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Ras/cAMP信号通路和类周期蛋白依赖性激酶Ime2调节酿酒酵母中的丝裂原活化蛋白激酶Smk1和孢子形态发生。

The Ras/cAMP pathway and the CDK-like kinase Ime2 regulate the MAPK Smk1 and spore morphogenesis in Saccharomyces cerevisiae.

作者信息

McDonald Christine M, Wagner Marisa, Dunham Maitreya J, Shin Marcus E, Ahmed Noreen T, Winter Edward

机构信息

Department of Genome Science, University of Washington, Seattle, Washington 98195, USA.

出版信息

Genetics. 2009 Feb;181(2):511-23. doi: 10.1534/genetics.108.098434. Epub 2008 Dec 15.

Abstract

Meiotic development (sporulation) in the yeast Saccharomyces cerevisiae is induced by nutritional deprivation. Smk1 is a meiosis-specific MAP kinase homolog that controls spore morphogenesis after the meiotic divisions have taken place. In this study, recessive mutants that suppress the sporulation defect of a smk1-2 temperature-sensitive hypomorph were isolated. The suppressors are partial function alleles of CDC25 and CYR1, which encode the Ras GDP/GTP exchange factor and adenyl cyclase, respectively, and MDS3, which encodes a kelch-domain protein previously implicated in Ras/cAMP signaling. Deletion of PMD1, which encodes a Mds3 paralog, also suppressed the smk1-2 phenotype, and a mds3-Delta pmd1-Delta double mutant was a more potent suppressor than either single mutant. The mds3-Delta, pmd1-Delta, and mds3-Delta pmd1-Delta mutants also exhibited mitotic Ras/cAMP phenotypes in the same rank order. The effect of Ras/cAMP pathway mutations on the smk1-2 phenotype required the presence of low levels of glucose. Ime2 is a meiosis-specific CDK-like kinase that is inhibited by low levels of glucose via its carboxy-terminal regulatory domain. IME2-DeltaC241, which removes the carboxy-terminal domain of Ime2, exacerbated the smk1-2 spore formation phenotype and prevented cyr1 mutations from suppressing smk1-2. Inhibition of Ime2 in meiotic cells shortly after Smk1 is expressed revealed that Ime2 promotes phosphorylation of Smk1's activation loop. These findings demonstrate that nutrients can negatively regulate Smk1 through the Ras/cAMP pathway and that Ime2 is a key activator of Smk1 signaling.

摘要

酿酒酵母中的减数分裂发育(孢子形成)是由营养剥夺诱导的。Smk1是一种减数分裂特异性的丝裂原活化蛋白激酶同源物,在减数分裂完成后控制孢子形态发生。在本研究中,分离出了抑制smk1-2温度敏感型亚效等位基因孢子形成缺陷的隐性突变体。这些抑制子是CDC25和CYR1的部分功能等位基因,它们分别编码Ras GDP/GTP交换因子和腺苷酸环化酶,以及MDS3,其编码一种先前与Ras/cAMP信号传导有关的kelch结构域蛋白。编码Mds3旁系同源物的PMD1缺失也抑制了smk1-2表型,mds3-Δpmd1-Δ双突变体比任何一个单突变体都是更强效的抑制子。mds3-Δ、pmd1-Δ和mds3-Δpmd1-Δ突变体在有丝分裂Ras/cAMP表型方面也表现出相同的等级顺序。Ras/cAMP途径突变对smk1-2表型的影响需要低水平葡萄糖的存在。Ime2是一种减数分裂特异性的CDK样激酶,其通过羧基末端调节结构域被低水平葡萄糖抑制。去除Ime2羧基末端结构域的IME2-ΔC241加剧了smk1-2孢子形成表型,并阻止了cyr1突变对smk1-2的抑制。在Smk1表达后不久对减数分裂细胞中的Ime2进行抑制表明,Ime2促进Smk1激活环的磷酸化。这些发现表明,营养物质可通过Ras/cAMP途径对Smk1进行负调控,且Ime2是Smk1信号传导的关键激活因子。

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