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用于检测动物组织中合成糖皮质激素的双荧光素酶报告基因筛选测定法的开发。

Development of a dual luciferase reporter screening assay for the detection of synthetic glucocorticoids in animal tissues.

作者信息

Schumacher Sylvie Briand, Van den Hauwe Olivia, Van Peteghem Carlos H, Naegeli Hanspeter

机构信息

Institute of Pharmacology and Toxicology, University of Zürich-Tierspital, Winterthurerstrasse 260, CH-8057 Zürich, Switzerland.

出版信息

Analyst. 2003 Dec;128(12):1406-12. doi: 10.1039/b309539h. Epub 2003 Nov 11.

Abstract

Synthetic glucocorticoids belong to the most frequently administered drugs in livestock production. These synthetic hormones are employed for therapeutic purposes against inflammatory reactions, disorders of the musculoskeletal system, bovine ketosis and many other diseases of farm animals. A widespread illegal use of synthetic glucocorticoids to improve feed intake and weight gain has also been observed. To enforce the residue limits imposed on glucocorticoid drugs and preclude their illicit administration as growth promoters, it is necessary to establish high throughput analytical methods that can be applied to the screening of animal tissues. Here, we developed a dual luciferase reporter assay that detects residues or contaminants with glucocorticoid activity. This screening assay is performed by transfection of human cell lines with two reporter constructs followed by the measurement of two distinct luminescence signals, one of which serves as internal control to correct for assay variabilities and unspecific matrix effects. The limit of detection (1.25 microg for dexamethasone in liver) depends on the biological potency of each synthetic glucocorticoid but, with all drugs tested, the maximal response reaches a 20 to 30 fold induction of luciferase activity. In combination with an appropriate sample clean-up method (recovery of 82%), this luciferase assay has been applied to the analysis of liver samples from calves treated with a single therapeutic injection of either dexamethasone or flumethasone. Thus, the dual luciferase reporter assay provides a new screening tool to detect unwanted glucocorticoid activities in animal tissues or other crude biological samples without knowledge of the precise chemical entity of the parent compounds or their metabolites.

摘要

合成糖皮质激素是畜牧生产中最常用的药物之一。这些合成激素用于治疗炎症反应、肌肉骨骼系统疾病、牛酮血症以及许多其他家畜疾病。人们还观察到合成糖皮质激素被广泛非法用于提高采食量和体重增加。为了执行对糖皮质激素药物规定的残留限量,并防止其作为生长促进剂的非法使用,有必要建立可应用于动物组织筛查的高通量分析方法。在此,我们开发了一种双荧光素酶报告基因检测方法,用于检测具有糖皮质激素活性的残留物或污染物。该筛查检测方法是通过用两种报告基因构建体转染人细胞系,然后测量两种不同的发光信号来进行的,其中一种用作内对照,以校正检测变异性和非特异性基质效应。检测限(肝脏中地塞米松为1.25微克)取决于每种合成糖皮质激素的生物学效价,但对于所有测试药物,最大反应可使荧光素酶活性诱导20至30倍。结合适当的样品净化方法(回收率为82%)后,该荧光素酶检测方法已应用于分析单次治疗注射地塞米松或氟米松的犊牛肝脏样品。因此,双荧光素酶报告基因检测方法提供了一种新的筛查工具,可用于检测动物组织或其他粗生物样品中不需要的糖皮质激素活性,而无需了解母体化合物或其代谢物的确切化学实体。

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