High Expression of SRSF10 Promotes Colorectal Cancer Progression by Aberrant Alternative Splicing of RFC5.

IF 2.7 4区 医学 Q3 ONCOLOGY Technology in Cancer Research & Treatment Pub Date : 2024-01-01 DOI:10.1177/15330338241271906
Shuai Xu, Fangmin Zhong, Junyao Jiang, Fangyi Yao, Meiyong Li, Mengxin Tang, Ying Cheng, Yulin Yang, Wen Wen, Xueru Zhang, Bo Huang, Xiaozhong Wang
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Abstract

Background: Colorectal cancer (CRC) remains a global health concern with persistently high incidence and mortality rates. However, the specific pathogenesis of CRC remains poorly understood. This study aims to investigate the role and pathogenesis of serine and arginine rich splicing factor 10 (SRSF10) in colorectal cancer.

Methods: Bioinformatics analysis was employed to predict SRSF10 gene expression in CRC patients. Functional experiments involving SRSF10 knockdown and overexpression were conducted using CCK8, transwell, scratch assay, and flow cytometry. Additionally, the PRIdictor website was utilized to predict the SRSF10 interaction site with RFC5. The identification of different transcripts of SRSF10-acting RFC5 pre-mRNA was achieved through agarose gel electrophoresis.

Result: The knockdown of SRSF10 inhibited the proliferation and migration ability of CRC cells, while promoting apoptosis and altering the DNA replication of CRC cells. Conversely, when SRSF10 was highly expressed, it enhanced the proliferation and migration ability of CRC cells and caused changes in the cell cycle of colorectal cancer cells. This study revealed a change in the replicating factor C subunit 5 (RFC5) gene in colorectal cancer cells following SRSF10 knockdown. Furthermore, it was confirmed that SRSF10 increased RFC5 exon2-AS1(S) transcription variants, thereby promoting the development of colorectal cancer through AS1 exclusion to exon 2 of RFC5.

Conclusion: In summary, this study demonstrates that SRSF10 promotes the progression of colorectal cancer by generating an aberrantly spliced exclusion isoform of AS1 within RFC5 exon 2. These findings suggest that SRSF10 could serve as a crucial target for the clinical diagnosis and treatment of CRC.

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SRSF10的高表达通过RFC5的异常替代剪接促进结直肠癌的进展
背景:结肠直肠癌(CRC)的发病率和死亡率居高不下,仍然是全球关注的健康问题。然而,人们对 CRC 的具体发病机制仍然知之甚少。本研究旨在探讨富丝氨酸和精氨酸剪接因子 10(SRSF10)在结直肠癌中的作用和发病机制:方法:采用生物信息学分析预测 SRSF10 基因在 CRC 患者中的表达。使用 CCK8、transwell、划痕试验和流式细胞术进行了 SRSF10 基因敲除和过表达的功能实验。此外,还利用 PRIdictor 网站预测了 SRSF10 与 RFC5 的相互作用位点。通过琼脂糖凝胶电泳鉴定了SRSF10作用于RFC5前mRNA的不同转录本:结果:SRSF10的敲除抑制了CRC细胞的增殖和迁移能力,同时促进了CRC细胞的凋亡和DNA复制的改变。相反,当 SRSF10 高表达时,它能增强 CRC 细胞的增殖和迁移能力,并引起结直肠癌细胞周期的变化。这项研究揭示了 SRSF10 敲除后大肠癌细胞中复制因子 C 亚基 5(RFC5)基因的变化。此外,研究还证实SRSF10增加了RFC5外显子2-AS1(S)的转录变异,从而通过AS1对RFC5外显子2的排斥促进了结直肠癌的发生:总之,本研究表明,SRSF10 通过在 RFC5 第 2 外显子内产生异常剪接的 AS1 排斥异构体,促进了结直肠癌的发展。这些发现表明,SRSF10 可作为临床诊断和治疗 CRC 的关键靶点。
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来源期刊
CiteScore
4.40
自引率
0.00%
发文量
202
审稿时长
2 months
期刊介绍: Technology in Cancer Research & Treatment (TCRT) is a JCR-ranked, broad-spectrum, open access, peer-reviewed publication whose aim is to provide researchers and clinicians with a platform to share and discuss developments in the prevention, diagnosis, treatment, and monitoring of cancer.
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