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人类细胞周期蛋白D结合Myb样蛋白(hDMP1)的可变剪接产生一种截短的蛋白质异构体,该异构体改变巨噬细胞分化模式。

Alternative splicing of the human cyclin D-binding Myb-like protein (hDMP1) yields a truncated protein isoform that alters macrophage differentiation patterns.

作者信息

Tschan Mario P, Fischer Kimberlee M, Fung Vivian S, Pirnia Farzaneh, Borner Markus M, Fey Martin F, Tobler Andreas, Torbett Bruce E

机构信息

Scripps Research Institute, Department of Molecular and Experimental Medicine, La Jolla, California 92037, USA.

出版信息

J Biol Chem. 2003 Oct 31;278(44):42750-60. doi: 10.1074/jbc.M307067200. Epub 2003 Aug 12.

DOI:10.1074/jbc.M307067200
PMID:12917399
Abstract

We have cloned two novel, alternatively spliced messages of human cyclin D-binding Myb-like protein (hDMP1). The known, full-length protein has been named hDMP1alpha and the new isoforms, hDMP1beta and hDMP1gamma. The hDMP1alpha, -beta, and -gamma splice variants have unique expression patterns in normal hematopoietic cells; hDMP1beta mRNA transcripts are strongly expressed in quiescent CD34+ cells and freshly isolated peripheral blood leukocytes, as compared with hDMP1alpha. In contrast, activated T-cells and developing myeloid cells, macrophages, and granulocytes express low levels of hDMP1beta transcripts, and hDMP1gamma is ubiquitously and weakly expressed. Mouse Dmp1 has been shown to activate CD13/aminopeptidase N (APN) and p19ARF gene expression via binding to canonical DNA recognition sites in the respective promoters. Assessment of CD13/APN promoter responsiveness demonstrated that hDMP1alpha but not hDMP1beta and -gamma, is a transcriptional activator. Furthermore, hDMP1beta was found to inhibit the CD13/APN promoter transactivation ability of hDMP1alpha. Stable, ectopic expression of hDMP1beta and, to a lesser extent hDMP1gamma, reduced endogenous cell surface levels of CD13/APN in U937 cells. Moreover, stable, ectopic expression of hDMP1beta altered phorbol 12-myristate 13-acetate-induced terminal differentiation of U937 cells to macrophages and resulted in maintenance of proliferation. These results demonstrate that hDMP1beta antagonizes hDMP1alpha activity and suggest that cellular functions of hDMP1 may be regulated by cellular hDMP1 isoform levels.

摘要

我们克隆了人细胞周期蛋白D结合Myb样蛋白(hDMP1)的两种新的可变剪接转录本。已知的全长蛋白已被命名为hDMP1α,新的异构体为hDMP1β和hDMP1γ。hDMP1α、β和γ剪接变体在正常造血细胞中有独特的表达模式;与hDMP1α相比,hDMP1β mRNA转录本在静止的CD34+细胞和新鲜分离的外周血白细胞中强烈表达。相反,活化的T细胞、发育中的髓系细胞、巨噬细胞和粒细胞表达低水平的hDMP1β转录本,而hDMP1γ则普遍且微弱表达。已证明小鼠Dmp1通过与各自启动子中的典型DNA识别位点结合来激活CD13/氨肽酶N(APN)和p19ARF基因表达。对CD13/APN启动子反应性的评估表明,hDMP1α是转录激活因子,而hDMP1β和γ不是。此外,发现hDMP1β可抑制hDMP1α的CD13/APN启动子反式激活能力。hDMP1β以及程度较轻的hDMP1γ的稳定异位表达降低了U937细胞中内源性CD13/APN的细胞表面水平。此外,hDMP1β的稳定异位表达改变了佛波醇12-肉豆蔻酸酯13-乙酸酯诱导的U937细胞向巨噬细胞的终末分化,并导致增殖维持。这些结果表明hDMP1β拮抗hDMP1α活性,并提示hDMP1的细胞功能可能受细胞内hDMP1异构体水平的调节。

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