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HsOrc1基因(一种人类ORC1同源物)的表达通过E2F转录因子受细胞增殖调控。

Expression of the HsOrc1 gene, a human ORC1 homolog, is regulated by cell proliferation via the E2F transcription factor.

作者信息

Ohtani K, DeGregori J, Leone G, Herendeen D R, Kelly T J, Nevins J R

机构信息

Department of Genetics, Howard Hughes Medical Institute, Duke University Medical Center, Durham, North Carolina 27710, USA.

出版信息

Mol Cell Biol. 1996 Dec;16(12):6977-84. doi: 10.1128/MCB.16.12.6977.

Abstract

The initiation of DNA replication in Saccharomyces cerevisiae requires the action of a multisubunit complex of six proteins known as the origin recognition complex (ORC). The identification of higher eukaryotic homologs of several ORC components suggests a universal role for this complex in DNA replication. We now demonstrate that the expression of one of these homologs is regulated by cell proliferation. Expression of the human Orc1 gene (HsOrc1) is low in quiescent cells, and it is then dramatically induced upon stimulation of cell growth. In contrast, expression of the HsOrc2 gene does not appear to be similarly regulated. We have isolated the promoter that regulates HsOrc1 transcription, and we show that the promoter confers cell growth-dependent expression. We also demonstrate that the cell growth control is largely the consequence of E2F-dependent negative transcription control in quiescent cells. Activation of HsOrc1 transcription following growth stimulation requires G1 cyclin-dependent kinase activity, and forced E2F1 expression can bypass this requirement. These results thus provide a direct link between the initiation of DNA replication and the cell growth regulatory pathway involving G1 cyclin-dependent kinases, the Rb tumor suppressor, and E2F.

摘要

酿酒酵母中DNA复制的起始需要一种由六种蛋白质组成的多亚基复合物的作用,该复合物被称为起始识别复合物(ORC)。几种ORC组分的高等真核生物同源物的鉴定表明该复合物在DNA复制中具有普遍作用。我们现在证明这些同源物之一的表达受细胞增殖调控。人Orc1基因(HsOrc1)在静止细胞中的表达较低,在细胞生长受到刺激后会被显著诱导。相比之下,HsOrc2基因的表达似乎没有受到类似的调控。我们分离出了调控HsOrc1转录的启动子,并表明该启动子赋予细胞生长依赖性表达。我们还证明,细胞生长控制在很大程度上是静止细胞中E2F依赖性负转录控制的结果。生长刺激后HsOrc1转录的激活需要G1周期蛋白依赖性激酶活性,而强制表达E2F1可以绕过这一需求。因此,这些结果在DNA复制的起始与涉及G1周期蛋白依赖性激酶、Rb肿瘤抑制因子和E2F的细胞生长调控途径之间建立了直接联系。

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