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在哺乳动物减数分裂I期间,黏连蛋白的Rec8 kleisin亚基被裂解酶切割的作用。

Role of cleavage by separase of the Rec8 kleisin subunit of cohesin during mammalian meiosis I.

作者信息

Kudo Nobuaki R, Anger Martin, Peters Antoine H F M, Stemmann Olaf, Theussl Hans-Christian, Helmhart Wolfgang, Kudo Hiromi, Heyting Christa, Nasmyth Kim

机构信息

Research Institute of Molecular Pathology, A-1030 Vienna, Austria.

出版信息

J Cell Sci. 2009 Aug 1;122(Pt 15):2686-98. doi: 10.1242/jcs.035287.

Abstract

Proteolytic activity of separase is required for chiasma resolution during meiosis I in mouse oocytes. Rec8, the meiosis-specific alpha-kleisin subunit of cohesin, is a key target of separase in yeast. Is the equivalent protein also a target in mammals? We show here that separase cleaves mouse Rec8 at three positions in vitro but only when the latter is hyper-phosphorylated. Expression of a Rec8 variant (Rec8-N) that cannot be cleaved in vitro at these sites causes sterility in male mice. Their seminiferous tubules lack a normal complement of 2 C secondary spermatocytes and 1 C spermatids and contain instead a high proportion of cells with enlarged nuclei. Chromosome spreads reveal that Rec8-N expression has no effect in primary spermatocytes but produces secondary spermatocytes and spermatids with a 4 C DNA content, suggesting that the first and possibly also the second meiotic division is abolished. Expression of Rec8-N in oocytes causes chromosome segregation to be asynchronous and delays its completion by 2-3 hours during anaphase I, probably due to inefficient proteolysis of Rec8-N by separase. Despite this effect, chromosome segregation must be quite accurate as Rec8-N does not greatly reduce female fertility. Our data is consistent with the notion that Rec8 cleavage is important and probably crucial for the resolution of chiasmata in males and females.

摘要

在小鼠卵母细胞减数分裂I期间,分离酶的蛋白水解活性是交叉点分辨率所必需的。Rec8是黏连蛋白中减数分裂特异性的α- kleisin亚基,是酵母中分离酶的关键靶点。在哺乳动物中,其等效蛋白也是靶点吗?我们在此表明,分离酶在体外可在三个位置切割小鼠Rec8,但仅在后者过度磷酸化时才会发生。一种在这些位点不能在体外被切割的Rec8变体(Rec8-N)的表达会导致雄性小鼠不育。它们的生精小管缺乏正常数量的2C次级精母细胞和1C精子细胞,取而代之的是含有高比例核增大的细胞。染色体铺展显示,Rec8-N的表达在初级精母细胞中没有影响,但会产生具有4C DNA含量的次级精母细胞和精子细胞,这表明第一次减数分裂以及可能的第二次减数分裂都被废除了。在卵母细胞中表达Rec8-N会导致染色体分离不同步,并在后期I将其完成时间延迟2至3小时,这可能是由于分离酶对Rec8-N的蛋白水解效率低下所致。尽管有这种影响,但由于Rec8-N不会大幅降低雌性生育力,所以染色体分离一定相当准确。我们的数据与以下观点一致,即Rec8切割对于雄性和雌性交叉点的分辨率很重要,可能也是至关重要的。

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