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在没有渗透感应器的情况下, Hog1 MAPK 的激活不足以触发酿酒酵母的渗透压应激适应。

Activation of the Hog1 MAPK by the Ssk2/Ssk22 MAP3Ks, in the absence of the osmosensors, is not sufficient to trigger osmostress adaptation in Saccharomyces cerevisiae.

机构信息

Departamento de Genética Molecular, Instituto de Fisiología Celular, Universidad Nacional Autónoma de México, Cd de México, México.

Cell Signaling Research Group, Departament de Ciències, Experimentals i de la Salut, Universitat Pompeu Fabra, Barcelona, Spain.

出版信息

FEBS J. 2018 Mar;285(6):1079-1096. doi: 10.1111/febs.14385. Epub 2018 Jan 30.

DOI:10.1111/febs.14385
PMID:29341399
Abstract

Yeast cells respond to hyperosmotic stress by activating the high-osmolarity glycerol (HOG) pathway, which consists of two branches, Hkr1/Msb2-Sho1 and Sln1, which trigger phosphorylation and nuclear internalization of the Hog1 mitogen-activated protein kinase. In the nucleus, Hog1 regulates gene transcription and cell cycle progression, which allows the cell to respond and adapt to hyperosmotic conditions. This study demonstrates that the uncoupling of the known sensors of both branches of the pathway at the level of Ssk1 and Ste11 impairs cell growth in hyperosmotic medium. However, under these conditions, Hog1 was still phosphorylated and internalized into the nucleus, suggesting the existence of an alternative Hog1 activation mechanism. In the ssk1ste11 mutant, phosphorylated Hog1 failed to associate with chromatin and to activate transcription of canonical hyperosmolarity-responsive genes. Accordingly, Hog1 also failed to induce glycerol production at the levels of a wild-type strain. Inactivation of the Ptp2 phosphatase moderately rescued growth impairment of the ssk1ste11 mutant under hyperosmotic conditions, indicating that downregulation of the HOG pathway only partially explains the phenotypes displayed by the ssk1ste11 mutant. Cell cycle defects were also observed in response to stress when Hog1 was phosphorylated in the ssk1ste11 mutant. Taken together, these observations indicate that Hog1 phosphorylation by noncanonical upstream mechanisms is not sufficient to trigger a protective response to hyperosmotic stress.

摘要

酵母细胞通过激活高渗透压甘油(HOG)途径来应对高渗透压胁迫,该途径由 Hkr1/Msb2-Sho1 和 Sln1 两个分支组成,这两个分支触发 Hog1 丝裂原活化蛋白激酶的磷酸化和核内内化。在细胞核中,Hog1 调节基因转录和细胞周期进程,使细胞能够对高渗透压条件做出反应并适应。本研究表明,在 Ssk1 和 Ste11 水平上,对途径的两个分支的已知传感器进行解偶联,会损害高渗培养基中的细胞生长。然而,在这些条件下,Hog1 仍然被磷酸化并内化到核内,这表明存在替代的 Hog1 激活机制。在 ssk1ste11 突变体中,磷酸化的 Hog1 无法与染色质结合,也无法激活典型的高渗透压响应基因的转录。因此,Hog1 也无法像在野生型菌株中那样诱导甘油的产生。Ptp2 磷酸酶的失活在高渗透压条件下适度挽救了 ssk1ste11 突变体的生长缺陷,这表明 HOG 途径的下调仅部分解释了 ssk1ste11 突变体所表现出的表型。当 Hog1 在 ssk1ste11 突变体中被磷酸化时,也观察到细胞周期缺陷作为对胁迫的反应。总之,这些观察结果表明,非典型上游机制的 Hog1 磷酸化不足以引发对高渗透压胁迫的保护反应。

相似文献

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Activation of the Hog1 MAPK by the Ssk2/Ssk22 MAP3Ks, in the absence of the osmosensors, is not sufficient to trigger osmostress adaptation in Saccharomyces cerevisiae.在没有渗透感应器的情况下, Hog1 MAPK 的激活不足以触发酿酒酵母的渗透压应激适应。
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Osmostress enhances activating phosphorylation of Hog1 MAP kinase by mono-phosphorylated Pbs2 MAP2K.渗透胁迫通过单磷酸化 Pbs2 MAP2K 增强 Hog1 MAP 激酶的激活磷酸化。
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Osmostress enhances activating phosphorylation of Hog1 MAP kinase by mono-phosphorylated Pbs2 MAP2K.
渗透胁迫通过单磷酸化 Pbs2 MAP2K 增强 Hog1 MAP 激酶的激活磷酸化。
EMBO J. 2020 Mar 2;39(5):e103444. doi: 10.15252/embj.2019103444. Epub 2020 Feb 3.
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Hog1-Mediated Rds2 Phosphorylation Alters Glycerophospholipid Composition To Coordinate Osmotic Stress in .Hog1 介导的 Rds2 磷酸化改变甘油磷脂组成以协调渗透压应激。
Appl Environ Microbiol. 2019 Mar 6;85(6). doi: 10.1128/AEM.02822-18. Print 2019 Mar 15.