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TORC1 and TORC2 work together to regulate ribosomal protein S6 phosphorylation in Saccharomyces cerevisiae

机译:TORC1和TORC2共同调节酿酒酵母中的核糖体蛋白S6磷酸化

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摘要

Nutrient-sensitive phosphorylation of the S6 protein of the 40S subunit of the eukaryote ribosome is highly conserved. However, despite four decades of research, the functional consequences of this modification remain unknown. Revisiting this enigma in Saccharomyces cerevisiae, we found that the regulation of Rps6 phosphorylation on Ser-232 and Ser-233 is mediated by both TOR complex 1 (TORC1) and TORC2. TORC1 regulates phosphorylation of both sites via the poorly characterized AGC-family kinase Ypk3 and the PP1 phosphatase Glc7, whereas TORC2 regulates phosphorylation of only the N-terminal phosphosite via Ypk1. Cells expressing a nonphosphorylatable variant of Rps6 display a reduced growth rate and a 40S biogenesis defect, but these phenotypes are not observed in cells in which Rps6 kinase activity is compromised. Furthermore, using polysome profiling and ribosome profiling, we failed to uncover a role of Rps6 phosphorylation in either global translation or translation of individual mRNAs. Taking the results together, this work depicts the signaling cascades orchestrating Rps6 phosphorylation in budding yeast, challenges the notion that Rps6 phosphorylation plays a role in translation, and demonstrates that observations made with Rps6 knock-ins must be interpreted cautiously.
机译:真核生物核糖体40S亚基S6蛋白的营养敏感磷酸化高度保守。但是,尽管进行了四十年的研究,但这种修饰的功能后果仍然未知。回顾酿酒酵母中的这个谜,我们发现Ser-232和Ser-233上Rps6磷酸化的调控是由TOR复合物1(TORC1)和TORC2介导的。 TORC1通过特征较差的AGC家族激酶Ypk3和PP1磷酸酶Glc7调节两个位点的磷酸化,而TORC2仅通过Ypk1调节N末端磷酸位的磷酸化。表达Rps6不可磷酸化变体的细胞显示出降低的生长速率和40S生物发生缺陷,但在其中Rps6激酶活性受到损害的细胞中未观察到这些表型。此外,使用多核糖体分析和核糖体分析,我们未能揭示Rps6磷酸化在整体翻译或单个mRNA翻译中的作用。结合结果,这项工作描述了在发芽酵母中协调Rps6磷酸化的信号级联,挑战了Rps6磷酸化在翻译中起作用的观点,并证明必须谨慎解释Rps6敲入的观察结果。

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