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通过Mpk1细胞壁完整性丝裂原活化蛋白激酶对酵母Rlm1转录因子的调控。

Regulation of the yeast Rlm1 transcription factor by the Mpk1 cell wall integrity MAP kinase.

作者信息

Jung Un Sung, Sobering Andrew K, Romeo Martin J, Levin David E

机构信息

Department of Biochemistry and Molecular Biology, Bloomberg School of Public Health, The Johns Hopkins University, Baltimore, MD 21205, USA.

出版信息

Mol Microbiol. 2002 Nov;46(3):781-9. doi: 10.1046/j.1365-2958.2002.03198.x.

DOI:10.1046/j.1365-2958.2002.03198.x
PMID:12410835
Abstract

The Mpk1 MAP kinase of the Saccharomyces cerevisiae cell wall integrity signalling pathway phosphorylates and activates the Rlm1 transcription factor in response to cell wall stress. Rlm1 is related to mammalian MEF2 isoforms, and shares a similar DNA-binding specificity. Signalling through Rlm1 regulates the expression of at least 25 genes, most of which have been implicated in cell wall biogenesis. We report here the transcriptional induction by agents of cell wall stress of a set of lacZ reporter plasmids derived from several Rlm1-responsive genes. Analysis of substitution mutations at putative Mpk1 phosphorylation sites within Rlm1 revealed that Ser427 and Thr439 are important for its stress-induced transcriptional activation of these reporter plasmids. Assessment of Rlm1 activation potency when fused to a heterologous DNA-binding domain showed that the identified seryl and threonyl residues are necessary for the Rlm1 transcriptional activation function independently of its DNA binding. We also demonstrate that a MAP kinase docking site, shown recently to mediate activation of MEF2A and MEF2C, is conserved in Rlm1 and is required for its ability to mediate transcriptional activation in response to agents that induce cell wall stress. Finally, intracellular localization analyses show that Rlm1 resides in the nucleus regardless of its activation and phosphorylation status. Together these observations support the inference that Mpk1 regulates the Rlm1 transcriptional activation function by phosphorylation of Ser427 and Thr439.

摘要

酿酒酵母细胞壁完整性信号通路中的Mpk1丝裂原活化蛋白激酶在响应细胞壁应激时会磷酸化并激活Rlm1转录因子。Rlm1与哺乳动物MEF2亚型相关,且具有相似的DNA结合特异性。通过Rlm1的信号传导调节至少25个基因的表达,其中大多数基因与细胞壁生物合成有关。我们在此报告了一组源自几个Rlm1反应基因的lacZ报告质粒在细胞壁应激因子作用下的转录诱导情况。对Rlm1内假定的Mpk1磷酸化位点的取代突变分析表明,Ser427和Thr439对其应激诱导的这些报告质粒的转录激活很重要。当与异源DNA结合结构域融合时对Rlm1激活能力的评估表明,所鉴定的丝氨酸和苏氨酸残基对于Rlm1转录激活功能是必需的,且与其DNA结合无关。我们还证明,最近显示介导MEF2A和MEF2C激活的丝裂原活化蛋白激酶对接位点在Rlm1中是保守的,并且是其响应诱导细胞壁应激的因子介导转录激活能力所必需的。最后,细胞内定位分析表明,无论Rlm1的激活和磷酸化状态如何,它都位于细胞核中。这些观察结果共同支持了Mpk1通过磷酸化Ser427和Thr439来调节Rlm1转录激活功能的推断。

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