Please use this identifier to cite or link to this item: https://doi.org/10.1261/rna.066951.118
DC FieldValue
dc.titleAn important class of intron retention events in human erythroblasts is regulated by cryptic exons proposed to function as splicing decoys
dc.contributor.authorParra M.
dc.contributor.authorBooth B.W.
dc.contributor.authorWeiszmann R.
dc.contributor.authorYee B.
dc.contributor.authorYeo G.W.
dc.contributor.authorBrown J.B.
dc.contributor.authorCelniker S.E.
dc.contributor.authorConboy J.G.
dc.date.accessioned2019-03-06T05:06:04Z
dc.date.available2019-03-06T05:06:04Z
dc.date.issued2018
dc.identifier.citationParra M., Booth B.W., Weiszmann R., Yee B., Yeo G.W., Brown J.B., Celniker S.E., Conboy J.G. (2018). An important class of intron retention events in human erythroblasts is regulated by cryptic exons proposed to function as splicing decoys. RNA 24 (9) : 699. ScholarBank@NUS Repository. https://doi.org/10.1261/rna.066951.118
dc.identifier.issn13558382
dc.identifier.urihttp://scholarbank.nus.edu.sg/handle/10635/152026
dc.description.abstractDuring terminal erythropoiesis, the splicing machinery in differentiating erythroblasts executes a robust intron retention (IR) program that impacts expression of hundreds of genes. We studied IR mechanisms in the SF3B1 splicing factor gene, which expresses ?50% of its transcripts in late erythroblasts as a nuclear isoform that retains intron 4. RNA-seq analysis of nonsense-mediated decay (NMD)-inhibited cells revealed previously undescribed splice junctions, rare or not detected in normal cells, that connect constitutive exons 4 and 5 to highly conserved cryptic cassette exons within the intron. Minigene splicing reporter assays showed that these cassettes promote IR. Genome-wide analysis of splice junction reads demonstrated that cryptic noncoding cassettes are much more common in large (>1 kb) retained introns than they are in small retained introns or in nonretained introns. Functional assays showed that heterologous cassettes can promote retention of intron 4 in the SF3B1 splicing reporter. Although many of these cryptic exons were spliced inefficiently, they exhibited substantial binding of U2AF1 and U2AF2 adjacent to their splice acceptor sites. We propose that these exons function as decoys that engage the intron-terminal splice sites, thereby blocking cross-intron interactions required for excision. Developmental regulation of decoy function underlies a major component of the erythroblast IR program. � 2018 Parra et al.
dc.publisherCold Spring Harbor Laboratory Press
dc.sourceScopus
dc.subjectAlternative splicing
dc.subjectIntron retention
dc.subjectSF3B1
dc.typeArticle
dc.contributor.departmentPSYCHOLOGY
dc.description.doi10.1261/rna.066951.118
dc.description.sourcetitleRNA
dc.description.volume24
dc.description.issue9
dc.description.page699
dc.description.codenRNARF
dc.grant.idUC Berkeley
dc.grant.idS10 OD018174
dc.grant.id5R01DK108020
dc.grant.fundingagencyUniversity of California Berkeley
dc.grant.fundingagencyNIH, National Institutes of Health
dc.grant.fundingagencyNIH, National Institutes of Health
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