4.6 Article

Role of p38 in stress activation of Sp1

Journal

GENE
Volume 379, Issue -, Pages 51-61

Publisher

ELSEVIER SCIENCE BV
DOI: 10.1016/j.gene.2006.04.012

Keywords

filamin A; Spl; mechanical force; stress; MAP kinases; promoter activity

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Cell stressors such as physical forces can activate Sp1-dependent genes but the regulatory mechanisms are not defined. We determined if the stress-induced MAP kinase, p38, can phosphorylate Sp1 and thereby regulate the Sp1 target gene FLNA. We used Rat-2 cells and human gingival fibroblasts to examine stress-induced activation of an Sp1-dependent gene and SL2 cells, an Sp1-deficient model system, to facilitate interaction studies of transfected Sp1 with regulatory factors. Mechanical stress applied to Rat-2 cells increased promoter activity of the Sp1 target gene filamin A by > 5-fold; activation was blocked by mutations to Sp1 binding sites in the filamin A promoter. Transfection experiments in SL2 cells with Sp1 expression vectors showed that when co-transfected with constitutively active p38, wild-type Spl but not an Spl binding mutant, increased promoter activity of the Spl target gene, filamin A, and enhanced binding of nuclear extracts to a filamin A promoter oligonucleotide. Filamin A promoter activity was blocked by dominant negative p38. Spl that was phosphorylated at Thr(453) and Thr(739) by constitutively active p38 bound to the filamin A promoter more effectively than un-phosphorylated Spl. Recombinant active p38 phosphorylated wild-type Spl in vitro while the Spl Thr(453)Thr(739) double mutant protein showed > 3-fold reduction of phosphorylation. We conclude that stress activation of p38 phosphorylates Spl at specific threonine residues, modifications which in turn enhance the expression of Sp1-dependent genes. (c) 2006 Elsevier B.V. All rights reserved.

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