Human spliceosomal snRNA sequence variants generate variant spliceosomes

生物 假基因 剪接体 snRNP公司 RNA剪接 小核RNA 遗传学 核糖核酸 小核核糖核蛋白 前体mRNA Prp24型 内含子 细胞生物学 外显子 小核仁RNA 基因 分子生物学 核糖核蛋白 选择性拼接 拼接因子 基因组 信使核糖核酸 非编码RNA
作者
Justin W. Mabin,Peter W. Lewis,David A. Brow,Heidi Dvinge
出处
期刊:RNA [Cold Spring Harbor Laboratory Press]
卷期号:27 (10): 1186-1203 被引量:9
标识
DOI:10.1261/rna.078768.121
摘要

Human pre-mRNA splicing is primarily catalyzed by the major spliceosome, comprising five small nuclear ribonucleoprotein complexes, U1, U2, U4, U5, and U6 snRNPs, each of which contains the corresponding U-rich snRNA. These snRNAs are encoded by large gene families exhibiting significant sequence variation, but it remains unknown if most human snRNA genes are untranscribed pseudogenes or produce variant snRNAs with the potential to differentially influence splicing. Since gene duplication and variation are powerful mechanisms of evolutionary adaptation, we sought to address this knowledge gap by systematically profiling human U1, U2, U4, and U5 snRNA variant gene transcripts. We identified 55 transcripts that are detectably expressed in human cells, 38 of which incorporate into snRNPs and spliceosomes in 293T cells. All U1 snRNA variants are more than 1000-fold less abundant in spliceosomes than the canonical U1, whereas at least 1% of spliceosomes contain a variant of U2 or U4. In contrast, eight U5 snRNA sequence variants occupy spliceosomes at levels of 1% to 46%. Furthermore, snRNA variants display distinct expression patterns across five human cell lines and adult and fetal tissues. Different RNA degradation rates contribute to the diverse steady state levels of snRNA variants. Our findings suggest that variant spliceosomes containing noncanonical snRNAs may contribute to different tissue- and cell-type-specific alternative splicing patterns.

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