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c-ets/PU.1和c-myb原癌基因产物在调控人及小鼠集落刺激因子-1受体(c-fms)基因的巨噬细胞特异性启动子中的相反作用。

Opposing actions of c-ets/PU.1 and c-myb protooncogene products in regulating the macrophage-specific promoters of the human and mouse colony-stimulating factor-1 receptor (c-fms) genes.

作者信息

Reddy M A, Yang B S, Yue X, Barnett C J, Ross I L, Sweet M J, Hume D A, Ostrowski M C

机构信息

Department of Microbiology, Duke University Medical Center, Durham, North Carolina 27710.

出版信息

J Exp Med. 1994 Dec 1;180(6):2309-19. doi: 10.1084/jem.180.6.2309.

Abstract

The receptor for macrophage colony stimulating factor (CSF-1), the c-fms gene product, is a key determinant in the differentiation of monocytic phagocytes. Dissection of the human and mouse c-fms proximal promoters revealed opposing roles for nuclear protooncogenes in the transcriptional regulation of this gene. On the one hand, c-ets-1, c-ets-2, and the macrophage-specific factor PU.1, but not the ets-factor PEA3, trans-activated the c-fms proximal promoter. On the other hand c-myb repressed proximal promoter activity in macrophages and blocked the action of c-ets-1 and c-ets-2. Basal c-fms promoter activity was almost undetectable in the M1 leukaemia line, which expressed high levels of c-myb, but was activated as cells differentiated in response to leukemia inhibitory factor and expressed c-fms mRNA. The repressor function of c-myb depended on the COOH-terminal domain of the protein. We propose that ets-factors are necessary for the tissue-restricted expression of c-fms and that c-myb acts to ensure correct temporal expression of c-fms during myeloid differentiation.

摘要

巨噬细胞集落刺激因子(CSF-1)的受体,即c-fms基因产物,是单核吞噬细胞分化的关键决定因素。对人和小鼠c-fms近端启动子的剖析揭示了核原癌基因在该基因转录调控中的相反作用。一方面,c-ets-1、c-ets-2和巨噬细胞特异性因子PU.1,但不是ets因子PEA3,可反式激活c-fms近端启动子。另一方面,c-myb抑制巨噬细胞中近端启动子的活性,并阻断c-ets-1和c-ets-2的作用。在表达高水平c-myb的M1白血病细胞系中,c-fms启动子的基础活性几乎检测不到,但随着细胞在白血病抑制因子的作用下分化并表达c-fms mRNA,其活性被激活。c-myb的抑制功能依赖于该蛋白的COOH末端结构域。我们提出,ets因子对于c-fms的组织限制性表达是必需的,并且c-myb在髓系分化过程中起作用以确保c-fms的正确时间表达。

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