[微小RNA-203a-5p通过靶向作用抑制多发性骨髓瘤细胞增殖和细胞周期进程]
[MiR-203a-5p Inhibits Multiple Myeloma Cell Proliferation and Cell Cycle Progression via Targeting ].
作者信息
Zhang Yue, Chen Ting-Ting, Zhou He-Bing, Chen Wen-Ming
机构信息
Department of Hematology, Beijing Luhe Hospital, Capital Medical University, Beijing 101149, China.
Department of Hematology, Beijing Luhe Hospital, Capital Medical University, Beijing 101149, China,E-mail:
出版信息
Zhongguo Shi Yan Xue Ye Xue Za Zhi. 2023 Jun;31(3):801-809. doi: 10.19746/j.cnki.issn.1009-2137.2023.03.027.
OBJECTIVE
To investigate the biological function of miR-203a-5p and the underlying mechanism in multiple myeloma (MM).
METHODS
Three miRNA expression profiles (GSE16558, GSE24371 and GSE17498) were downloaded from the GEO database. The three miRNA expression profiles contained 131 MM samples and 17 normal plasmacyte samples. The robust rank aggregation (RRA) method was used to identify the differentially expressed miRNAs between MM and normal plasmacytes. In order to carry out cytological experiments, MM cell line with stable over-expression of miR-203a-5p was constructed with lentivirus. Expression levels of miR-203a-5p in MM cells were quantified by qRT-PCR. The effects of miR-203a-5p on MM cells were investigated using assays of cell viability and cell cycle. Cell proliferation was measured using the Cell Counting kit (CCK)8 assay. The percentage of cells in each cell cycle was measured with a FACSCalibur system. Xenograft tumor models were established to evaluate the role of miR-203a-5p in tumorigenesis . To elucidate the underlying molecular mechanisms of miR-203a-5p in mediating cell proliferation inhibition and cell cycle arrest in MM, we used TargetScan and miRanda to predict the candidate targets of miR-203a-5p. The potential target of miR-203a-5p in MM cells was explored using the luciferase reporter assay, qRT-PCR, and Western blot.
RESULTS
An integrated analysis of three MM miRNA expression datasets showed that the levels of miR-203a-5p in MM were notably downregulated compared with those in normal plasmacytes. Accordingly, the relative expression levels of miR-203a-5p were decreased in MM cell lines. In addition, overexpression of miR-203a-5p inhibited the proliferation and cell cycle progression of RPMI8226 and U266 cells. experiments demonstrated that upregulation of miR-203a-5p expression could significantly inhibit the tumorigenesis of subcutaneous myeloma xenografts in nude mice. Mechanistic investigation led to the identification of Jagged 1 () as a novel and direct downstream target of miR-203a-5p. Interestingly, the reintroduction of abrogated miR-203a-5p-induced MM cell growth inhibition and cell cycle arrest.
CONCLUSION
Our data demonstrate that miR-203a-5p inhibits cell proliferation and cell cycle progression in MM cells by targeting , supporting the utility of miR-203a-5p as a novel and potential therapeutic agent for miRNA-based MM therapy.
目的
探讨miR-203a-5p在多发性骨髓瘤(MM)中的生物学功能及潜在机制。
方法
从基因表达综合数据库(GEO数据库)下载三个miRNA表达谱(GSE16558、GSE24371和GSE17498)。这三个miRNA表达谱包含131例MM样本和17例正常浆细胞样本。采用稳健秩聚合(RRA)方法鉴定MM与正常浆细胞之间差异表达的miRNA。为进行细胞学实验,用慢病毒构建了miR-203a-5p稳定过表达的MM细胞系。通过qRT-PCR定量MM细胞中miR-203a-5p的表达水平。使用细胞活力测定和细胞周期测定研究miR-203a-5p对MM细胞的影响。使用细胞计数试剂盒(CCK)8测定法测量细胞增殖。用FACSCalibur系统测量每个细胞周期中的细胞百分比。建立异种移植肿瘤模型以评估miR-203a-5p在肿瘤发生中的作用。为阐明miR-203a-5p介导MM细胞增殖抑制和细胞周期阻滞的潜在分子机制,我们使用TargetScan和miRanda预测miR-203a-5p的候选靶标。使用荧光素酶报告基因测定、qRT-PCR和蛋白质免疫印迹法探索miR-203a-5p在MM细胞中的潜在靶标。
结果
对三个MM miRNA表达数据集的综合分析表明,与正常浆细胞相比,MM中miR-203a-5p的水平显著下调。因此,MM细胞系中miR-203a-5p的相对表达水平降低。此外,miR-203a-5p的过表达抑制了RPMI8226和U266细胞的增殖和细胞周期进程。实验表明,miR-203a-5p表达上调可显著抑制裸鼠皮下骨髓瘤异种移植瘤的肿瘤发生。机制研究确定锯齿状蛋白1(Jagged 1)为miR-203a-5p的一个新的直接下游靶标。有趣的是,重新引入Jagged 1可消除miR-203a-5p诱导的MM细胞生长抑制和细胞周期阻滞。
结论
我们的数据表明,miR-203a-5p通过靶向Jagged 1抑制MM细胞的增殖和细胞周期进程,支持miR-203a-5p作为基于miRNA的MM治疗的一种新型潜在治疗药物的实用性。
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