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Spatial and temporal translational control of germ cell mRNAs mediated by the eIF4E isoform IFE-1

dc.contributor.authorFriday, Andrew J.
dc.contributor.authorHenderson, Melissa A.
dc.contributor.authorMorrison, J. Kaitlin
dc.contributor.authorHoffman, Jenna L.
dc.contributor.authorKeiper, Brett D.
dc.date.accessioned2020-04-17T17:40:46Z
dc.date.available2020-04-17T17:40:46Z
dc.date.issued2015
dc.description.abstractRegulated mRNA translation is vital for germ cells to produce new proteins in the spatial and temporal patterns that drive gamete development. Translational control involves the de-repression of stored mRNAs and their recruitment by eukaryotic initiation factors (eIFs) to ribosomes. C. elegans expresses five eIF4Es (IFE-1–IFE-5); several have been shown to selectively recruit unique pools of mRNA. Individual IFE knockouts yield unique phenotypes due to inefficient translation of certain mRNAs. Here, we identified mRNAs preferentially translated through the germline-specific eIF4E isoform IFE-1. Differential polysome microarray analysis identified 77 mRNAs recruited by IFE-1. Among the IFE-1-dependent mRNAs are several required for late germ cell differentiation and maturation. Polysome association of gld-1, vab-1, vpr-1, rab-7 and rnp-3 mRNAs relies on IFE-1. Live animal imaging showed IFE-1-dependent selectivity in spatial and temporal translation of germline mRNAs. Altered MAPK activation in oocytes suggests dual roles for IFE-1, both promoting and suppressing oocyte maturation at different stages. This single eIF4E isoform exerts positive, selective translational control during germ cell differentiation.en_US
dc.identifier.doi10.1242/jcs.172684
dc.identifier.urihttp://hdl.handle.net/10342/8201
dc.subjectmRNA translational control, Oogenesis, C. elegans, Translation state array analysis, TSAA, Protein synthesis, Meiotic maturationen_US
dc.titleSpatial and temporal translational control of germ cell mRNAs mediated by the eIF4E isoform IFE-1en_US
dc.typeArticleen_US
ecu.journal.issue24en_US
ecu.journal.nameJournal of Cell Scienceen_US
ecu.journal.pages4487-4498en_US
ecu.journal.volume128en_US

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