A network of DZF proteins controls alternative splicing regulation and fidelity

Author:

Haque Nazmul1,Will Alexander2,Cook Atlanta G2ORCID,Hogg J Robert1ORCID

Affiliation:

1. Biochemistry and Biophysics Center, National Heart, Lung, and Blood Institute, National Institutes of Health , Bethesda , MD 20892 , USA

2. Wellcome Centre for Cell Biology, School of Biological Sciences, University of Edinburgh, Max Born Crescent , Edinburgh  EH9 3BF, UK

Abstract

Abstract Proteins containing DZF (domain associated with zinc fingers) modules play important roles throughout gene expression, from transcription to translation. Derived from nucleotidyltransferases but lacking catalytic residues, DZF domains serve as heterodimerization surfaces between DZF protein pairs. Three DZF proteins are widely expressed in mammalian tissues, ILF2, ILF3 and ZFR, which form mutually exclusive ILF2–ILF3 and ILF2–ZFR heterodimers. Using eCLIP-Seq, we find that ZFR binds across broad intronic regions to regulate the alternative splicing of cassette and mutually exclusive exons. ZFR preferentially binds dsRNA in vitro and is enriched on introns containing conserved dsRNA elements in cells. Many splicing events are similarly altered upon depletion of any of the three DZF proteins; however, we also identify independent and opposing roles for ZFR and ILF3 in alternative splicing regulation. Along with widespread involvement in cassette exon splicing, the DZF proteins control the fidelity and regulation of over a dozen highly validated mutually exclusive splicing events. Our findings indicate that the DZF proteins form a complex regulatory network that leverages dsRNA binding by ILF3 and ZFR to modulate splicing regulation and fidelity.

Funder

National Heart, Lung, and Blood Institute

National Institutes of Health

Wellcome Trust

Darwin Trust of Edinburgh

Publisher

Oxford University Press (OUP)

Subject

Genetics

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