an investigation of a role for u2 snrnp spliceosomal components in regulating transcription一个角色的调查u2 snrnp spliceosomal组件在调节转录.pdfVIP
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an investigation of a role for u2 snrnp spliceosomal components in regulating transcription一个角色的调查u2 snrnp spliceosomal组件在调节转录
An Investigation of a Role for U2 snRNP Spliceosomal
Components in Regulating Transcription
¤
Susannah L. McKay , Tracy L. Johnson*
Molecular Biology Section, Division of Biological Sciences, University of California San Diego, La Jolla, California, United States of America
Abstract
There is mounting evidence to suggest that the synthesis of pre-mRNA transcripts and their subsequent splicing are
coordinated events. Previous studies have implicated the mammalian spliceosomal U2 snRNP as having a novel role in
stimulating transcriptional elongation in vitro through interactions with the elongation factors P-TEFb and Tat-SF1; however,
the mechanism remains unknown [1]. These factors are conserved in Saccharomyces cerevisiae, a fact that suggests that a
similar interaction may occur in yeast to stimulate transcriptional elongation in vivo. To address this possibility we have
looked for evidence of a role for the yeast Tat-SF1 homolog, Cus2, and the U2 snRNA in regulating transcription. Specifically,
we have performed a genetic analysis to look for functional interactions between Cus2 or U2 snRNA and the P-TEFb yeast
homologs, the Bur1/2 and Ctk1/2/3 complexes. In addition, we have analyzed Cus2-deleted or -overexpressing cells and U2
snRNA mutant cells to determine if they show transcription-related phenotypes similar to those displayed by the P-TEFb
homolog mutants. In no case have we been able to observe phenotypes consistent with a role for either spliceosomal factor
in transcription elongation. Furthermore, we did not find evidence for physical interactions between the yeast U2 snRNP
factors and the P-TEFb homologs. These results suggest that in vivo, S. cerevisiae do not exhibit functional or physical
interactions similar to those exhibited by their mammalian counterparts in vitro. The signific
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