(Spo11)-寡核苷酸复合物。

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Programmed DNA double-strand breaks (DSBs) in meiosis are formed by Spo11 (Rec12 in fission yeast), a topoisomerase II-like protein, which becomes covalently attached to DNA 5′ ends. For DSB repair through homologous recombination, the protein must be removed from these DNA ends. We show here that Rec12 is endonucleolytically removed from DSB ends attached to a short oligonucleotide (Rec12-oligonucleotide complex), as is Spo11 in budding yeast. Fission yeast, however, has only one size class of Rec12-oligonucleotide complexes, whereas budding yeast has two size classes, suggesting different endonucleolytic regulatory mechanisms. Rec12-oligonucleotide generation strictly requires Ctp1 (Sae2 nuclease homolog), the Rad32 (Mre11) nuclease domain, and Rad50 of the MRN complex. Surprisingly, Nbs1 is not strictly required, indicating separable roles for the MRN subunits. On the basis of these and other data, we propose that Rad32 nuclease has the catalytic site for Rec12-oligonucleotide generation and is activated by Ctp1, which plays an additional role in meiotic recombination.
机译:减数分裂中的程序化DNA双链断裂(DSB)由Spo11(裂变酵母中的Rec12)形成,这是一种拓扑异构酶II样蛋白,它共价连接到DNA 5'末端。为了通过同源重组修复DSB,必须从这些DNA末端去除蛋白质。我们在这里显示,Rec12是从与短寡核苷酸(Rec12-寡核苷酸复合物)连接的DSB末端进行内切酶去除的,就像芽芽酵母中的Spo11一样。然而,裂变酵母仅具有一个大小类别的Rec12-寡核苷酸复合物,而出芽酵母具有两个大小类别,表明不同的内切核酸调节机制。 Rec12-寡核苷酸的产生严格要求Ctp1(Sae2核酸酶同源物),Rad32(Mre11)核酸酶结构域和MRN复合物的Rad50。出乎意料的是,并非严格要求Nbs1,这表明MRN亚基的作用可分。根据这些和其他数据,我们建议Rad32核酸酶具有Rec12寡核苷酸生成的催化位点,并被Ctp1激活,这在减数分裂重组中起着另外的作用。

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