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Article Abstract

Splicing in has been shown to proceed cotranscriptionally, but the nature of the coupling remains a subject of debate. Here, we examine the effect of nineteen complex-related splicing factor Prp45 (a homolog of SNW1/SKIP) on cotranscriptional splicing. RNA-sequencing and RT-qPCR showed elevated pre-mRNA levels but only limited reduction of spliced mRNAs in cells expressing C-terminally truncated Prp45, Prp45(1-169). Assays with a series of reporters containing the intron with regulatable splicing confirmed decreased splicing efficiency and showed the leakage of unspliced RNAs in (1-169) cells. We also measured pre-mRNA accumulation of the meiotic gene, which depends on the expression of Mer1 factor for splicing. (1-169) cells accumulated approximately threefold higher levels of pre-mRNA than WT cells only when splicing was induced. To monitor cotranscriptional splicing, we determined the presence of early spliceosome assembly factors and snRNP complexes along the and genes. We found that (1-169) hampered the cotranscriptional recruitment of U2 and, to a larger extent, U5 and NTC, while the U1 profile was unaffected. The recruitment of Prp45(1-169) was impaired similarly to U5 snRNP and NTC. Our results imply that Prp45 is required for timely formation of complex A, prior to stable physical association of U5/NTC with the emerging pre-mRNA substrate. We suggest that Prp45 facilitates conformational rearrangements and/or contacts that couple U1 snRNP-recognition to downstream assembly events.

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http://www.ncbi.nlm.nih.gov/pmc/articles/PMC5602110PMC
http://dx.doi.org/10.1261/rna.061986.117DOI Listing

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