In vivo and in vitro modulation of the mRNA-binding activity of iron-regulatory factor. Tissue distribution and effects of cell proliferation, iron levels and redox state

Détails

ID Serval
serval:BIB_F4DDD2359D07
Type
Article: article d'un périodique ou d'un magazine.
Collection
Publications
Institution
Titre
In vivo and in vitro modulation of the mRNA-binding activity of iron-regulatory factor. Tissue distribution and effects of cell proliferation, iron levels and redox state
Périodique
European Journal of Biochemistry
Auteur⸱e⸱s
Mullner  E. W., Rothenberger  S., Muller  A. M., Kuhn  L. C.
ISSN
0014-2956 (Print)
Statut éditorial
Publié
Date de publication
09/1992
Volume
208
Numéro
3
Pages
597-605
Notes
Journal Article
Research Support, Non-U.S. Gov't --- Old month value: Sep 15
Résumé
The mRNA-binding protein, iron-regulatory factor (IRF) has a central role in iron metabolism. It coordinately increases transferrin-receptor mRNA stability and inhibits translation of ferritin and erythroid delta-aminolevulinate synthase mRNA by binding to specific mRNA structures, the iron-responsive elements (IRE). In gel-retardation assays, IRF had a broad tissue distribution, showing activity in cytosolic extracts from 12 mouse organs tested. In all these extracts, IRF could be further activated in vitro by 2-mercaptoethanol. In cultured mouse 3T6 fibroblasts, growth stimulation after low serum arrest increased IRF activity 10-fold, mainly through activation of existing inactive IRF. No change was observed during progression of 3T6 cells through the cell cycle. IRF activation by iron chelators has been postulated to result in the reduction of an intramolecular sulfhydryl group. In a search for redox conditions that regulate IRE binding of IRF, we studied several compounds in vitro or in vivo. Hemin, known to inactivate IRF in vivo, showed a similar, reversible effect in vitro, presumably by oxidizing IRF. However, this did not appear to be relevant for the mode of IRF regulation in vivo. Addition of protoporphyrin IX to intact cells induced IRF activity almost to the same extent as desferrioxamine. This effect was inhibited by iron salts, indicating that IRF is activated in vivo through depletion of a chelatable iron pool. In vitro activation by reductants other than 2-mercaptoethanol suggested some selectivity in their access to relevant sulfhydryl groups, but did not reveal which natural redox-sensitive compound might regulate IRF in vivo. However, in cultured cells, inactivation of free IRF by the sulfhydryl-specific oxidizing agent diamide was much more rapidly reversed than inactivation by iron salts. This indicates the direct involvement of a cellular reductant in setting IRF activity and suggests a rate-limiting IRF conformation that is reached only in the presence of iron, but not after diamide oxidation.
Mots-clé
Animals *Cell Cycle Iron/metabolism Iron-Regulatory Proteins L Cells (Cell Line) Mice Mice, Inbred BALB C Oxidation-Reduction RNA, Messenger/*metabolism RNA-Binding Proteins/*metabolism Tissue Distribution
Pubmed
Web of science
Création de la notice
25/01/2008 14:36
Dernière modification de la notice
20/08/2019 16:21
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