par Gueydan, Cyril 
;Droogmans, Louis ;Chalon, Pascale;Huez, Georges ;Caput, Daniel;Kruys, Véronique
Référence The Journal of biological chemistry, 274, 4, page (2322-2326)
Publication Publié, 1999-01
;Droogmans, Louis ;Chalon, Pascale;Huez, Georges ;Caput, Daniel;Kruys, Véronique Référence The Journal of biological chemistry, 274, 4, page (2322-2326)
Publication Publié, 1999-01
Article révisé par les pairs
| Résumé : | In monocyte/macrophages, the translation of tumor necrosis factor alpha (TNF-alpha) mRNA is tightly regulated. In unstimulated cells, translation of TNF-alpha mRNA is blocked. Upon stimulation with lipopolysaccharides, this repression is overcome, and the mRNA becomes efficiently translated. The key element in this regulation is the AU-rich element (ARE). We have previously reported the binding of two cytosolic protein complexes to the TNF-alpha mRNA ARE. One of these complexes (complex 1) forms with extracts of both unstimulated and lipopolysaccharide-stimulated macrophages and requires a large fragment of the ARE containing clustered AUUUA pentamers. The other complex (complex 2) is only detected after cell activation, binds to a minimal UUAUUUAUU nonamer, and is composed of a 55-kDa protein. Here, we report the identification of the RNA-binding protein TIAR as a protein involved in complex 1. The RNA sequence bound by TIAR and the cytoplasmic localization of this protein in macrophages argue for an involvement of TIAR in TNF mRNA posttranscriptional regulation. |
