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Extending an In Vitro Panel for Estrogenicity Testing: The Added Value of Bioassays for Measuring Antiandrogenic Activities and Effects on Steroidogenesis

机译:扩展用于雌激素测试的体外研究小组:用于测定抗雄激素活性及其对类固醇形成作用的生物测定的附加价值

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摘要

In the present study, a previously established integrated testing strategy (ITS) for in vitro estrogenicity testing was extended with additional in vitro assays in order to broaden its sensitivity to different modes of action resulting in apparent estrogenicity, i.e., other than estrogen receptor (ER) binding. To this end, an extra set of 10 estrogenic compounds with modes of action in part different from ER binding, were tested in the previously defined ITS, consisting of a yeast estrogen reporter gene assay, an U2OS ERα CALUX reporter gene assay and a cell-free coregulator binding assay. Two androgen reporter gene assays and the enhanced H295R steroidogenesis assay were added to that previous defined ITS. These assays had added value, as several estrogenic model compounds also elicited clear and potent antiandrogenic properties and in addition also showed effects on steroidogenesis that might potentiate their apparent estrogenic effects in vivo. Adding these assays, examining mechanisms of action for estrogenicity apart from ERα binding, gives a more complete and comprehensive assessment of the ability of test compounds to interfere with endocrine signaling. It was concluded that the extended ITS will go beyond in vivo estrogenicity testing by the uterotrophic assay, thereby contributing to the 3R-principles.
机译:在本研究中,先前建立的用于体外雌激素测试的综合测试策略(ITS)进行了额外的体外测定,以扩大其对导致表观雌激素的不同作用方式的敏感性,即除雌激素受体(ER) ) 捆绑。为此,在先前定义的ITS中测试了另外一组10种作用方式与ER结合部分不同的雌激素化合物,包括酵母雌激素报告基因测定,U2OSERαCALUX报告基因测定和细胞-免费的coregulator结合测定。将两个雄激素报告基因测定法和增强的H295R类固醇生成测定法添加到先前定义的ITS中。这些测定具有附加价值,因为几种雌激素模型化合物还具有清晰而有效的抗雄激素特性,此外还显示了对类固醇生成的作用,可能增强了它们在体内的明显雌激素作用。添加这些检测方法,检查除ERα结合以外的雌激素作用机制,可以更完整全面地评估受试化合物干扰内分泌信号的能力。得出的结论是,扩展的ITS将超越通过子宫营养测定法进行的体内雌激素测试,从而有助于3R原理。

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