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The Hsp70 homolog Ssb is essential for glucose sensing via the SNF1 kinase network.

机译:Hsp70同源物Ssb对于通过SNF1激酶网络进行葡萄糖感测至关重要。

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摘要

Yeast senses the availability of external energy sources via multiple interconnected signaling networks. One of the central components is SNF1, the homolog of mammalian AMP-activated protein kinase, which in yeast is essential for the expression of glucose-repressed genes. When glucose is available hyperphosphorylated SNF1 is rendered inactive by the type 1 protein phosphatase Glc7. Dephosphorylation requires Reg1, which physically targets Glc7 to SNF1. Here we show that the chaperone Ssb is required to keep SNF1 in the nonphosphorylated state in the presence of glucose. Using a proteome approach we found that the Deltassb1Deltassb2 strain displays alterations in protein expression and suffers from phenotypic characteristics reminiscent of glucose repression mutants. Microarray analysis revealed a correlation between deregulation on the protein and on the transcript level. Supporting studies uncovered that SSB1 was an effective multicopy suppressor of severe growth defects caused by the Deltareg1 mutation. Suppression of Deltareg1 by high levels of Ssb was coupled to a reduction of Snf1 hyperphosphorylation back to the wild-type phosphorylation level. The data are consistent with a model in which Ssb is crucial for efficient regulation within the SNF1 signaling network, thereby allowing an appropriate response to changing glucose levels.
机译:酵母通过多个互连的信令网络来感知外部能源的可用性。核心成分之一是SNF1,它是哺乳动物AMP激活的蛋白激酶的同源物,在酵母中对于表达葡萄糖抑制基因至关重要。当葡萄糖可用时,1型蛋白磷酸酶Glc7使高磷酸化SNF1失活。去磷酸化需要Reg1,其物理上将Glc7靶向SNF1。在这里,我们显示了在葡萄糖存在下,需要将伴侣Ssb保持在非磷酸化状态的SNF1。使用蛋白质组学方法,我们发现Deltassb1Deltassb2菌株显示出蛋白质表达的变化,并具有让人联想到葡萄糖阻抑突变体的表型特征。微阵列分析揭示了在蛋白质和转录水平上的放松调节之间的相关性。支持性研究发现,SSB1是有效的多拷贝抑制剂,可抑制由Deltareg1突变引起的严重生长缺陷。高水平的Ssb对Deltareg1的抑制作用与Snf1的过度磷酸化水平降低回到野生型磷酸化水平相关。数据与其中Ssb对于SNF1信号网络内有效调节至关重要的模型相一致,从而允许对变化的葡萄糖水平做出适当的响应。

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