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裂殖酵母中蛋白激酶C(PKC)直系同源物的差异功能调控

Differential functional regulation of protein kinase C (PKC) orthologs in fission yeast.

作者信息

Madrid Marisa, Vázquez-Marín Beatriz, Soto Teresa, Franco Alejandro, Gómez-Gil Elisa, Vicente-Soler Jero, Gacto Mariano, Pérez Pilar, Cansado José

机构信息

From the Yeast Physiology Group, Department of Genetics and Microbiology, Facultad de Biología, Universidad de Murcia, 30071 Murcia, Spain and

From the Yeast Physiology Group, Department of Genetics and Microbiology, Facultad de Biología, Universidad de Murcia, 30071 Murcia, Spain and.

出版信息

J Biol Chem. 2017 Jul 7;292(27):11374-11387. doi: 10.1074/jbc.M117.786087. Epub 2017 May 23.

Abstract

The two PKC orthologs Pck1 and Pck2 in the fission yeast operate in a redundant fashion to control essential functions, including morphogenesis and cell wall biosynthesis, as well as the activity of the cell integrity pathway and its core element, the MAPK Pmk1. We show here that, despite the strong structural similarity and functional redundancy of these two enzymes, the mechanisms regulating their maturation, activation, and stabilization have a remarkably distinct biological impact on both kinases. We found that, in contrast to Pck2, putative phosphorylation of Pck1 within the conserved activation loop, turn, and hydrophobic motifs is essential for Pck1 stability and biological functions. Constitutive Pck activation promoted dephosphorylation and destabilization of Pck2, whereas it enhanced Pck1 levels to interfere with proper downstream signaling to the cell integrity pathway via Pck2. Importantly, although catalytic activity was essential for Pck1 function, Pck2 remained partially functional independent of its catalytic activity. Our findings suggest that early divergence from a common ancestor in fission yeast involved important changes in the mechanisms regulating catalytic activation and stability of PKC family members to allow for flexible and dynamic control of downstream functions, including MAPK signaling.

摘要

裂殖酵母中的两个蛋白激酶C(PKC)直系同源物Pck1和Pck2以冗余方式发挥作用,以控制包括形态发生和细胞壁生物合成在内的基本功能,以及细胞完整性途径及其核心元件丝裂原活化蛋白激酶(MAPK)Pmk1的活性。我们在此表明,尽管这两种酶在结构上有很强的相似性且功能冗余,但调节它们成熟、激活和稳定的机制对这两种激酶具有显著不同的生物学影响。我们发现,与Pck2不同,保守激活环、转角和疏水基序内Pck1的假定磷酸化对于Pck1的稳定性和生物学功能至关重要。组成型Pck激活促进了Pck2的去磷酸化和不稳定,而它提高了Pck1的水平,从而通过Pck2干扰向细胞完整性途径的适当下游信号传导。重要的是,尽管催化活性对Pck1功能至关重要,但Pck2在其催化活性之外仍保持部分功能。我们的研究结果表明,裂殖酵母中与共同祖先的早期分化涉及调节PKC家族成员催化激活和稳定性的机制的重要变化,以便对包括MAPK信号传导在内的下游功能进行灵活和动态的控制。

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