| Literature DB >> 27315556 |
Ulas Tenekeci1, Michael Poppe1, Knut Beuerlein1, Christin Buro1, Helmut Müller1, Hendrik Weiser1, Daniela Kettner-Buhrow1, Katharina Porada1, Doris Newel1, Ming Xu2, Zhijian J Chen2, Julia Busch3, M Lienhard Schmitz3, Michael Kracht4.
Abstract
Signals and posttranslational modifications regulating the decapping step in mRNA degradation pathways are poorly defined. In this study we reveal the importance of K63-linked ubiquitylation for the assembly of decapping factors, P-body formation, and constitutive decay of instable mRNAs encoding mediators of inflammation by various experimental approaches. K63-branched ubiquitin chains also regulate IL-1-inducible phosphorylation of the P-body component DCP1a. The E3 ligase TRAF6 binds to DCP1a and indirectly regulates DCP1a phosphorylation, expression of decapping factors, and gene-specific mRNA decay. Mutation of six C-terminal lysines of DCP1a suppresses decapping activity and impairs the interaction with the mRNA decay factors DCP2, EDC4, and XRN1, but not EDC3, thus remodeling P-body architecture. The usage of ubiquitin chains for the proper assembly and function of the decay-competent mammalian decapping complex suggests an additional layer of control to allow a coordinated function of decapping activities and mRNA metabolism in higher eukaryotes.Entities:
Keywords: DCP1a; IL-1; K63R ubiquitin; P-body; TRAF6; ubiquitin
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Year: 2016 PMID: 27315556 DOI: 10.1016/j.molcel.2016.05.017
Source DB: PubMed Journal: Mol Cell ISSN: 1097-2765 Impact factor: 17.970