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DMP1对CD13/氨肽酶N基因的调控,DMP1是一种受D型细胞周期蛋白拮抗的转录因子。

Regulation of the CD13/aminopeptidase N gene by DMP1, a transcription factor antagonized by D-type cyclins.

作者信息

Inoue K, Sherr C J, Shapiro L H

机构信息

Department of Tumor Cell Biology, St. Jude Children's Research Hospital, Memphis, Tennessee 38105, USA.

出版信息

J Biol Chem. 1998 Oct 30;273(44):29188-94. doi: 10.1074/jbc.273.44.29188.

DOI:10.1074/jbc.273.44.29188
PMID:9786929
Abstract

The binding of the Myb-like DMP1 transcription factor to DNA consensus sequences [CCCG(G/T)ATGT] in artificial promoters is antagonized by D-type cyclins with no requirement for their catalytic partners, cyclin-dependent kinase (CDK) 4 and CDK6. The subset of DMP1 binding sites containing the GGA core can bind Ets family transcription factors Ets-1 and Ets-2. Screening of a series of natural promoters revealed that the CD13/aminopeptidase N (APN; EC 3.4.11.2) promoter could bind and be activated by DMP1. Activation of CD13/APN required both the intact DNA binding and transactivation domains of DMP1 and was inhibited by D-type cyclins, but not by cyclins A, B, C, or H, in a CDK-independent manner. CD13/APN is transactivated by a cooperative interaction between c-Myb bound to its cognate site and Ets-1 tethered to one of three GGA core-containing sites located 30-50 base pairs downstream. DMP1 binds to one of the Ets binding sites (designated Ets C) and synergizes with c-Myb in activating CD13/APN expression. Analysis of nuclear lysates from KG1a early myeloid cells using an oligonucleotide probe containing only the DMP1/Ets C binding site indicated that endogenous DMP1 and a putative Ets family member bind this element in vivo. DMP1-DNA complexes were significantly more stable than those containing the Ets factor. These data indicate that two different Myb family proteins collaborate in regulating APN gene expression and point to a role for DMP1 in normal myeloid cell development.

摘要

Myb样DMP1转录因子与人工启动子中的DNA共有序列[CCCG(G/T)ATGT]的结合受到D型细胞周期蛋白的拮抗,且不需要其催化伴侣细胞周期蛋白依赖性激酶(CDK)4和CDK6。包含GGA核心的DMP1结合位点子集可结合Ets家族转录因子Ets-1和Ets-2。对一系列天然启动子的筛选表明,CD13/氨肽酶N(APN;EC 3.4.11.2)启动子可与DMP1结合并被其激活。CD13/APN的激活需要DMP1完整的DNA结合域和反式激活域,且以不依赖CDK的方式受到D型细胞周期蛋白的抑制,但不受细胞周期蛋白A、B、C或H的抑制。CD13/APN通过与其同源位点结合的c-Myb与 tethered到位于下游30-50个碱基对处的三个含GGA核心位点之一的Ets-1之间的协同相互作用而被反式激活。DMP1与Ets结合位点之一(称为Ets C)结合,并在激活CD13/APN表达方面与c-Myb协同作用。使用仅包含DMP1/Ets C结合位点的寡核苷酸探针分析KG1a早期髓样细胞的核裂解物表明,内源性DMP1和一种假定的Ets家族成员在体内结合该元件。DMP1-DNA复合物比包含Ets因子的复合物显著更稳定。这些数据表明,两种不同的Myb家族蛋白协同调节APN基因表达,并指出DMP1在正常髓样细胞发育中的作用。

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