| Literature DB >> 32783880 |
Racha Chouaib1, Adham Safieddine1, Xavier Pichon2, Arthur Imbert3, Oh Sung Kwon4, Aubin Samacoits5, Abdel-Meneem Traboulsi2, Marie-Cécile Robert2, Nikolay Tsanov2, Emeline Coleno2, Ina Poser6, Christophe Zimmer5, Anthony Hyman6, Hervé Le Hir4, Kazem Zibara7, Marion Peter2, Florian Mueller8, Thomas Walter9, Edouard Bertrand10.
Abstract
Local translation allows spatial control of gene expression. Here, we performed a dual protein-mRNA localization screen, using smFISH on 523 human cell lines expressing GFP-tagged genes. 32 mRNAs displayed specific cytoplasmic localizations with local translation at unexpected locations, including cytoplasmic protrusions, cell edges, endosomes, Golgi, the nuclear envelope, and centrosomes, the latter being cell-cycle-dependent. Automated classification of mRNA localization patterns revealed a high degree of intercellular heterogeneity. Surprisingly, mRNA localization frequently required ongoing translation, indicating widespread co-translational RNA targeting. Interestingly, while P-body accumulation was frequent (15 mRNAs), four mRNAs accumulated in foci that were distinct structures. These foci lacked the mature protein, but nascent polypeptide imaging showed that they were specialized translation factories. For β-catenin, foci formation was regulated by Wnt, relied on APC-dependent polysome aggregation, and led to nascent protein degradation. Thus, translation factories uniquely regulate nascent protein metabolism and create a fine granular compartmentalization of translation.Entities:
Keywords: ASPM; Beta-catenin; RNA localization; RNA transport; co-translational targeting; local translation; smFISH; translation factories
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Year: 2020 PMID: 32783880 DOI: 10.1016/j.devcel.2020.07.010
Source DB: PubMed Journal: Dev Cell ISSN: 1534-5807 Impact factor: 12.270