Concentration‐dependent effects of dutasteride on prostate‐specific membrane antigen (PSMA) expression and uptake of 177Lu‐PSMA‐617 in LNCaP cells

LNCaP公司 杜他星 谷氨酸羧肽酶Ⅱ 前列腺癌 流式细胞术 前列腺 医学 内化 免疫细胞化学 化学 癌症研究 内分泌学 内科学 受体 癌症 免疫学
作者
Benedikt Kranzbühler,Souzan Salemi,Christoph A. Umbricht,Luisa M. Deberle,Cristina Müller,Irene A. Burger,Thomas Hermanns,Tullio Sulser,Daniel Eberli
出处
期刊:The Prostate [Wiley]
卷期号:79 (12): 1477-1483 被引量:6
标识
DOI:10.1002/pros.23868
摘要

Abstract Background Prostate‐specific membrane antigen (PSMA)‐based imaging and therapy are increasingly used in the management of prostate cancer. However, low PSMA surface expression in certain patients is a limitation for PSMA‐based technologies. We have previously shown that high doses of dutasteride, a 5α‐reductase inhibitor generally used for the treatment of benign prostatic enlargement, increase the PSMA expression in vitro. We now further analyzed the concentration‐ and time‐dependent effects of dutasteride in LNCaP cells. Methods Androgen receptor (AR) expressing prostate cancer cells (LNCaP) were treated for 7 to 14 days with vehicle control (0.1% dimethyl sulfoxide) or different concentrations of dutasteride (0.25 , 0.5 , 1 , and 5 μM). In addition to cell proliferation, PSMA surface expression was assessed using flow cytometry (FACS) and immunocytochemistry. Total PSMA and AR expression was analyzed by capillary western immunoassay (WES). In addition, tumor cell uptake and internalization assays of 177 Lu‐PSMA‐617 were performed. Results Dutasteride treatment resulted in a significant upregulation of PSMA surface expression compared to vehicle control after 7 days in all tested concentrations. After 14 days a further, concentration‐dependent increase of PSMA surface expression was detectable. Total PSMA protein expression significantly increased after treatment of cells with high concentrations of dutasteride using 5 μM for 7 or 14 days. However, when lower concentrations were used total PSMA expression was not significantly altered compared to vehicle control. Further testing revealed a dose‐dependent increase in uptake and internalization of 177Lu ‐PSMA‐617 after 7 and 14 days. Though, a significantly increased uptake was only observed using a 5 μM dutasteride concentration for 7 days as well as 1 and 5 μM for 14 days. Conclusion Our investigations revealed a concentration‐ and time‐dependent effect of dutasteride on PSMA expression and uptake of 177Lu ‐PSMA‐617 in LNCaP cells. A short‐term treatment of patients with high doses of dutasteride might increase the detection rate of PSMA‐based imaging and increase the effect of 177Lu ‐PSMA‐617 therapy via upregulation of PSMA expression.
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