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Letters to Nature
Nature 428, 959-963 (29 April 2004) | doi:10.1038/nature02521; Received 19 December 2003; Accepted 23 March 2004
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Section Chief of Molecular Diagnostics and Medical Director of Molecular Diagnotics Laboratory
- M. D. Anderson Cancer Center
- Houston, Texas, USA
Professor / Reader
- LSTM
- Liverpool, United Kingdom
Splicing of oskar RNA in the nucleus is coupled to its cytoplasmic localization
Olivier Hachet & Anne Ephrussi
- European Molecular Biology Laboratory, Meyerhofstrasse 1, Postfach 10.2209, D-69117 Heidelberg, Germany
Correspondence to: Anne Ephrussi Email: ephrussi@embl-heidelberg.de
Abstract
oskar messenger RNA localization at the posterior pole of the Drosophila oocyte is essential for germline and abdomen formation in the future embryo1, 2. The nuclear shuttling proteins Y14/Tsunagi and Mago nashi are required for oskar mRNA localization, and they co-localize with oskar mRNA at the posterior pole of the oocyte3, 4, 5. Their human homologues, Y14/RBM8 and Magoh, are core components of the exon–exon junction complex (EJC)6, 7, 8, 9. The EJC is deposited on mRNAs in a splicing-dependent manner, 20–24 nucleotides upstream of exon–exon junctions, independently of the RNA sequence6, 7, 8. This indicates a possible role of splicing in oskar mRNA localization, challenging the established notion that the oskar 3' untranslated region (3'UTR) is sufficient for this process. Here we show that splicing at the first exon–exon junction of oskar RNA is essential for oskar mRNA localization at the posterior pole. We revisit the issue of sufficiency of the oskar 3'UTR for posterior localization and show that the localization of unrelated transcripts bearing the oskar 3'UTR is mediated by endogenous oskar mRNA. Our results reveal an important new function for splicing: regulation of messenger ribonucleoprotein complex assembly and organization for mRNA cytoplasmic localization.
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