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用于药物代谢动力学、药物安全性评价及药物效应动力学的生物发光分析

Bioluminescent assays for ADMET.

作者信息

Cali James J, Niles Andrew, Valley Michael P, O'Brien Martha A, Riss Terry L, Shultz John

机构信息

Promega Corp., 2800 Woods Hollow Road, Madison, WI 53711, USA.

出版信息

Expert Opin Drug Metab Toxicol. 2008 Jan;4(1):103-20. doi: 10.1517/17425255.4.1.103.

DOI:10.1517/17425255.4.1.103
PMID:18370862
Abstract

Bioluminescent assays couple a limiting component of a luciferase-catalyzed photon-emitting reaction to a variable parameter of interest, while holding the other components constant or non-limiting. In this way light output varies with the parameter of interest. This review describes three bioluminescent assay types that use firefly luciferase to measure properties of drugs and other xenobiotics which affect their absorption, distribution, metabolism, elimination and toxicity. First, levels of the luciferase enzyme itself are measured in gene reporter assays that place a luciferase cDNA under the control of regulatory sequences from ADMET-related genes. This approach identifies activators of nuclear receptors that regulate expression of genes encoding drug-metabolizing enzymes and drug transporters. Second, drug effects on enzyme activities are monitored with luminogenic probe substrates that are inactive derivatives of the luciferase substrate luciferin. The enzymes of interest convert the substrates to free luciferin, which is detected in a second reaction with luciferase. This approach is used with the drug-metabolizing CYP and monoamine oxidase enzymes, apoptosis-associated caspase proteases, a marker protease for non-viable cells and with glutathione-S-transferase to measure glutathione levels in cell lysates. Third, ATP concentration is monitored as a marker of cell viability or cell death and as a way of identifying substrates for the ATP-dependent drug transporter, P-glycoprotein. Luciferase activity is measured in the presence of a sample that supplies the requisite luciferase substrate, ATP, so that light output varies with ATP concentration. The bioluminescent ADMET assays are rapid and sensitive, amenable to automated high-throughput applications and offer significant advantages over alternative methods.

摘要

生物发光测定法将荧光素酶催化的光子发射反应的一个限制成分与感兴趣的可变参数相关联,同时使其他成分保持恒定或非限制状态。通过这种方式,光输出随感兴趣的参数而变化。本综述描述了三种生物发光测定类型,它们使用萤火虫荧光素酶来测量药物和其他影响其吸收、分布、代谢、消除和毒性的外源性物质的特性。首先,在基因报告测定中测量荧光素酶本身的水平,该测定将荧光素酶cDNA置于与药物代谢和转运相关基因的调控序列控制之下。这种方法可识别调节编码药物代谢酶和药物转运蛋白基因表达的核受体激活剂。其次,使用荧光素酶底物荧光素的无活性衍生物作为发光探针底物来监测药物对酶活性的影响。感兴趣的酶将底物转化为游离荧光素,然后在与荧光素酶的第二个反应中进行检测。这种方法用于药物代谢的细胞色素P450酶和单胺氧化酶、与细胞凋亡相关的半胱天冬酶蛋白酶、非存活细胞的标记蛋白酶以及谷胱甘肽-S-转移酶,以测量细胞裂解物中的谷胱甘肽水平。第三,监测ATP浓度作为细胞活力或细胞死亡的标志物,并作为识别ATP依赖性药物转运蛋白P-糖蛋白底物的一种方式。在提供必需荧光素酶底物ATP的样品存在下测量荧光素酶活性,以使光输出随ATP浓度而变化。生物发光药物代谢和转运相关测定快速且灵敏,适用于自动化高通量应用,并且比其他方法具有显著优势。

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