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      Chironomus tentans-repressor splicing factor represses SR protein function locally on pre-mRNA exons and is displaced at correct splice sites.

      Molecular Biology of the Cell
      Animals, Cells, Cultured, Chironomidae, genetics, metabolism, Exons, Protein Binding, RNA Precursors, RNA Splice Sites, RNA Splicing, RNA-Binding Proteins, Transcription, Genetic

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          Abstract

          Chironomus tentans-repressor splicing factor (Ct-RSF) represses the activation of splicing by SR proteins in vitro. Ct-RSF colocalizes with the Ser-Arg-rich (SR) protein hrp45 in interchromatin granule clusters and coimmunoprecipitates with hrp45 in nuclear extracts. Ct-RSF and hrp45 can also interact directly in vitro. Ct-RSF and hrp45 are recruited together to transcribing genes and associate with growing pre-mRNAs. Ct-RSF and hrp45 colocalize at a large number of gene loci. Injection of anti-Ct-RSF antibodies into nuclei of living cells blocks association of both Ct-RSF and hrp45 with the growing pre-mRNA, whereas binding of U2 small nuclear ribonucleoprotein particle (snRNP) to the pre-mRNA is unaffected. On the intron-rich Balbiani ring (BR) 3 pre-mRNA, hrp45 as well as U1 and U2 snRNPs bind extensively, whereas relatively little Ct-RSF is present. In contrast, the BR1 and BR2 pre-mRNAs, dominated by exon sequences, bind relatively much Ct-RSF compared with hrp45 and snRNPs. Our data suggest that Ct-RSF represses SR protein function at exons and that the assembly of spliceosomes at authentic splice sites displaces Ct-RSF locally.

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          Author and article information

          Journal
          16236800
          1345644
          10.1091/mbc.E05-04-0339

          Chemistry
          Animals,Cells, Cultured,Chironomidae,genetics,metabolism,Exons,Protein Binding,RNA Precursors,RNA Splice Sites,RNA Splicing,RNA-Binding Proteins,Transcription, Genetic

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