Identificador persistente para citar o vincular este elemento: http://hdl.handle.net/10553/50581
Título: c-Jun is a downstream target for ceramide-activated protein phosphatase in A431 cells
Autores/as: Reyes, Juan González
Robayna, Ignacio González 
Delgado, Pino Santana 
González, Inmaculada Hernández 
Aguiar, José Quintana 
Estévez Rosas, F. 
Fanjul, Luisa F. 
Ruiz de Galarreta, C. M.
Clasificación UNESCO: 32 Ciencias médicas
2302 Bioquímica
Palabras clave: Tumor-Necrosis-Factor
Sphingolipid Breakdown Products
Signal-Transduction
Cellular-Regulation
Factor-Alpha, et al.
Fecha de publicación: 1996
Publicación seriada: Journal of Biological Chemistry 
Resumen: Stimulation of [H-3]serine-labeled A431 cells with tumor necrosis factor-alpha (TNF alpha) or bacterial sphingomyelinase (SMase) resulted in a rapid decrease (similar to 50% by 15 min) in cellular [H-3]sphingomyelin content and generation of the lipid moiety [H-3]ceramide, which remained elevated 60 min later, Sphingomyelin hydrolysis in response to TNF alpha or bacterial SMase resulted in a time-dependent decrease in the phosphorylation state of c-Jun protein, an effect that was also observed in cells treated with the membrane-permeable ceramide analogue N-hexanoylsphingosine (C-6-ceramide). The rapid dephosphorylation of the c-Jun gene product in response to TNF alpha, SMase, or C-6-ceramide was not observed in A431 cells treated with the serine-threonine phosphatase inhibitor okadaic acid. After the initial steps of previously described methods for the purification of a ceramide-activated protein phosphatase termed CAPP (Dobrowsky, R, T., Kamibayashi, C,, Mumby, M, C., and Hannun, Y. A, (1993) J, Biol, Chen. 268, 15523-15530), we obtained a cytosolic fraction from A431 cells that specifically dephosphorylated P-32(i)-labeled c-Jun protein used as substrate in an immunocomplex phosphatase assay, Phosphatase activity in vitro was apparent only in the presence of ceramide (5 mu m) and was specifically abrogated when okadaic acid (1 nM) was included in the immunocomplex phosphatase assay, These results provide strong evidence for c-Jun as a downstream target for CAPP activated in response to post-TNF signaling in A431 cells.
URI: http://hdl.handle.net/10553/50581
ISSN: 0021-9258
DOI: 10.1074/jbc.271.35.21375
Fuente: Journal Of Biological Chemistry[ISSN 0021-9258],v. 271 (35), p. 21375-21380 (Septiembre 199
Colección:Artículos
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