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The U1 snRNP-associated factor Luc7p affects 5 ' splice site selection in yeast and human

机译:U1 snRNP相关因子Luc7p影响酵母和人类5'剪接位点的选择

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yLuc7p is an essential subunit of the yeast U1 snRNP and contains two putative zinc fingers. Using RNAprotein cross-linking and directed site-specific proteolysis (DSSP), we have established that the N-terminal zinc finger of yLuc7p contacts the pre-mRNA in the 5 exon in a region close to the cap. Modifying the pre-mRNA sequence in the region contacted by yLuc7p affects splicing in a yLuc7p-dependent manner indicating that yLuc7p stabilizes U1 snRNPpre-mRNA interaction, thus reminding of the mode of action of another U1 snRNP component, Nam8p. Database searches identified three putative human yLuc7p homologs (hLuc7A, hLuc7B1 and hLuc7B2). These proteins have an extended C-terminal tail rich in RS and RE residues, a feature characteristic of splicing factors. Consistent with a role in pre-mRNA splicing, hLuc7A localizes in the nucleus and antibodies raised against hLuc7A specifically co-precipitate U1 snRNA from human cell extracts. Interestingly, hLuc7A overexpression affects splicing of a reporter in vivo. Taken together, our data suggest that the formation of a wide network of proteinRNA interactions around the 5 splice site by U1 snRNP-associated factors contributes to alternative splicing regulation.
机译:yLuc7p是酵母U1 snRNP的必需亚基,包含两个推定的锌指。使用RNA蛋白质交联和定向的位点特异性蛋白水解(DSSP),我们已经确定yLuc7p的N末端锌指在靠近帽的区域中与5个外显子中的pre-mRNA接触。修饰yLuc7p接触区域中的pre-mRNA序列会以yLuc7p依赖性方式影响剪接,表明yLuc7p稳定了U1 snRNPpre-mRNA相互作用,从而提醒了另一个U1 snRNP组件Nam8p的作用方式。数据库搜索确定了三个假定的人类yLuc7p同源物(hLuc7A,hLuc7B1和hLuc7B2)。这些蛋白质具有丰富的RS和RE残基的延伸的C末端尾巴,这是剪接因子的特征。与在mRNA剪接前的作用一致,hLuc7A定位在细胞核中,针对hLuc7A的抗体特异性地从人细胞提取物中共沉淀U1 snRNA。有趣的是,hLuc7A过表达影响体内报道基因的剪接。两者合计,我们的数据表明,U1 snRNP相关因子在5个剪接位点周围形成一个广泛的蛋白RNA相互作用网络,有助于替代剪接调控。

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