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Phosphate-Activated Cyclin-Dependent Kinase Stabilizes G1 Cyclin To Trigger Cell Cycle Entry

机译:磷酸激活的细胞周期蛋白依赖性激酶稳定G1细胞周期蛋白触发细胞周期进入。

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摘要

G1 cyclins, in association with a cyclin-dependent kinase (CDK), are universal activators of the transcriptional G1-S machinery during entry into the cell cycle. Regulation of cyclin degradation is crucial for coordinating progression through the cell cycle, but the mechanisms that modulate cyclin stability to control cell cycle entry are still unknown. Here, we show that a lack of phosphate downregulates Cln3 cyclin and leads to G1 arrest in Saccharomyces cerevisiae. The stability of Cln3 protein is diminished in strains with low activity of Pho85, a phosphate-sensing CDK. Cln3 is an in vitro substrate of Pho85, and both proteins interact in vivo. More interestingly, cells that carry a CLN3 allele encoding aspartic acid substitutions at the sites of Pho85 phosphorylation maintain high levels of Cln3 independently of Pho85 activity. Moreover, these cells do not properly arrest in G1 in the absence of phosphate and they die prematurely. Finally, the activity of Pho85 is essential for accumulating Cln3 and for reentering the cell cycle after phosphate refeeding. Taken together, our data indicate that Cln3 is a molecular target of the Pho85 kinase that is required to modulate cell cycle entry in response to environmental changes in nutrient availability.
机译:G1细胞周期蛋白与细胞周期蛋白依赖性激酶(CDK)结合,是进入细胞周期过程中转录G1-S机制的通用激活因子。细胞周期蛋白降解的调节对于协调整个细胞周期的进展至关重要,但是调节细胞周期蛋白稳定性以控制细胞周期进入的机制仍然未知。在这里,我们表明缺乏磷酸盐下调Cln3细胞周期蛋白,并导致酿酒酵母中的G1逮捕。 Cln3蛋白的稳定性在低活性Pho85(一种磷酸盐感应CDK)的菌株中会降低。 Cln3是Pho85的体外底物,并且两种蛋白都在体内相互作用。更有趣的是,在Pho85磷酸化位点上携带编码天冬氨酸取代的CLN3等位基因的细胞可独立于Pho85活性而维持高水平的Cln3。而且,这些细胞在不存在磷酸盐的情况下不能适当地滞留在G1中,并且过早死亡。最后,Pho85的活性对于积累Cln3和重新输入磷酸盐后重新进入细胞周期至关重要。两者合计,我们的数据表明Cln3是Pho85激酶的分子靶标,它是调节细胞周期进入以响应营养物可利用性的环境变化所必需的。

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