[No authors listed]
The present study aimed to explore the role and underlying molecular mechanism of microRNAâ663b (miRâ663b) in the tumorigenesis of bladder cancer. The miRâ663b expression in human bladder cancer tissues and cell lines was measured determined reverse transcriptionâquantitative polymerase chain reaction. TargetScan was used to predict the potential targets of miRâ663b, and a dualâluciferase reporter assay was performed to validate tumor suppressor candidate 2 (TUSC2) as a target of miRâ663b. Cell Counting Kitâ8 was used for cell viability analysis, and cell apoptosis was evaluated by flow cytometry. In addition, western blot analysis was performed to detect protein expression in current study. The findings suggested that miRâ663b was upregulated in bladder cancer tissues and cell lines compared with normal tissue and cells. TUSC2 was validated as a direct target of miRâ663b and was negatively regulated by miRâ663b. miRâ663b inhibition significantly reduced the viability of T24 cells, and T24 cell apoptosis was markedly induced. In addition, miRâ663b inhibition enhanced the expression levels of p53 and p21 in T24 cells. Furthermore, the changes caused by miRâ663b inhibitor in T24 cells were eliminated by TUSC2 gene silencing. In conclusion, inhibition of miRâ663b reduced viability and induced apoptosis in bladder cancer cells by targeting TUSC2. These findings provide a promising novel therapeutic target for bladder cancer treatment.
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