Analog-sensitive Cdk1 as a tool to study mitotic exit: protein phosphatase 1 is required downstream from Cdk1 inactivation in budding yeast.

IF 4.6 Q2 MATERIALS SCIENCE, BIOMATERIALS
Jason M Keaton, Benjamin G Workman, Linfeng Xie, James R Paulson
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Abstract

We show that specific inactivation of the protein kinase Cdk1/cyclin B (Cdc28/Clb2) triggers exit from mitosis in the budding yeast Saccharomyces cerevisiae. Cells carrying the allele cdc28-as1, which makes Cdk1 (Cdc28) uniquely sensitive to the ATP analog 1NM-PP1, were arrested with spindle poisons and then treated with 1NM-PP1 to inhibit Cdk1. This caused the cells to leave mitosis and enter G1-phase as shown by initiation of rebudding (without cytokinesis), induction of mating projections ("shmoos") by α-factor, stabilization of Sic1, and degradation of Clb2. It is known that Cdk1 must be inactivated for cells to exit mitosis, but our results show that inactivation of Cdk1 is not only necessary but also sufficient to initiate the transition from mitosis to G1-phase. This result suggests a system in which to test requirements for particular gene products downstream from Cdk1 inactivation, for example, by combining cdc28-as1 with conditional mutations in the genes of interest. Using this approach, we demonstrate that protein phosphatase 1 (PPase1; Glc7 in S. cerevisiae) is required for mitotic exit and reestablishment of interphase following Cdk1 inactivation. This system could be used to test the need for other protein phosphatases downstream from Cdk1 inactivation, such as PPase 2A and Cdc14, and it could be combined with phosphoproteomics to gain information about the substrates that the various phosphatases act upon during mitotic exit.

Abstract Image

类似物敏感的Cdk1作为研究有丝分裂退出的工具:出芽酵母中Cdk1失活下游需要蛋白磷酸酶1。
我们发现蛋白激酶Cdk1/细胞周期蛋白B(Cdc28/Clb2)的特异性失活触发出芽酵母酿酒酵母的有丝分裂退出。携带使Cdk1(cdc28)对ATP类似物1NM-PP1唯一敏感的等位基因cdc28-as1的细胞用纺锤体毒素捕获,然后用1NM-PPl处理以抑制Cdk1。这导致细胞离开有丝分裂并进入G1期,如重新构建的开始(没有胞质分裂)、α-因子诱导交配投射(“shmoos”)、Sic1的稳定和Clb2的降解所示。众所周知,细胞必须灭活Cdk1才能退出有丝分裂,但我们的研究结果表明,Cdk1的灭活不仅是必要的,而且足以启动从有丝分裂到G1期的过渡。这一结果表明了一种系统,在该系统中,例如通过将cdc28-as1与感兴趣基因中的条件突变相结合,来测试对Cdk1失活下游特定基因产物的需求。使用这种方法,我们证明了蛋白磷酸酶1(PPase1;酿酒酵母中的Glc7)是Cdk1失活后有丝分裂退出和间期重建所必需的。该系统可用于测试Cdk1失活下游对其他蛋白磷酸酶的需求,如PPase 2A和Cdc14,并可与磷酸蛋白质组学结合,以获得各种磷酸酶在有丝分裂退出过程中作用的底物的信息。
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来源期刊
ACS Applied Bio Materials
ACS Applied Bio Materials Chemistry-Chemistry (all)
CiteScore
9.40
自引率
2.10%
发文量
464
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