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真核双组分组氨酸激酶Sln1p通过转录因子Skn7p调控OCH1。

The eukaryotic two-component histidine kinase Sln1p regulates OCH1 via the transcription factor, Skn7p.

作者信息

Li Sheng, Dean Susan, Li Zhijian, Horecka Joe, Deschenes Robert J, Fassler Jan S

机构信息

Department of Biological Sciences, University of Iowa, University of Iowa, Iowa City, Iowa 52242, USA.

出版信息

Mol Biol Cell. 2002 Feb;13(2):412-24. doi: 10.1091/mbc.01-09-0434.

Abstract

The yeast "two-component" osmotic stress phosphorelay consists of the histidine kinase, Sln1p, the phosphorelay intermediate, Ypd1p and two response regulators, Ssk1p and Skn7p, whose activities are regulated by phosphorylation of a conserved aspartyl residue in the receiver domain. Dephospho-Ssk1p leads to activation of the hyper-osmotic response (HOG) pathway, whereas phospho-Skn7p presumably leads to activation of hypo-osmotic response genes. The multifunctional Skn7 protein is important in oxidative as well as osmotic stress; however, the Skn7p receiver domain aspartate that is the phosphoacceptor in the SLN1 pathway is dispensable for oxidative stress. Like many well-characterized bacterial response regulators, Skn7p is a transcription factor. In this report we investigate the role of Skn7p in osmotic response gene activation. Our studies reveal that the Skn7p HSF-like DNA binding domain interacts with a cis-acting element identified upstream of OCH1 that is distinct from the previously defined HSE-like Skn7p binding site. Our data support a model in which Skn7p receiver domain phosphorylation affects transcriptional activation rather than DNA binding to this class of DNA binding site.

摘要

酵母“双组分”渗透应激磷酸化信号转导途径由组氨酸激酶Sln1p、磷酸化信号转导中间体Ypd1p以及两个应答调节因子Ssk1p和Skn7p组成,它们的活性通过受体结构域中保守天冬氨酸残基的磷酸化来调节。去磷酸化的Ssk1p会激活高渗应答(HOG)途径,而磷酸化的Skn7p可能会激活低渗应答基因。多功能的Skn7蛋白在氧化应激和渗透应激中都很重要;然而,在SLN1途径中作为磷酸化受体的Skn7p受体结构域天冬氨酸对于氧化应激是可有可无的。与许多已充分表征的细菌应答调节因子一样,Skn7p是一种转录因子。在本报告中,我们研究了Skn7p在渗透应答基因激活中的作用。我们的研究表明,Skn7p的热休克因子样DNA结合结构域与在OCH1上游鉴定出的一个顺式作用元件相互作用,该元件不同于先前定义的类热休克元件的Skn7p结合位点。我们的数据支持这样一个模型,即Skn7p受体结构域的磷酸化影响转录激活,而不是影响与这类DNA结合位点的DNA结合。

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