A Snu114–GTP–Prp8 module forms a relay station for efficient splicing in yeast

Author:

Jia Junqiao1,Ganichkin Oleg M1,Preußner Marco2,Absmeier Eva1,Alings Claudia1,Loll Bernhard1ORCID,Heyd Florian2,Wahl Markus C13ORCID

Affiliation:

1. Freie Universität Berlin, Laboratory of Structural Biochemistry, Takustraβe 6, D-14195 Berlin, Germany

2. Freie Universität Berlin, Laboratory of RNA Biochemistry, Takustraβe 6, D-14195 Berlin, Germany

3. Helmholtz-Zentrum Berlin für Materialien und Energie, Macromolecular Crystallography, Albert-Einstein-Straße 15, D-12489 Berlin, Germany

Abstract

Abstract The single G protein of the spliceosome, Snu114, has been proposed to facilitate splicing as a molecular motor or as a regulatory G protein. However, available structures of spliceosomal complexes show Snu114 in the same GTP-bound state, and presently no Snu114 GTPase-regulatory protein is known. We determined a crystal structure of Snu114 with a Snu114-binding region of the Prp8 protein, in which Snu114 again adopts the same GTP-bound conformation seen in spliceosomes. Snu114 and the Snu114–Prp8 complex co-purified with endogenous GTP. Snu114 exhibited weak, intrinsic GTPase activity that was abolished by the Prp8 Snu114-binding region. Exchange of GTP-contacting residues in Snu114, or of Prp8 residues lining the Snu114 GTP-binding pocket, led to temperature-sensitive yeast growth and affected the same set of splicing events in vivo. Consistent with dynamic Snu114-mediated protein interactions during splicing, our results suggest that the Snu114–GTP–Prp8 module serves as a relay station during spliceosome activation and disassembly, but that GTPase activity may be dispensable for splicing.

Funder

Chinese Scholarship Council Fellowship

Peter and Traudl Engelhorn Foundation Post-doctoral Fellowship

Deutsche Forschungsgemeinschaft

Publisher

Oxford University Press (OUP)

Subject

Genetics

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