PARP-1体外活性测定方法的建立及其应用

Establishment and Application of Enzymatic Assay for Poly(ADP-Ribose) Polymerase-1

DOI：10.3969/j.issn.1673-1689.2015.03.015

中文关键词: 多聚二磷酸腺苷核糖基聚合酶-1 活性测定 抑制剂 高通量筛选

英文关键词: poly(ADP-ribose) polymerase-1, enzymatic assay, inhibitors, high-throughput screening

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中文摘要:

建立PARP-1的体外活性测定方法并对84个具有潜在PARP抑制活性的化合物进行筛选。从Sf9昆虫细胞中提取酶液,以NAD+为底物,DNA为激活剂,建立PARP-1的活性测定方法;以高通量技术参数评价此方法,用已知PARP抑制剂进行验证,并以此方法进行PARP抑制剂的筛选。结果显示,确定的酶促反应体系为:12.5 nmol/L NAD+,15 μg/mL DNA,6.25×10-4 U PARP-1。评价Z'因子为0.76,S/B值为3.58。基于此模型筛出47个化合物在浓度7.4 μmol/L时对PARP-1的抑制率达到60%以上。表明所建立的PARP-1活性测定方法,适用于PARP-1抑制剂的高通量筛选。

英文摘要:

To establish an enzymatic assay for poly(ADP-ribose) polymerase-1 and screen PARP inhibitors from 84 potential compounds. Crude PARP-1 was extracted from Sf9 insect cells. With nicked DNA as activator,PARP-1 was used to catalyze the hydrolysis of the substrate NAD+,the RFU value measured from the remaining NAD+ was used to evaluate the activity of PARP-1 or efficiency of PARP inhibitors. A 96-microwell screening method was set up by optimizing the reaction system．The screening method was assessed with high throughput index,such as Z' factor,signal to back ground (S/B) and validated by well-known PARP inhibitors such as PHE,DPQ and AZD2281. 84 compounds were assayed for PARP inhibition through the established method. The enzymatic reaction system was optimized as:12.5 nmol/L NAD+,15 μg/mL DNA,6.25×10-4 U PARP-1. The Z' factor is 0.76,S/B is 3.58 and the IC50 of PHE,DPQ and AZD2281 is 562.4 nmol/L,369.6 nmol/L and 6.8 nmol/L. There are 47 compounds showed 60% or more PARP-1 inhibition efficiency at the concentration of 7.4 μmol/L. An enzymatic assay of PARP-1 was successfully established. It can be effectively applied to high-throughput screening for PARP inhibitors．

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