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减数分裂特异性检查点激酶Mek1对裂殖酵母减数分裂进程的调控

Regulation of meiotic progression by the meiosis-specific checkpoint kinase Mek1 in fission yeast.

作者信息

Pérez-Hidalgo Livia, Moreno Sergio, San-Segundo Pedro A

机构信息

Centro de Investigación del Cáncer, CSIC/University of Salamanca, Campus Unamuno, 37007 Salamanca, Spain.

出版信息

J Cell Sci. 2003 Jan 15;116(Pt 2):259-71. doi: 10.1242/jcs.00232.

DOI:10.1242/jcs.00232
PMID:12482912
Abstract

During the eukaryotic cell cycle, accurate transmission of genetic information to progeny is ensured by the operation of cell cycle checkpoints. Checkpoints are regulatory mechanisms that block cell cycle progression when key cellular processes are defective or chromosomes are damaged. During meiosis, genetic recombination between homologous chromosomes is essential for proper chromosome segregation at the first meiotic division. In response to incomplete recombination, the pachytene checkpoint (also known as the meiotic recombination checkpoint) arrests or delays meiotic cell cycle progression, thus preventing the formation of defective gametes. Here, we describe a role for a meiosis-specific kinase, Mek1, in the meiotic recombination checkpoint in fission yeast. Mek1 belongs to the Cds1/Rad53/Chk2 family of kinases containing forkhead-associated domains, which participate in a number of checkpoint responses from yeast to mammals. We show that defects in meiotic recombination generated by the lack of the fission yeast Meu13 protein lead to a delay in entry into meiosis I owing to inhibitory phosphorylation of the cyclin-dependent kinase Cdc2 on tyrosine 15. Mutation of mek1(+) alleviates this checkpoint-induced delay, resulting in the formation of largely inviable meiotic products. Experiments involving ectopic overexpression of the mek1(+) gene indicate that Mek1 inhibits the Cdc25 phosphatase, which is responsible for dephosphorylation of Cdc2 on tyrosine 15. Furthermore, the meiotic recombination checkpoint is impaired in a cdc25 phosphorylation site mutant. Thus, we provide the first evidence of a connection between an effector kinase of the meiotic recombination checkpoint and a crucial cell cycle regulator and present a model for the operation of this meiotic checkpoint in fission yeast.

摘要

在真核细胞周期中,细胞周期检查点的运作确保了遗传信息准确传递给子代。检查点是一种调节机制,当关键细胞过程出现缺陷或染色体受损时,会阻止细胞周期进程。在减数分裂过程中,同源染色体之间的遗传重组对于第一次减数分裂时染色体的正确分离至关重要。作为对不完全重组的响应,粗线期检查点(也称为减数分裂重组检查点)会阻止或延迟减数分裂细胞周期进程,从而防止有缺陷配子的形成。在此,我们描述了一种减数分裂特异性激酶Mek1在裂殖酵母减数分裂重组检查点中的作用。Mek1属于含有叉头相关结构域的Cds1/Rad53/Chk2激酶家族,该家族参与从酵母到哺乳动物的多种检查点反应。我们发现,由于裂殖酵母Meu13蛋白缺失导致减数分裂重组缺陷,会使细胞周期蛋白依赖性激酶Cdc2的酪氨酸15位点发生抑制性磷酸化,从而导致进入减数分裂I延迟。mek1(+)基因突变可缓解这种检查点诱导的延迟,导致大量减数分裂产物无法存活。涉及mek1(+)基因异位过表达的实验表明,Mek1抑制Cdc25磷酸酶,该磷酸酶负责Cdc2酪氨酸15位点的去磷酸化。此外,在cdc25磷酸化位点突变体中,减数分裂重组检查点功能受损。因此,我们首次证明了减数分裂重组检查点的效应激酶与关键细胞周期调节因子之间的联系,并提出了裂殖酵母中这种减数分裂检查点的运作模型。

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