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Gene Expression

Absence of Dbp2p Alters Both Nonsense-Mediated mRNA Decay and rRNA Processing

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Pages 7366-7379 | Received 23 May 2001, Accepted 07 Aug 2001, Published online: 27 Mar 2023
 

Abstract

Dbp2p, a member of the large family of DEAD-box proteins and a yeast homolog of human p68, was shown to interact with Upf1p, an essential component of the nonsense-mediated mRNA decay pathway. Dbp2p:Upf1p interaction occurs within a large conserved region in the middle of Upf1p that is largely distinct from its Nmd2p and Sup35/45p interaction domains. Deletion of DBP2, or point mutations within its highly conserved DEAD-box motifs, increased the abundance of nonsense-containing transcripts, leading us to conclude that Dbp2p also functions in the nonsense-mediated mRNA decay pathway. Dbp2p, like Upf1p, acts before or at decapping, is predominantly cytoplasmic, and associates with polyribosomes. Interestingly, Dbp2p also plays an important role in rRNA processing. In dbp2Δ cells, polyribosome profiles are deficient in free 60S subunits and the mature 25S rRNA is greatly reduced. The ribosome biogenesis phenotype, but not the mRNA decay function, of dbp2Δ cells can be complemented by the human p68 gene. We propose a unifying model in which Dbp2p affects both nonsense-mediated mRNA decay and rRNA processing by altering rRNA structure, allowing specific processing events in one instance and facilitating dissociation of the translation termination complex in the other.

ACKNOWLEDGMENTS

This work was supported by a grant to A.J. (GM27757) from the National Institutes of Health and a postdoctoral fellowship to D.M. from the Medical Foundation/Charles A. King Trust.

We are indebted to Richard Iggo for helpful information, Stanley Hollenberg, Richard Iggo, Elizabeth Jones, David Lane, and Stuart Peltz for plasmids, antibodies, and yeast strains, and the members of the Jacobson lab for their experimental advice and editorial comments.

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