Human DDX6 regulates translation and decay of inefficiently translated mRNAs

Author:

Weber Ramona12ORCID,Chang Chung-Te13ORCID

Affiliation:

1. Department of Biochemistry, Max Planck Institute for Developmental Biology

2. Institute for Regenerative Medicine (IREM), University of Zurich

3. Institute of Biochemistry and Molecular Biology, National Yang Ming Chiao Tung University

Abstract

Recent findings indicate that the translation elongation rate influences mRNA stability. One of the factors that has been implicated in this link between mRNA decay and translation speed is the yeast DEAD-box helicase Dhh1p. Here, we demonstrated that the human ortholog of Dhh1p, DDX6, triggers the deadenylation-dependent decay of inefficiently translated mRNAs in human cells. DDX6 interacts with the ribosome through the Phe-Asp-Phe (FDF) motif in its RecA2 domain. Furthermore, RecA2-mediated interactions and ATPase activity are both required for DDX6 to destabilize inefficiently translated mRNAs. Using ribosome profiling and RNA sequencing, we identified two classes of endogenous mRNAs that are regulated in a DDX6-dependent manner. The identified targets are either translationally regulated or regulated at the steady-state-level and either exhibit signatures of poor overall translation or of locally reduced ribosome translocation rates. Transferring the identified sequence stretches into a reporter mRNA caused translation- and DDX6-dependent degradation of the reporter mRNA. In summary, these results identify DDX6 as a crucial regulator of mRNA translation and decay triggered by slow ribosome movement and provide insights into the mechanism by which DDX6 destabilizes inefficiently translated mRNAs.

Funder

National Science and Technology Council

Yen Tjing Ling Medical Foundation

Publisher

eLife Sciences Publications, Ltd

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