| 酶标仪法5α-还原酶抑制剂体外筛选模型的建立 |
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| 引用本文: | 吴建辉,孙祖越.酶标仪法5α-还原酶抑制剂体外筛选模型的建立[J].中华男科学杂志,2013,19(6):483-486. |
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| 作者姓名: | 吴建辉 孙祖越 |
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| 作者单位: | 吴建辉 (上海市计划生育科学研究所,中国生育调节药物毒理检测中心,上海200032); 孙祖越 (上海市计划生育科学研究所,中国生育调节药物毒理检测中心,上海200032); |
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| 基金项目: | 国家自然科学青年基金(项目编号:21007041)十二五"重大新药创制"科技重大专项(项目编号:2011ZX09301-005)grants,from,National,Natural,Science,Foundation,for,Young,Scientists,of,China(项目编号:21007041)Key,Specialized,Sci-Tech,Project,for,Major,Drug,Development,of,the,12th,Five-Year,Plan(项目编号:2011ZX09301-005) |
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| 摘 要: | 目的:建立酶标仪法5α-还原酶抑制剂体外筛选模型。方法:取6只雌性SD大鼠肝脏制备5α-还原酶,检测酶活性后,利用96孔板、酶标仪及酶标仪法分析软件建立5α-还原酶抑制剂体外筛选模型,并通过已知5α-还原酶抑制剂爱普列特及非那甾胺验证模型的可靠性。实验分别设置0、30、60 nmol/L爱普列特组及0、30、60 nmol/L非那甾胺组,96孔板依次加入终浓度0~40μmol/L系列睾酮溶液、22μmol/L的NADPH、终浓度0~60 nmol/L爱普列特或0~60 nmol/L非那甾胺及20μl 5α-还原酶,Tris-HCl缓冲液将每孔溶液体积调至200μl。将96孔板放置于酶标仪中,分别测定0、10 min的A340 nm,并对读取数据进行分析。结果:5α-还原酶的Km值为3.794μmol/L,Vmax为0.271μmol/(L.min);爱普列特的酶抑制常数(Ki)为148.2 nmol/L,半数抑制浓度(IC50)为31.5 nmol/L,曲线图分析为反竞争性抑制剂;非那甾胺的Ki为158.8 nmol/L,IC50为13.6 nmol/L,曲线图分析为竞争性抑制剂;二者结果均同文献报道相同。结论:建立的体外快速筛选模型能够有效地筛选5α-还原酶抑制剂。
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| 关 键 词: | 5α-还原酶抑制剂 筛药模型 体外 良性前列腺增生 大鼠 |
Establishment of an in vitro screening model for steroid 5 alpha-reductase inhibitors with the microplate reader |
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| WU Jian-hui,SUN Zu-yue.Establishment of an in vitro screening model for steroid 5 alpha-reductase inhibitors with the microplate reader[J].National Journal of Andrology,2013,19(6):483-486. |
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| Authors: | WU Jian-hui SUN Zu-yue |
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| Institution: | National Evaluation Center for the Toxicology of Fertility Regulating Drugs,Shanghai Institute of Planned Parenthood Research,Shanghai 200032,China |
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| Abstract: | Objective: To establish an in vitro screening model for steroid 5 alpha-reductase inhibitors using the microplate reader.Methods: Steroid 5 alpha-reductase was obtained from the liver of female rats,an in vitro screening model for steroid 5 alpha-reductase inhibitors established using the 96-well plate and microplate reader after determination of the enzymatic activity,and the reliability of the model verified with the known 5 alpha-reductase inhibitors epristeride and finasteride.Added to the 96-well plate were the final concentrations of testosterone(0-40 μmol/L),NADPH(22 μmol/L),epristeride(0-60 nmol/L) or finasteride(0-60 nmol/L) and steroid 5 alpha-reductase(20 μl),the total volume of each well adjusted to 200 μl with Tris-Hcl buffer.The 96-well plate was placed in the microplate reader,mixed and incubated at 37 ℃,followed by detection of the A340 nm value at 0 and 10 min and analysis of the data.Results: The Km value of steroid 5 alpha-reductase was 3.794 μmol/L,with a Vmax of 0.271 μmol/(L.min).The Ki of epristeride was 148.2 nmol/L,with an IC50 of 31.5 nmol/L,and the enzymatic reaction kinetic curve suggested that epristeride was an uncompetitive enzyme inhibitor.The Ki of finasteride was 158.8 nmol/L,with an IC50 of 13.6 nmol/L.The enzymatic reaction kinetic curve showed that both epristeride and finasteride were competitive enzyme inhibitors,similar to those reported in the published literature.Conclusion: A screening model was successfully established,which could rapidly and effectively screen steroid 5 alpha-reductase inhibitors in vitro. |
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| Keywords: | 5 alpha-reductase inhibitor screening model in vitro benign prostatic hyperplasia rat |
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