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细胞内甘油水平调节酿酒酵母双组分调节因子Sln1p的活性。

Intracellular glycerol levels modulate the activity of Sln1p, a Saccharomyces cerevisiae two-component regulator.

作者信息

Tao W, Deschenes R J, Fassler J S

机构信息

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

出版信息

J Biol Chem. 1999 Jan 1;274(1):360-7. doi: 10.1074/jbc.274.1.360.

Abstract

The HOG mitogen-activated protein kinase pathway mediates the osmotic stress response in Saccharomyces cerevisiae, activating genes like GPD1 (glycerol phosphate dehydrogenase), required for survival under hyperosmotic conditions. Activity of this pathway is regulated by Sln1p, a homolog of the "two-component" histidine kinase family of signal transduction molecules prominent in bacteria. Sln1p also regulates the activity of a Hog1p-independent pathway whose transcriptional output can be monitored using an Mcm1p-dependent lacZ reporter gene. The relationship between the two Sln1p branches is unclear, however, the requirement for unphosphorylated pathway intermediates in Hog1p pathway activation and for phosphorylated intermediates in the activation of the Mcm1p reporter suggests that the two Sln1p branches are reciprocally regulated. To further investigate the signals and molecules involved in modulating Sln1p activity, we have screened for new mutations that elevate the activity of the Mcm1p-dependent lacZ reporter gene. We find that loss of function mutations in FPS1, a gene encoding the major glycerol transporter in yeast activates the reporter in a SLN1-dependent fashion. We propose that elevated intracellular glycerol levels in the fps1 mutant shift Sln1p to the phosphorylated state and trigger the Sln1-dependent activity of the Mcm1 reporter. These observations are consistent with a model in which Sln1p autophosphorylation is triggered by a hypo-osmotic stimulus and indicate that the Sln1p osmosensor is tied generally to osmotic balance, and may not specifically sense an external osmolyte.

摘要

Hog丝裂原活化蛋白激酶途径介导酿酒酵母中的渗透应激反应,激活如GPD1(甘油磷酸脱氢酶)等在高渗条件下生存所需的基因。该途径的活性由Sln1p调节,Sln1p是细菌中突出的信号转导分子“双组分”组氨酸激酶家族的同源物。Sln1p还调节一条不依赖Hog1p的途径的活性,其转录输出可使用依赖Mcm1p的lacZ报告基因进行监测。然而,两个Sln1p分支之间的关系尚不清楚,Hog1p途径激活中对未磷酸化途径中间体的需求以及Mcm1p报告基因激活中对磷酸化中间体的需求表明这两个Sln1p分支是相互调节的。为了进一步研究参与调节Sln1p活性的信号和分子,我们筛选了能提高依赖Mcm1p的lacZ报告基因活性的新突变。我们发现,FPS1(编码酵母中主要甘油转运蛋白的基因)功能缺失突变以依赖SLN1的方式激活报告基因。我们提出,fps1突变体中细胞内甘油水平升高会使Sln1p转变为磷酸化状态,并触发Mcm1报告基因的Sln1依赖性活性。这些观察结果与一个模型一致,在该模型中,Sln1p自磷酸化由低渗刺激触发,表明Sln1p渗透感受器通常与渗透平衡相关,可能不会特异性地感知外部渗透溶质。

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