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哺乳动物CDC6的细胞周期调控表达依赖于E2F。

Cell cycle-regulated expression of mammalian CDC6 is dependent on E2F.

作者信息

Hateboer G, Wobst A, Petersen B O, Le Cam L, Vigo E, Sardet C, Helin K

机构信息

Department of Experimental Oncology, European Institute of Oncology, 20141 Milan, Italy.

出版信息

Mol Cell Biol. 1998 Nov;18(11):6679-97. doi: 10.1128/MCB.18.11.6679.

Abstract

The E2F transcription factors are essential regulators of cell growth in multicellular organisms, controlling the expression of a number of genes whose products are involved in DNA replication and cell proliferation. In Saccharomyces cerevisiae, the MBF and SBF transcription complexes have functions similar to those of E2F proteins in higher eukaryotes, by regulating the timed expression of genes implicated in cell cycle progression and DNA synthesis. The CDC6 gene is a target for MBF and SBF-regulated transcription. S. cerevisiae Cdc6p induces the formation of the prereplication complex and is essential for initiation of DNA replication. Interestingly, the Cdc6p homolog in Schizosaccharomyces pombe, Cdc18p, is regulated by DSC1, the S. pombe homolog of MBF. By cloning the promoter for the human homolog of Cdc6p and Cdc18p, we demonstrate here that the cell cycle-regulated transcription of this gene is dependent on E2F. In vivo footprinting data demonstrate that the identified E2F sites are occupied in resting cells and in exponentially growing cells, suggesting that E2F is responsible for downregulating the promoter in early phases of the cell cycle and the subsequent upregulation when cells enter S phase. Our data also demonstrate that the human CDC6 protein (hCDC6) is essential and limiting for DNA synthesis, since microinjection of an anti-CDC6 rabbit antiserum blocks DNA synthesis and CDC6 cooperates with cyclin E to induce entry into S phase in cotransfection experiments. Furthermore, E2F is sufficient to induce expression of the endogenous CDC6 gene even in the absence of de novo protein synthesis. In conclusion, our results provide a direct link between regulated progression through G1 controlled by the pRB pathway and the expression of proteins essential for the initiation of DNA replication.

摘要

E2F转录因子是多细胞生物中细胞生长的重要调节因子,控制着许多基因的表达,这些基因的产物参与DNA复制和细胞增殖。在酿酒酵母中,MBF和SBF转录复合体具有与高等真核生物中E2F蛋白类似的功能,通过调节与细胞周期进程和DNA合成相关基因的定时表达来实现。CDC6基因是MBF和SBF调节转录的靶标。酿酒酵母Cdc6p诱导前复制复合体的形成,对DNA复制的起始至关重要。有趣的是,粟酒裂殖酵母中Cdc6p的同源物Cdc18p受DSC1调节,DSC1是MBF在粟酒裂殖酵母中的同源物。通过克隆人类Cdc6p和Cdc18p同源物的启动子,我们在此证明该基因的细胞周期调节转录依赖于E2F。体内足迹数据表明,所鉴定的E2F位点在静止细胞和指数生长细胞中均被占据,这表明E2F负责在细胞周期早期下调启动子,并在细胞进入S期时随后上调。我们的数据还表明,人类CDC6蛋白(hCDC6)对DNA合成至关重要且具有限制作用,因为注射抗CDC6兔抗血清会阻断DNA合成,并且在共转染实验中CDC6与细胞周期蛋白E协同作用诱导进入S期。此外,即使在没有从头蛋白质合成的情况下,E2F也足以诱导内源性CDC6基因的表达。总之,我们的结果提供了一条直接联系,即在由pRB途径控制的G1期调节进程与DNA复制起始所必需的蛋白质表达之间建立了联系。

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