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The snRNP-free U1A (SF-A) complex(es): identification of the largest subunit as PSF, the polypyrimidine-tract binding protein-associated splicing factor.

机译:无snRNP的U1A(SF-A)复合物:最大的亚基鉴定为PSF,即多嘧啶束结合蛋白相关的剪接因子。

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摘要

We have previously shown that a specific monoclonal antibody prepared against the U1A protein, MAb 12E12, is unique in its ability to recognize a form of U1A which is not associated with the U1snRNP. This unique form of U1A, termed snRNP-free U1A or SF-A, was found to be complexed with a novel set of non-snRNP proteins (O'Connor et al., 1997, RNA 3:1444-1455). Here we demonstrate that the largest protein in these SF-A complex(es), p105, is the polypyrimidine-tract binding protein-associated factor (PSF), an auxiliary splicing factor. We show that PSF copurifies and co-immunoprecipitates with SF-A from 293T cell nucleoplasm and that it interacts with SF-A in vitro. In addition, we show that MAb 12E12 inhibits both splicing and polyadenylation in an in vitro coupled splicing and polyadenylation reaction. This suggests that SF-A and/or the SF-A complex(es) perform an important function in both processing reactions and possibly in last exon definition.
机译:先前我们已经表明,针对U1A蛋白MAb 12E12制备的特异性单克隆抗体在识别与U1snRNP不相关的U1A形式方面具有独特的能力。发现这种独特的U1A形式,称为无snRNP的U1A或SF-A,与一组新的非snRNP蛋白复合(O'Connor等,1997,RNA 3:1444-1455)。在这里,我们证明了这些SF-A复合物中最大的蛋白质p105是聚嘧啶束结合蛋白相关因子(PSF),一种辅助剪接因子。我们显示,PSF与293T细胞核质中的SF-A共纯化和共免疫沉淀,并且在体外与SF-A相互作用。另外,我们显示MAb 12E12在体外偶联的剪接和聚腺苷酸化反应中抑制剪接和聚腺苷酸化。这表明SF-A和/或SF-A复合物在加工反应和可能在最后一个外显子定义中均起重要作用。

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