Abstract

TAB1, a subunit of the kinase TAK1, was phosphorylated by SAPK2a/p38 at Ser423, Thr431 and Ser438 in vitro. TAB1 became phosphorylated at all three sites when cells were exposed to cellular stresses, or stimulated with tumour necrosis factor- (TNF-), interleukin-1 (IL-1) or lipopolysaccharide (LPS). The phosphorylation of Ser423 and Thr431 was prevented if cells were pre-incubated with SB 203580, while the phosphorylation of Ser438 was partially inhibited by PD 184352. Ser423 is the first residue phosphorylated by SAPK2a/p38 that is not followed by proline. The activation of TAK1 was enhanced by SB 203580 in LPS-stimulated macrophages, and by proinflammatory cytokines or osmotic shock in epithelial KB cells or embryonic fibroblasts. The activation of TAK1 by TNF-, IL-1 or osmotic shock was also enhanced in embryonic fibroblasts from SAPK2a/p38-deficient mice, while incubation of these cells with SB 203580 had no effect. Our results suggest that TAB1 participates in a SAPK2a/p38-mediated feedback control of TAK1, which not only limits the activation of SAPK2a/p38 but synchronizes its activity with other signalling pathways that lie downstream of TAK1 (JNK and IKK).