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c-myb通过人cdc2基因5'-侧翼区域中的Myb结合位点反式激活cdc2的表达。

c-myb transactivates cdc2 expression via Myb binding sites in the 5'-flanking region of the human cdc2 gene.

作者信息

Ku D H, Wen S C, Engelhard A, Nicolaides N C, Lipson K E, Marino T A, Calabretta B

机构信息

Department of Microbiology, Thomas Jefferson University, Philadelphia, Pennsylvania 19107.

出版信息

J Biol Chem. 1993 Jan 25;268(3):2255-9.

PMID:8420994
Abstract

The c-myb protooncogene is preferentially expressed in hematopoietic cells and is required for cell cycle progression at the G1/S boundary. Because c-myb encodes a transcriptional activator that functions via DNA binding, it is likely that c-myb exerts its biological activity by regulating the transcription of genes required for DNA synthesis and cell cycle progression. One such gene, cdc2, encodes a 34-kDa serine-threonine kinase that appears to be required for G1/S transition in normal human T-lymphocytes. To determine whether c-myb is a transcriptional regulator of cdc2 expression, we subcloned a segment of a cdc2 human genomic clone containing extensive 5'-flanking sequences and part of the first exon. Sequence analysis revealed the presence of two closely spaced Myb binding sites that interact with bacterially synthesized Myb protein within a region extending from nucleotides -410 to -392 upstream of the transcription initiation site. A 465-base pair segment of 5'-flanking sequence containing these sites was linked to the CAT gene and had promoter activity in rodent fibroblasts. Cotransfection of this construct with a full-length human c-myb cDNA driven by the early simian virus 40 promoter resulted in a 6-8-fold enhancement of CAT activity that was abrogated by mutations in the Myb binding sites. These data suggest that c-myb participates in the regulation of cell cycle progression by activating the expression of the cdc2 gene.

摘要

c-myb原癌基因在造血细胞中优先表达,是细胞在G1/S边界进行细胞周期进程所必需的。由于c-myb编码一种通过DNA结合发挥作用的转录激活因子,c-myb很可能通过调节DNA合成和细胞周期进程所需基因的转录来发挥其生物学活性。其中一个这样的基因,cdc2,编码一种34 kDa的丝氨酸-苏氨酸激酶,它似乎是正常人T淋巴细胞中G1/S转换所必需的。为了确定c-myb是否是cdc2表达的转录调节因子,我们亚克隆了一个cdc2人类基因组克隆的片段,该片段包含广泛的5'侧翼序列和第一个外显子的一部分。序列分析显示,在转录起始位点上游从核苷酸-410到-392的区域内存在两个紧密间隔的Myb结合位点,它们与细菌合成的Myb蛋白相互作用。包含这些位点的5'侧翼序列的465碱基对片段与CAT基因相连,并在啮齿动物成纤维细胞中具有启动子活性。用早期猿猴病毒40启动子驱动的全长人类c-myb cDNA与该构建体共转染,导致CAT活性增强6至8倍,而Myb结合位点的突变可消除这种增强。这些数据表明,c-myb通过激活cdc2基因的表达参与细胞周期进程的调节。

相似文献

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c-myb transactivates cdc2 expression via Myb binding sites in the 5'-flanking region of the human cdc2 gene.c-myb通过人cdc2基因5'-侧翼区域中的Myb结合位点反式激活cdc2的表达。
J Biol Chem. 1993 Jan 25;268(3):2255-9.
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