[No authors listed]
MicroRNA (miR)â26aâ5p and miRâ26bâ5p consistently play an antitumor role in many types of cancers, but the underlying mechanism remains unclear in bladder cancer (BC). In the present study, we found that, in BC tissues, the levels of miRâ26aâ5p and miRâ26bâ5p were lower than in paired normal tissues. The upregulation of miRâ26â5p significantly inhibited the proliferation of BC cell lines (T24 and 5637). Bioinformatics analysis indicated that Programmed (PDCD10) was the downstream target gene of miRâ26aâ5p/miRâ26bâ5p, and this was ascertained by western blotting and quantitative realâtime reverse transcription PCR (RTâqPCR). In addition, in the 3'âUTR of PDCD10, the binding site was identified using a luciferase reporter assay. We determined that clinical BC tissues presented higher PDCD10 levels than adjacent normal tissues and that PDCD10 promoted proliferation of BC cell lines. Overexpression of miRâ26aâ5p/miRâ26bâ5p inhibited the stimulatory effect on proliferation of BC cells induced by PDCD10. In addition, in vivo experiments and clinical data revealed that the prognosis of BC patients with high expression of miRâ26aâ5p/miRâ26bâ5p and low expression of PDCD10 was better than that of patients with low miRâ26â5p and high PDCD10 expression. These data revealed that miRâ26aâ5p and miRâ26bâ5p were pivotal regulators in BC progression by targeting the proliferationârelated protein, PDCD10. The miRâ26â5p/PDCD10 interaction may provide important insight into the pathway of BC progression and present novel opportunities for future diagnosis and treatment strategies, especially for patients with high levels of PDCD10.
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