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An exonic splicing enhancer in human IGF-I pre-mRNA mediates recognition of alternative exon 5 by the serine-arginine protein splicing factor-2/alternative splicing factor

机译:人类IGF-I pre-mRNA中的外显子剪接增强子通过丝氨酸-精氨酸蛋白剪接因子-2 /其他剪接因子介导对备选外显子5的识别

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摘要

The human IGF-I gene has six exons, four of which are alternatively spliced. Variations in splicing involving exon 5 may occur, depending on the tissue type and hormonal environment. To study the regulation of splicing to IGF-I exon 5, we established an in vitro splicing assay, using a model pre-mRNA containing IGF-I exons 4 and 5 and part of the intervening intron. Using a series of deletion mutants, we identified an 18-nucleotide purine-rich splicing enhancer in exon 5 that increases the splicing efficiency of the upstream intron from 6 to 35%. We show that the serine-arginine protein splicing factor-2/alternative splicing factor specifically promotes splicing in cultured cells and in vitro and is recruited to the spliceosome in an enhancer-specific manner. Our findings are consistent with a role for splicing factor-2/alternative splicing factor in the regulation of splicing of IGF-I alternative exon 5 via a purine-rich exonic splicing enhancer.
机译:人IGF-I基因具有六个外显子,其中四个被剪接。取决于组织类型和激素环境,涉及外显子5的剪接可能会发生变化。为了研究剪接至IGF-I外显子5的调控,我们使用包含IGF-I外显子4和5以及部分内含子的模型pre-mRNA建立了体外剪接测定。使用一系列缺失突变体,我们在第5外显子中鉴定了18个核苷酸的富含嘌呤的剪接增强子,它将上游内含子的剪接效率从6%提高到35%。我们显示丝氨酸精氨酸蛋白剪接因子2 /替代剪接因子在培养细胞中和体外特异性促进剪接,并以增强子特异性方式募集至剪接体。我们的发现与剪接因子-2 /替代剪接因子在经由富含嘌呤的外显子剪接增强子调节IGF-1替代外显子5的剪接中的作用是一致的。

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