4.7 Article

Regulated Expression of the α Isoform of the Human Thromboxane A2 Receptor during Megakaryocyte Differentiation: A Coordinated Role for WT1, Egr1, and Sp1

Journal

JOURNAL OF MOLECULAR BIOLOGY
Volume 394, Issue 1, Pages 29-45

Publisher

ACADEMIC PRESS LTD- ELSEVIER SCIENCE LTD
DOI: 10.1016/j.jmb.2009.09.007

Keywords

thromboxane receptor gene; megakaryocytic differentiation; WT1; Egr1; Sp1

Funding

  1. The Wellcome Trust
  2. Science Foundation, Ireland
  3. The Health Research Board (Ireland)

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Thromboxane plays an essential role in hemostasis, regulating platelet aggregation and vessel tone. In humans, it signals through the TP alpha and TP beta isoforms that are transcriptionally regulated by distinct promoters Prm1 and Prm3, respectively. Herein, the consequence of megakaryocytic differentiation on Prm1-directed TP alpha expression was investigated. Phorbol 12-myristate 13-acetate (PMA) treatment substantially increased TP alpha mRNA and Prm1-directed gene expression in human erythroleukemia and K562 cells. Deletional analyses localized the major responsive element(s) to the upstream -8500 to -7504 region while mutation of four WT1/Egr1/Sp1 cis elements therein established that each contributes to the induction. Moreover, PMA increased Egr1, but not WT1 or Sp1, expression while the NGFI-A-binding protein 1 co-repressor impaired PMA induction of Egr1- and Prm1-directed gene expression. Chromatin immunoprecipitations established that WT1 is predominantly bound in vivo to the 5' Prm1 region in non-differentiated human erythroleukemia cells. In response to PMA, there was initial induction in Egr1 and associated reduction in WT1 binding to Prm1 in vivo, which was displaced by Sp1 following sustained treatment. Collectively, data establish that regulated WT1 followed by sequential Egr1 and Sp1 binding to elements within Prm1 mediate repression and subsequent induction of TP alpha during differentiation into the megakaryocytic phenotype, shedding significant insights into factors regulating TP alpha expression therein. (C) 2009 Elsevier Ltd. All rights reserved.

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