| Literature DB >> 34555349 |
Jade Sales-Lee1, Daniela S Perry1, Bradley A Bowser2, Jolene K Diedrich3, Beiduo Rao1, Irene Beusch1, John R Yates3, Scott W Roy4, Hiten D Madhani5.
Abstract
We determined that over 40 spliceosomal proteins are conserved between many fungal species and humans but were lost during the evolution of S. cerevisiae, an intron-poor yeast with unusually rigid splicing signals. We analyzed null mutations in a subset of these factors, most of which had not been investigated previously, in the intron-rich yeast Cryptococcus neoformans. We found they govern splicing efficiency of introns with divergent spacing between intron elements. Importantly, most of these factors also suppress usage of weak nearby cryptic/alternative splice sites. Among these, orthologs of GPATCH1 and the helicase DHX35 display correlated functional signatures and copurify with each other as well as components of catalytically active spliceosomes, identifying a conserved G patch/helicase pair that promotes splicing fidelity. We propose that a significant fraction of spliceosomal proteins in humans and most eukaryotes are involved in limiting splicing errors, potentially through kinetic proofreading mechanisms, thereby enabling greater intron diversity.Entities:
Keywords: Cryptococcus neoformans; RNA; Splicing; evolution; fidelity; spliceosome
Mesh:
Year: 2021 PMID: 34555349 PMCID: PMC8967684 DOI: 10.1016/j.cub.2021.09.004
Source DB: PubMed Journal: Curr Biol ISSN: 0960-9822 Impact factor: 10.834