PTBP1-dependent regulation of USP5 alternative RNA splicing plays a role in glioblastoma tumorigenesis

生物 选择性拼接 外显子 RNA剪接 多嘧啶结合蛋白 基因敲除 癌症研究 拼接因子 基因亚型 环状RNA 癌变 核糖核酸 长非编码RNA 遗传学 小RNA RNA结合蛋白 基因沉默 细胞生物学 癌症 基因 竞争性内源性RNA
作者
Daisy I. Izaguirre,Wen Zhu,Tao Hai,Hannah Cheung,Ralf Krahe,Gilbert J. Cote
出处
期刊:Molecular Carcinogenesis [Wiley]
卷期号:51 (11): 895-906 被引量:71
标识
DOI:10.1002/mc.20859
摘要

Aberrant RNA splicing is thought to play a key role in tumorigenesis. The assessment of its specific contributions is limited by the complexity of information derived from genome-wide array-based approaches. We describe how performing splicing factor-specific comparisons using both tumor and cell line data sets may more readily identify physiologically relevant tumor-specific splicing events. Affymetrix exon array data derived from glioblastoma (GBM) tumor samples with defined polypyrimidine tract-binding protein 1 (PTBP1) levels were compared with data from U251 GBM cells with and without PTBP1 knockdown. This comparison yielded overlapping gene sets that comprised only a minor fraction of each data set. The identification of a novel GBM-specific splicing event involving the USP5 gene led us to further examine its role in tumorigenesis. In GBM, USP5 generates a shorter isoform 2 through recognition of a 5' splice site within exon 15. Production of the USP5 isoform 2 was strongly correlated with PTBP1 expression in GBM tumor samples and cell lines. Splicing regulation was consistent with the presence of an intronic PTBP1 binding site and could be modulated through antisense targeting of the isoform 2 splice site to force expression of isoform 1 in GBM cells. The forced expression of USP5 isoform 1 in two GBM cell lines inhibited cell growth and migration, implying an important role for USP5 splicing in gliomagenesis. These results support a role for aberrant RNA splicing in tumorigenesis and suggest that changes in relatively few genes may be sufficient to drive the process.

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