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人类核糖体RNA合成的有丝分裂沉默:cdc2/细胞周期蛋白B介导的磷酸化使启动子选择性因子SL1失活。

Mitotic silencing of human rRNA synthesis: inactivation of the promoter selectivity factor SL1 by cdc2/cyclin B-mediated phosphorylation.

作者信息

Heix J, Vente A, Voit R, Budde A, Michaelidis T M, Grummt I

机构信息

Division of Molecular Biology of the Cell II, German Cancer Research Center, D-69120 Heidelberg, Germany.

出版信息

EMBO J. 1998 Dec 15;17(24):7373-81. doi: 10.1093/emboj/17.24.7373.

Abstract

We have used a reconstituted cell-free transcription system to investigate the molecular basis of mitotic repression of RNA polymerase I (pol I) transcription. We demonstrate that SL1, the TBP-containing promoter-binding factor, is inactivated by cdc2/cyclin B-directed phosphorylation, and reactivated by dephosphorylation. Transcriptional inactivation in vitro is accompanied by phosphorylation of two subunits, e.g. TBP and hTAFI110. To distinguish whether transcriptional repression is due to phosphorylation of TBP, hTAFI110 or both, SL1 was purified from two HeLa cell lines that express either full-length or the core domain of TBP only. Both TBP-TAFI complexes exhibit similar activity and both are repressed at mitosis, indicating that the variable N-terminal domain which contains multiple target sites for cdc2/cyclin B phosphorylation is dispensable for mitotic repression. Protein-protein interaction studies reveal that mitotic phosphorylation impairs the interaction of SL1 with UBF. The results suggest that phosphorylation of SL1 is used as a molecular switch to prevent pre-initiation complex formation and to shut down rDNA transcription at mitosis.

摘要

我们利用重组的无细胞转录系统来研究RNA聚合酶I(pol I)转录的有丝分裂抑制的分子基础。我们证明,含TBP的启动子结合因子SL1被cdc2/细胞周期蛋白B介导的磷酸化作用失活,并通过去磷酸化作用重新激活。体外转录失活伴随着两个亚基的磷酸化,例如TBP和hTAFI110。为了区分转录抑制是由于TBP、hTAFI110还是两者的磷酸化作用,从仅表达全长或TBP核心结构域的两种HeLa细胞系中纯化了SL1。两种TBP-TAFI复合物表现出相似的活性,并且在有丝分裂时均被抑制,这表明含有多个cdc2/细胞周期蛋白B磷酸化靶点的可变N末端结构域对于有丝分裂抑制是可有可无的。蛋白质-蛋白质相互作用研究表明,有丝分裂磷酸化会损害SL1与UBF的相互作用。结果表明,SL1的磷酸化被用作一种分子开关,以防止起始前复合物的形成,并在有丝分裂时关闭rDNA转录。

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