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巨核细胞分化过程中Gαq启动子上佛波酯12-肉豆蔻酸酯13-乙酸酯(PMA)反应序列。由早期生长反应蛋白-1(EGR-1)和丝裂原活化蛋白激酶(MAP)途径调控。

Phorbol 12-myristate 13-acetate (PMA) responsive sequence in Galphaq promoter during megakaryocytic differentiation. Regulation by EGR-1 and MAP kinase pathway.

作者信息

Jalagadugula Gauthami, Dhanasekaran Danny N, Rao A Koneti

机构信息

Sol Sherry Thrombosis Research Center, Temple University School of Medicine, 3400 N. Broad St., OMS-300, Philadelphia, PA 19140, USA.

出版信息

Thromb Haemost. 2008 Nov;100(5):821-8.

Abstract

Galphaq plays a major role in platelet signal transduction, but little is known regarding its transcriptional regulation. We have reported that Galphaq is upregulated during phorbol 12-myristate 13-acetate (PMA)-induced megakaryocytic transformation of human erythroleukemia (HEL) cells and regulated by EGR-1, an early growth transcription factor. These studies focused on the initial 238 bp of the 5' upstream region of the Galphaq gene. In the present studies we characterize a minimal region -1042/-1037 bp from ATG in the 5' upstream of the Galphaq promoter that is associated with PMA responsiveness. In luciferase reporter gene studies in HEL cells, Galphaq 5' upstream promoter sequence -1042/-1 showed an about four-fold increased activity in PMA-treated compared to untreated cells. Deletion of 6-nt -1042/-1037 eliminated the difference. Gel-shift studies on Galphaq probe (-1042/-1012 bp) revealed binding of EGR-1 with PMA-treated but not untreated nuclear extracts, and this was dependent on the sequence -1042/-1037. Silencing of endogenous EGR-1 inhibited Galphaq induction by PMA. MEK/ERK inhibitor U0126 blocked PMA effect on promoter activity of the -1042/-1 construct. In conclusion, EGR-1 binding to sequence -1042/-1037 bp in Galphaq promoter mediates the induction of Galphaq gene by PMA via the MEK/ERK signaling pathway. These studies provide the first evidence of a PMA-responsive element in Galphaq promoter, and new insights into regulation of Galphaq gene by EGR-1.

摘要

Gαq在血小板信号转导中起主要作用,但其转录调控情况却鲜为人知。我们曾报道,在佛波酯12 -肉豆蔻酸酯13 -乙酸酯(PMA)诱导人红白血病(HEL)细胞发生巨核细胞转化过程中,Gαq表达上调,且受早期生长转录因子EGR - 1调控。这些研究聚焦于Gαq基因5'上游区域起始的238 bp。在本研究中,我们鉴定出Gαq启动子5'上游距ATG - 1042 / - 1037 bp的一个最小区域,该区域与PMA反应性相关。在HEL细胞的荧光素酶报告基因研究中,与未处理细胞相比,Gαq 5'上游启动子序列 - 1042 / - 1在PMA处理的细胞中活性增加了约四倍。缺失6个核苷酸(- 1042 / - 1037)消除了这种差异。对Gαq探针(- 1042 / - 1012 bp)的凝胶迁移实验表明,EGR - 1与PMA处理而非未处理的细胞核提取物结合,且这种结合依赖于 - 1042 / - 1037序列。内源性EGR - 1的沉默抑制了PMA对Gαq的诱导作用。MEK / ERK抑制剂U0126阻断了PMA对 - 1042 / - 1构建体启动子活性的影响。总之,EGR - 1与Gαq启动子中 - 1042 / - 1037 bp序列的结合通过MEK / ERK信号通路介导了PMA对Gαq基因的诱导。这些研究首次提供了Gαq启动子中PMA反应元件的证据,并为EGR - 1对Gαq基因的调控提供了新见解。

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