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在酵母细胞周期中开启和关闭转录:Cln/Cdc28激酶在起始点激活结合的转录因子SBF(Swi4/Swi6),而Clb/Cdc28激酶在G2期将其从启动子上置换下来。

Switching transcription on and off during the yeast cell cycle: Cln/Cdc28 kinases activate bound transcription factor SBF (Swi4/Swi6) at start, whereas Clb/Cdc28 kinases displace it from the promoter in G2.

作者信息

Koch C, Schleiffer A, Ammerer G, Nasmyth K

机构信息

Research Institute of Molecular Pathology, Vienna, Austria.

出版信息

Genes Dev. 1996 Jan 15;10(2):129-41. doi: 10.1101/gad.10.2.129.

DOI:10.1101/gad.10.2.129
PMID:8566747
Abstract

When yeast cells reach a critical size in late G1 they simultaneously start budding, initiate DNA synthesis, and activate transcription of a set of genes that includes G1 cyclins CLN1, CLN2, and many DNA synthesis genes. Cell cycle-regulated expression of CLN1, CLN2 genes is attributable to the heteromeric transcription factor complex SBF. SBF is composed of Swi4 and Swi6 and binds to the promoters of CLN1 and CLN2. Different cyclin-Cdc28 complexes have different effects on late G1-specific transcription. Activation of transcription at the G1/S boundary requires Cdc28 and one of the G1 cyclins Cln1-Cln3, whereas repression of SBF-regulated genes in G2 requires the association of Cdc28 with G2-specific cyclins Clb1-Clb4. Using in vivo genomic footprinting, we show that SBF (Swi4/Swi6) binding to SCB elements (Swi4/Swi6 cell cycle box) in the CLN2 promoter is cell cycle regulated. SBF binds to the promoter prior to the activation of transcription in late G1, suggesting that Cln/Cdc28 kinase regulates the ability of previously bound SBF to activate transcription. In contrast, SBF dissociates from the CLN2 promoter when transcription is repressed during G2 and M phases, suggesting that Clb1-Clb4 repress SBF activity by inhibiting its DNA-binding activity. Switching transcription on and off by different mechanisms could be important to ensure that Clns are activated only once per cell cycle and could be a conserved feature of cell cycle-regulated transcription.

摘要

当酵母细胞在G1晚期达到临界大小时,它们会同时开始出芽、启动DNA合成,并激活一组基因的转录,这组基因包括G1细胞周期蛋白CLN1、CLN2以及许多DNA合成基因。CLN1、CLN2基因的细胞周期调控表达归因于异源转录因子复合物SBF。SBF由Swi4和Swi6组成,并与CLN1和CLN2的启动子结合。不同的细胞周期蛋白 - Cdc28复合物对G1晚期特异性转录有不同影响。在G1/S边界处的转录激活需要Cdc28和G1细胞周期蛋白Cln1 - Cln3中的一种,而在G2期对SBF调控基因的抑制则需要Cdc28与G2特异性细胞周期蛋白Clb1 - Clb4结合。通过体内基因组足迹分析,我们发现SBF(Swi4/Swi6)与CLN2启动子中的SCB元件(Swi4/Swi6细胞周期框)的结合是受细胞周期调控的。SBF在G1晚期转录激活之前就与启动子结合,这表明Cln/Cdc28激酶调节先前结合的SBF激活转录的能力。相反,当在G2期和M期转录受到抑制时,SBF会从CLN2启动子上解离,这表明Clb1 - Clb4通过抑制其DNA结合活性来抑制SBF活性。通过不同机制开启和关闭转录对于确保每个细胞周期中Cln仅被激活一次可能很重要,并且可能是细胞周期调控转录的一个保守特征。

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