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首页> 外文期刊>Chromosoma >Meiotic localization of Mre11 and Rad50 in wild type, spo11-1, and MRN complex mutants of Coprinus cinereus
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Meiotic localization of Mre11 and Rad50 in wild type, spo11-1, and MRN complex mutants of Coprinus cinereus

机译:Mre11和Rad50在野生型鬼臼的突变型,spo11-1和MRN复合突变体中的减数分裂定位

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The Mre11-Rad50-Nbs1 (MRN) complex is required for numerous cellular processes that involve interactions with DNA double-strand breaks. For the majority of these processes, the MRN complex is thought to act as a unit, with each protein aiding the activity of the others. We have examined the relationship between Mre11 and Rad50 during meiosis in the basidiomycete Coprinus cinereus (Coprinopsis cinerea), investigating to what extent activities of Mre11 and Rad50 are interdependent. We showed that mre11-1 is epistatic to rad50-1 with respect to the time of meiotic arrest, indicating that Mre11 activity facilitates the diffuse diplotene arrest of rad50 mutants. Anti-Mre11 and anti-Rad50 antibodies were used to examine MRN complex localization in a wild-type strain and in spo11, mre11, and rad50 mutants. In wild type, numbers of Mre11 and Rad50 foci peaked at time points corresponding to leptotene and early zygotene. In the spo11-1 mutant, which is defective in meiotic double-strand break formation, foci accumulated throughout prophase I. Of seven MRN mutants examined, only two rad50 strains exhibited Mre11 and Rad50 foci that localized to chromatin, although Mre11 protein was found in the cell for all of them. Analysis of predicted mutant structures showed that stable localization of Mre11 and Rad50 does not depend upon a wild-type hook-proximal coiled coil, but does require the presence of the Rad50 ATPase/adenylate cyclase domains. We found that Mre11 and Rad50 were interdependent for binding to meiotic chromosomes. However, the majority of foci observed apparently contained only one of the two proteins. Independent Mre11 and Rad50 foci might indicate disassociation of the complex during meiosis or could reflect independent structural roles for the two proteins in meiotic chromatin. Communicated by: S. Keeney
机译:Mre11-Rad50-Nbs1(MRN)复合物是涉及与DNA双链断裂相互作用的众多细胞过程所必需的。对于大多数这些过程,MRN复合物被认为是一个单元,每种蛋白质都有助于其他蛋白质的活性。我们研究了灰担子菌(Coprinopsis cinerea)减数分裂过程中Mre11和Rad50之间的关系,研究了Mre11和Rad50的活性在何种程度上相互依赖。我们表明,相对于减数分裂停滞的时间,mre11-1相对于rad50-1具有上位性,表明Mre11活性促进了rad50突变体的弥散二戊烯停滞。抗Mre11和抗Rad50抗体用于检查MRN复合体在野生型菌株以及spo11,mre11和rad50突变体中的定位。在野生型中,Mre11和Rad50病灶的数量在对应于瘦素和早期合子的时间点达到峰值。在减数分裂双链断裂形成有缺陷的spo11-1突变体中,病灶在前期I积累。在检查的7个MRN突变体中,尽管发现了Mre11蛋白,但只有两个rad50菌株显示了Mre11和Rad50病灶位于染色质。所有的细胞。对预测的突变体结构的分析表明,Mre11和Rad50的稳定定位不依赖于野生型钩状近端卷曲螺旋,而是需要Rad50 ATPase /腺苷酸环化酶结构域的存在。我们发现Mre11和Rad50是相互依赖的与减数分裂染色体的结合。但是,观察到的大多数病灶显然仅包含两种蛋白质之一。独立的Mre11和Rad50病灶可能表明在减数分裂过程中复合物解离,或反映了减数分裂染色质中这两种蛋白质的独立结构作用。沟通者:S. Keeney

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