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应激激活蛋白激酶介导的蛋白磷酸酶对细胞完整性通路促分裂原活化蛋白激酶Pmk1p的下调作用。

Stress-activated protein kinase-mediated down-regulation of the cell integrity pathway mitogen-activated protein kinase Pmk1p by protein phosphatases.

作者信息

Madrid Marisa, Núñez Andrés, Soto Teresa, Vicente-Soler Jero, Gacto Mariano, Cansado José

机构信息

Department of Genetics and Microbiology, Facultad de Biología, University of Murcia, 30071 Murcia, Spain.

出版信息

Mol Biol Cell. 2007 Nov;18(11):4405-19. doi: 10.1091/mbc.e07-05-0484. Epub 2007 Aug 29.

Abstract

Fission yeast mitogen-activated protein kinase (MAPK) Pmk1p is involved in morphogenesis, cytokinesis, and ion homeostasis as part of the cell integrity pathway, and it becomes activated under multiple stresses, including hyper- or hypotonic conditions, glucose deprivation, cell wall-damaging compounds, and oxidative stress. The only protein phosphatase known to dephosphorylate and inactivate Pmk1p is Pmp1p. We show here that the stress-activated protein kinase (SAPK) pathway and its main effector, Sty1p MAPK, are essential for proper deactivation of Pmk1p under hypertonic stress in a process regulated by Atf1p transcription factor. We demonstrate that tyrosine phosphatases Pyp1p and Pyp2p, and serine/threonine phosphatase Ptc1p, that negatively regulate Sty1p activity and whose expression is dependent on Sty1p-Atf1p function, are involved in Pmk1p dephosphorylation under osmostress. Pyp1p and Ptc1p, in addition to Pmp1p, also control the basal level of MAPK Pmk1p activity in growing cells and associate with, and dephosphorylate Pmk1p both in vitro and in vivo. Our results with Ptc1p provide the first biochemical evidence for a PP2C-type phosphatase acting on more than one MAPK in yeast cells. Importantly, the SAPK-dependent down-regulation of Pmk1p through Pyp1p, Pyp2p, and Ptc1p was not complete, and Pyp1p and Ptc1p phosphatases are able to negatively regulate MAPK Pmk1p activity by an alternative regulatory mechanism. Our data also indicate that Pmk1p phosphorylation oscillates as a function of the cell cycle, peaking at cell separation during cytokinesis, and that Pmp1p phosphatase plays a main role in regulating this process.

摘要

裂殖酵母丝裂原活化蛋白激酶(MAPK)Pmk1p作为细胞完整性途径的一部分,参与形态发生、胞质分裂和离子稳态,并且在多种应激条件下被激活,包括高渗或低渗条件、葡萄糖剥夺、细胞壁损伤化合物和氧化应激。已知唯一能使Pmk1p去磷酸化并使其失活的蛋白磷酸酶是Pmp1p。我们在此表明,应激激活蛋白激酶(SAPK)途径及其主要效应因子Sty1p MAPK,在由Atf1p转录因子调控的过程中,对于高渗应激下Pmk1p的正确失活至关重要。我们证明,酪氨酸磷酸酶Pyp1p和Pyp2p以及丝氨酸/苏氨酸磷酸酶Ptc1p,它们负向调节Sty1p活性且其表达依赖于Sty1p-Atf1p功能,参与了渗透应激下Pmk1p的去磷酸化过程。除了Pmp1p之外,Pyp1p和Ptc1p还控制生长细胞中MAPK Pmk1p活性的基础水平,并且在体外和体内都与Pmk1p结合并使其去磷酸化。我们对Ptc1p的研究结果为酵母细胞中一种PP2C型磷酸酶作用于多种MAPK提供了首个生化证据。重要的是,通过Pyp1p、Pyp2p和Ptc1p对Pmk1p进行的SAPK依赖性下调并不完全,并且Pyp1p和Ptc1p磷酸酶能够通过另一种调节机制负向调节MAPK Pmk1p活性。我们的数据还表明,Pmk1p的磷酸化作为细胞周期的函数而振荡,在胞质分裂期间细胞分离时达到峰值,并且Pmp1p磷酸酶在调节这一过程中起主要作用。

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