Literature DB >> 31271494

U2AF65 assemblies drive sequence-specific splice site recognition.

Manel Tari1, Valérie Manceau2, Jean de Matha Salone1, Asaki Kobayashi1, David Pastré1, Alexandre Maucuer1.   

Abstract

The essential splicing factor U2AF65 is known to help anchoring U2 snRNP at the branch site. Its C-terminal UHM domain interacts with ULM motifs of SF3b155, an U2 snRNP protein. Here, we report a cooperative binding of U2AF65 and the related protein CAPERα to the multi-ULM domain of SF3b155. In addition, we show that the RS domain of U2AF65 drives a liquid-liquid phase separation that is amplified by intronic RNA with repeated pyrimidine tracts. In cells, knockdown of either U2AF65 or CAPERα improves the inclusion of cassette exons that are preceded by such repeated pyrimidine-rich motifs. These results support a model in which liquid-like assemblies of U2AF65 and CAPERα on repetitive pyrimidine-rich RNA sequences are driven by their RS domains, and facilitate the recruitment of the multi-ULM domain of SF3b155. We anticipate that posttranslational modifications and proteins recruited in dynamical U2AF65 and CAPERα condensates may further contribute to the complex mechanisms leading to specific splice site choice that occurs in cells.
© 2019 The Authors.

Entities:  

Keywords:  RBM39; SF3b1; U2AF2; liquid-liquid phase separation; splicing

Mesh:

Substances:

Year:  2019        PMID: 31271494      PMCID: PMC6681011          DOI: 10.15252/embr.201847604

Source DB:  PubMed          Journal:  EMBO Rep        ISSN: 1469-221X            Impact factor:   8.807


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