长链非编码RNA DARS-AS1通过调控MicroRNA-628-5p/MTDH轴促进前列腺癌进展。
Long Non-Coding RNA DARS-AS1 Contributes to Prostate Cancer Progression Through Regulating the MicroRNA-628-5p/MTDH Axis.
作者信息
Fan Haitao, Hou Junhui, Liu Siqing, Xiao Zuomin, Cui Jia
机构信息
Department of Urology, The Second Hospital of Jilin University, Changchun, Jilin 130041, People's Republic of China.
Department of Oncology & Radiotherapy, Qingdao Central Medical Group, Qingdao, Shandong 266000, People's Republic of China.
出版信息
Cancer Manag Res. 2020 Sep 10;12:8363-8377. doi: 10.2147/CMAR.S271021. eCollection 2020.
PURPOSE
DARS antisense RNA 1 (DARS-AS1) is a long non-coding RNA that has been validated as a critical regulator in several human cancer types. Our study aimed to determine the expression profile of DARS-AS1 in prostate cancer (PCa) tissues and cell lines. Functional experiments were conducted to explore the detailed roles of DARS-AS1 in regulating PCa carcinogenesis. Furthermore, the detailed mechanisms by which DARS-AS1 regulates the oncogenicity of PCa cells were uncovered.
METHODS
Reverse transcription quantitative polymerase chain reaction was performed to analyze DARS-AS1 expression in PCa tissues and cell lines. Cell Counting Kit-8 assays, flow cytometry analyses, Transwell assays, and tumor xenograft experiments were conducted to determine the regulatory effects of DARS-AS1 knockdown on the malignant phenotype of PCa cells. Bioinformatics analysis was performed to identify putative microRNAs (miRNAs) targeting DARS-AS1, and the direct interaction between DARS-AS1 and miR-628-5p was verified using RNA immunoprecipitation and luciferase reporter assays.
RESULTS
DARS-AS1 was highly expressed in PCa tissues and cell lines. In vitro functional experiments demonstrated that DARS-AS1 depletion suppressed PCa cell proliferation, promoted cell apoptosis, and restricted cell migration and invasion. In vivo studies revealed that the downregulation of DARS-AS1 inhibited PCa tumor growth in nude mice. Mechanistic investigation verified that DARS-AS1 functioned as an endogenous miR-628-5p sponge in PCa cells and consequently promoted the expression of metadherin (MTDH). Furthermore, the involvement of miR-628-5p/MTDH axis in DARS-AS1-mediated regulatory actions in PCa cells was verified using rescue experiments.
CONCLUSION
DARS-AS1 functioned as a competing endogenous RNA in PCa by adsorbing miR-628-5p and thereby increasing the expression of MTDH, resulting in enhanced PCa progression. The identification of a novel DARS-AS1/miR-628-5p/MTDH regulatory network in PCa cells may offer a new theoretical basis for the development of promising therapeutic targets.
目的
DARS反义RNA 1(DARS-AS1)是一种长链非编码RNA,已被证实是多种人类癌症类型中的关键调节因子。我们的研究旨在确定DARS-AS1在前列腺癌(PCa)组织和细胞系中的表达谱。进行功能实验以探索DARS-AS1在调节PCa致癌过程中的详细作用。此外,还揭示了DARS-AS1调节PCa细胞致癌性的详细机制。
方法
采用逆转录定量聚合酶链反应分析DARS-AS1在PCa组织和细胞系中的表达。进行细胞计数试剂盒-8检测、流式细胞术分析、Transwell检测和肿瘤异种移植实验,以确定DARS-AS1敲低对PCa细胞恶性表型的调节作用。进行生物信息学分析以鉴定靶向DARS-AS1的假定微小RNA(miRNA),并使用RNA免疫沉淀和荧光素酶报告基因检测验证DARS-AS1与miR-628-5p之间的直接相互作用。
结果
DARS-AS1在PCa组织和细胞系中高表达。体外功能实验表明,DARS-AS1缺失抑制PCa细胞增殖,促进细胞凋亡,并限制细胞迁移和侵袭。体内研究表明,DARS-AS1的下调抑制了裸鼠体内PCa肿瘤的生长。机制研究证实,DARS-AS1在PCa细胞中作为内源性miR-628-5p海绵发挥作用,从而促进黏附素(MTDH)的表达。此外,通过挽救实验验证了miR-628-5p/MTDH轴在DARS-AS1介导的PCa细胞调节作用中的参与。
结论
DARS-AS1在PCa中作为竞争性内源性RNA发挥作用,通过吸附miR-628-5p从而增加MTDH的表达,导致PCa进展增强。在PCa细胞中鉴定出一种新的DARS-AS1/miR-628-5p/MTDH调节网络,可能为开发有前景的治疗靶点提供新的理论基础。
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