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DAG1, no gene for RNA regulation?

Academic Article
Publication Date:
2012
abstract:
DAG1 encodes for a precursor protein that liberates the two subunits featured by the dystroglycan (DG) adhesion complex that are involved in an increasing number of cellular functions in a wide variety of cells and tissues. Aside from the proteolytic events producing the alpha and beta subunits, especially the former undergoes extensive "post-production" modifications taking place within the ER/Golgi where its core protein is both N- and O-decorated with sugars. These post-translational events, that are mainly orchestrated by a plethora of certified, or putative, glycosyltransferases, prelude to the excocytosis-mediated trafficking and targeting of the DG complex to the plasma membrane. Extensive genetic and biochemical evidences have been accumulated so far on alpha-DG glycosylation, while little is know on possible regulatory events underlying the chromatine activation, transcription or post-transcription (splicing and escape from the nucleus) of DAG1 or of its mRNA. A scenario is envisaged in which cells would use a sort of preferential, and scarcely regulated, route for DAG1 activation, that would imply fast mRNA transcription, maturation and export to the cytosol, and would prelude to the multiple time-consuming enzymatic post-translational activities needed for its glycosylation. Such a provocative view might be helpful to trigger future work aiming at disclosing the complete molecular mechanisms underlying DAG1 activation and at improving our knowledge of any pre-translational step that is involved in dystroglycan regulation. (C) 2012 Elsevier B.V. All rights reserved.
Iris type:
01.01 Articolo in rivista
Keywords:
Dystroglycan; Large introns; Transcription; Splicing; Nucleus Escape; Post-translational modifications
List of contributors:
Brancaccio, Andrea
Authors of the University:
BRANCACCIO ANDREA
Handle:
https://iris.cnr.it/handle/20.500.14243/240661
Published in:
GENE
Journal
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