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MicroRNA‐181a promotes docetaxel resistance in prostate cancer cells
Author(s) -
Armstrong Cameron M.,
Liu Chengfei,
Lou Wei,
Lombard Alan P.,
Evans Christopher P.,
Gao Allen C.
Publication year - 2017
Publication title -
the prostate
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.295
H-Index - 123
eISSN - 1097-0045
pISSN - 0270-4137
DOI - 10.1002/pros.23358
Subject(s) - du145 , docetaxel , cabazitaxel , prostate cancer , gene knockdown , cancer research , western blot , transfection , apoptosis , medicine , cell culture , cancer , pharmacology , biology , androgen deprivation therapy , biochemistry , gene , lncap , genetics
BACKGROUND Docetaxel is one of the primary drugs used for treating castration resistant prostate cancer (CRPC). Unfortunately, over time patients invariably develop resistance to docetaxel therapy and their disease will continue to progress. The mechanisms by which resistance develops are still incompletely understood. This study seeks to determine the involvement of miRNAs, specifically miR‐181a, in docetaxel resistance in CRPC. METHODS Real‐time PCR was used to measure miR‐181a expression in parental and docetaxel resistant C4‐2B and DU145 cells (TaxR and DU145‐DTXR). miR‐181a expression was modulated in parental or docetaxel resistant cells by transfecting them with miR‐181a mimics or antisense, respectively. Following transfection, cell number was determined after 48 h with or without docetaxel. Cross resistance to cabazitaxel induced by miR‐181a was also determined. Western blots were used to determine ABCB1 protein expression and rhodamine assays used to assess activity. Phospho‐p53 expression was assessed by Western blot and apoptosis was measured by ELISA in C4‐2B TaxR and PC3 cells with inhibited or overexpressed miR‐181a expression with or without docetaxel. RESULTS miR‐181a is significantly overexpressed in TaxR and DU145‐DTXR cells compared to parental cells. Overexpression of miR‐181a in parental cells confers docetaxel and cabazitaxel resistance and knockdown of miR‐181a in TaxR cells re‐sensitizes them to treatment with both docetaxel and cabazitaxel. miR‐181a was not observed to impact ABCB1 expression or activity, a protein which was previously demonstrated to be highly involved in docetaxel resistance. Knockdown of miR‐181a in TaxR cells induced phospho‐p53 expression. Furthermore, miR‐181a knockdown alone induced apoptosis in TaxR cells which could be further enhanced by the addition of DTX. CONCLUSIONS Overexpression of mir‐181a in prostate cancer cells contributes to their resistance to docetaxel and cabazitaxel and inhibition of mir‐181a expression can restore treatment response. This is due, in part, to modulation of p53 phosphorylation and apoptosis.