NF-{kappa}B regulates thrombin-induced ICAM-1 gene expression in cooperation with NFAT by binding to the intronic NF-{kappa}B site in the ICAM-1 gene

doi:10.1152/physiolgenomics.00012.2009

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Physiol. Genomics 38: 42-53, 2009. First published April 7, 2009; doi:10.1152/physiolgenomics.00012.2009
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Received 16 January 2009; accepted in final form 1 April 2009.
Physiological Genomics 38:42-53 (2009)
1094-8341/09 $8.00 © 2009 American Physiological Society

NF- ${kappa}$ B regulates thrombin-induced ICAM-1 gene expression in cooperation with NFAT by binding to the intronic NF- ${kappa}$ B site in the ICAM-1 gene

Jiaping Xue ¹, Prabhakar B. Thippegowda ¹, Guochang Hu ¹, Kurt Bachmaier ¹, John W. Christman ²^,3, Asrar B. Malik ¹^,3 and Chinnaswamy Tiruppathi ¹^,3

¹ Department of Pharmacology, College of Medicine, University of Illinois, Chicago, Illinois
² Department of Medicine, Section of Pulmonary, Critical Care and Sleep Medicine, College of Medicine, University of Illinois, Chicago, Illinois
³ Center for Lung and Vascular Biology, College of Medicine, University of Illinois, Chicago, Illinois

Activation of NF- ${kappa}$ B is essential for protease-activated receptor-1(PAR-1)-mediated ICAM-1 expression in endothelial cells. Herewe show that PAR-1 activation induces binding of both p65/RelAand NFATc1 to the NF- ${kappa}$ B binding site localized in intron-1 ofthe ICAM-1 gene to initiate transcription in endothelial cells.We discovered the presence of two NF- ${kappa}$ B binding sites in intron-1(+70, NF- ${kappa}$ B site 1; +611, NF- ${kappa}$ B site 2) of the human ICAM-1 gene.Chromatin immunoprecipitation results showed that thrombin inducedbinding of p65/RelA and of NFATc1 specifically to intronic NF- ${kappa}$ Bsite 1 of the ICAM-1 gene. Electrophoretic mobility shift andsupershift assays confirmed the binding of p65/RelA and NFATc1to the intronic NF- ${kappa}$ B site 1 in thrombin-stimulated cells. Thrombinincreased the expression of ICAM-1-promoter-intron 1-reporter(–1,385 to +234) construct $~$ 25-fold and mutation of intronicNF- ${kappa}$ B site 1 markedly reduced thrombin-induced reporter expression.Moreover, inhibition of calcineurin, knockdown of either NFATc1or p65/RelA with siRNA significantly reduced thrombin-inducedICAM-1 expression and polymorphonuclear leukocyte adhesion toendothelial cells. In contrast, NFATc1 knockdown had no effecton TNF- ${alpha}$ -induced ICAM-1 expression. Thus these results suggestthat p65/RelA and NFATc1 bind to the intronic NF- ${kappa}$ B site 1 sequenceto induce optimal transcription of the ICAM-1 gene in responseto thrombin in endothelial cells.

endothelial cells; protease-activated receptor-1; tumor necrosis factor- ${alpha}$ ; intercellular adhesion molecule-1; calcineurin; nuclear factor- ${kappa}$ B; nuclear factor of activated T cells

NF-B regulates thrombin-induced ICAM-1 gene expression in cooperation with NFAT by binding to the intronic NF-B site in the ICAM-1 gene

NF- ${kappa}$ B regulates thrombin-induced ICAM-1 gene expression in cooperation with NFAT by binding to the intronic NF- ${kappa}$ B site in the ICAM-1 gene