Therapeutic targeting of the androgen receptor(AR)and AR variants in prostate cancer

Prostate cancer(PCa)accounted for over 300000 deaths world-wide in 2018.Most of the PCa deaths occurred due to the aggressive castration-resistant PCa(CRPC).Since the androgen receptor(AR)and its ligands contribute to the continued growth of androgendependent PCa(ADPCa)and CRPC,AR has become a well-characterized and pivotal therapeutic-target.Although AR signaling was identified as therapeutic-target in PCa over five-decades ago,there remains several practical issues such as lack of antagonist-bound AR crystal structure,stabilization of the AR in the presence of agonists due to N-terminus and C-terminus interaction,unfavorable large-molecule accommodation of the ligand-binding domain(LBD),and generation of AR splice variants that lack the LBD that impede the discovery of highly potent fail-safe drugs.This review summarizes the AR-signaling pathway targeted therapeutics currently used in PCa and the approaches that could be used in future ARtargeted drug development of potent next-generation molecules.The review also outlines the discovery of molecules that bind to domains other than the LBD and those that inhibit both the full length and splice variant of ARs.

臭椿酮对前列腺癌22RV1细胞内源性AR等的影响

目的探究臭椿酮对前列腺癌22RV1细胞内源性雄激素受体(androgen receptor,AR)及其下游基因前列腺特异性抗原(prostate-specific antigen,PSA)、FK506结合蛋白5(FK506 binding protein 5,FKBP5)、溶质转运蛋白家族45A3(solute carriers 45A3,SLC45A3)、N-myc下游调节基因(N-myc downstream regulated gene 1,NDRG1)mRNA表达的影响。方法取处于对数生长期的前列腺癌22RV1细胞,随机分为4组,分别为对照组、臭椿酮低剂量组、臭椿酮中剂量组和臭椿酮高剂量组,每组设置5个复孔。臭椿酮低、中和高剂量组分别采用0.4、0.8和1.0μmol·L^(-1)臭椿酮干预,对照组加入等量磷酸盐缓冲液(phosphate buffer saline,PBS)干预。用二甲基噻唑(dimethylthiazole,MTT)实验检测干预24、48、72 h后细胞的增殖情况;用流式细胞仪检测干预72 h后细胞的凋亡率;用实时荧光定量PCR检测干预72 h后各组内源性AR及其下游基因PSA、FKBP5、SLC45A3、NDRG1 mRNA的相对表达量。结果臭椿酮低、中和高剂量组MTT实验吸光度(A)及AR、PSA、FKBP5、SLC45A3 mRNA的相对表达量均低于对照组,臭椿酮高剂量组低于臭椿酮低、中剂量组,臭椿酮中剂量组MTT实验A值低于臭椿酮低剂量组(P<0.05);臭椿酮低、中和高剂量组的凋亡率、NDRG1 mRNA的相对表达量均高于对照组,臭椿酮高剂量组高于臭椿酮低、中剂量组,臭椿酮中剂量组高于臭椿酮低剂量组(P<0.05)。结论臭椿酮可抑制前列腺癌22RV1细胞的增殖,促进其凋亡,其中1.0μmol·L^(-1)臭椿酮的作用最强,可能与其调控内源性AR及其下游基因PSA、FKBP5、SLC45A3和NDRG1 mRNA的表达有关。

人前列腺癌雄激素受体分布特性及血清睾酮水平变化的研究

采用放射配基结合分析法测定人前列腺癌(PC)穿刺标本的雄激素受体(AR)含量,其胞浆受体(AcR)及胞核受体(AnR)分别为305.70±461.68,363.04±391.44pmol/g蛋白,与36例前列腺增生症(BPH)及9例正常前列腺组织含量相比均有显著性差异,显示前列腺癌的雄激素依赖性。22例前列腺癌患者中未转移组的AnR/AcR比值明显大于转移组,提示前列腺癌转移过程中AnR向胞浆转移的可能性。前列腺癌患者的血清睾酮水平明显低于前列腺增生症患者及正常人。放射自显影术显示雄激素受体定位以前列腺上皮细胞核为主,表明雄激素通过与核内受体结合调控肿瘤发生发展的可能性。

前列腺组织雄激素受体的测定

本室建立了雄激素受体(AR)测定的放射配基结合分析(RBA)法。测得人前列腺组织中胞浆、胞核的AR均可被约5nmol/l的双氢睾酮饱和,其最大结合容量分别为129.4fmol/mg胞浆蛋白和176.2fmol/mg胞核蛋白;平衡解离常数分别为0.88nmol/l和3.2nmol/l。人前列腺癌的胞浆胞核AR含量均高于正常前列腺及前列腺肥大的(P<0.05)。为前列腺癌病人选择治疗方案提供了理论依据。同时用融裱法放射自显影证实了AR主要分布在前列腺组织的腺区,尤其是腺上皮细胞核。

前列腺组织雄激素受体的测定方法

建立雄激素受体测定的放射配基结合分析法测得人前列腺组织中胞浆胞核雄激素受体均可被约5x10^(-9)mol/L的双氢睾酮饱和,其最大结合客量(B(-max))及平衡解离常数(Kd)分别为:胞浆129.4x10(-15)mol/mg,0.88x10(-9)mol/L;胞核176.2x10^(-15)mol/mg,3.2x10^(-9)mol/L。人前列腺癌胞浆、胞核雄激素受体均高于正常前列腺(n=3)及前列腺肥大者(n=32)。用融裱法放射自显影证实雄激素受体主要分布在前列腺组织的腺区,尤其是在腺上皮细胞核内。