Drosophila miR2 Primarily Targets the m7GpppN Cap Structure for Translational Repression

Agnieszka Zdanowicz, Rolf Thermann, Joanna Kowalska, Jacek Jemielity, Kent Duncan, Thomas Preiss, Edward Darzynkiewicz, Matthias W. Hentze*

*Corresponding author for this work

Research output: Contribution to journalArticlepeer-review

69 Citations (Scopus)

Abstract

Understanding the molecular mechanism(s) of how miRNAs repress mRNA translation is a fundamental challenge in RNA biology. Here we use a validated cell-free system from Drosophila embryos to investigate how miR2 inhibits translation initiation. By screening a library of chemical m7GpppN cap structure analogs, we identified defined modifications of the triphosphate backbone that augment miRNA-mediated inhibition of translation initiation but are "neutral" toward general cap-dependent translation. Interestingly, these caps also augment inhibition by 4E-BP. Kinetic dissection of translational repression and miR2-induced deadenylation shows that both processes proceed largely independently, with establishment of the repressed state involving a slow step. Our data demonstrate a primary role for the m7GpppN cap structure in miRNA-mediated translational inhibition, implicate structural determinants outside the core eIF4E-binding region in this process, and suggest that miRNAs may target cap-dependent translation through a mechanism related to the 4E-BP class of translational regulators.

Original languageEnglish
Pages (from-to)881-888
Number of pages8
JournalMolecular Cell
Volume35
Issue number6
DOIs
Publication statusPublished - 24 Sept 2009
Externally publishedYes

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