首页> 外文期刊>Toxicology in vitro: an international journal published in association with BIBRA >A new bioluminescent cellular assay to measure the transcriptional effects of chemicals that modulate the alpha-1 thyroid hormone receptor.
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A new bioluminescent cellular assay to measure the transcriptional effects of chemicals that modulate the alpha-1 thyroid hormone receptor.

机译:一种新的生物发光细胞测定法,用于测量调节α-1甲状腺激素受体的化学物质的转录作用。

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摘要

Interactions of environmental pollutants with the thyroid endocrine axis have received much attention especially because thyroid hormones (THs) play a major role in mammalian brain development. In order to screen for compounds that act on the triiodothyronine (T3) signaling pathway, we developed a new reporter gene assay expressing luciferase under the control of the TH receptor (TR). PC12 cells expressing the alpha1-isoform of TR of avian origin were stably transfected with a luciferase gene controlled by the SV40 promoter, and enhanced by a four-spaced direct repeat (DR4) thyroid response element (TRE). The resulting PC-DR-LUC cells were used to optimize a T3 assay in multiwell microplates. This assay was highly sensitive (30 pM T3) and reproducible, and responded as expected to TH analogues. Several halogenated phenolic (3,3',5,5'-tetrabromobisphenol A, 3,3',5,5'-tetrachlorobisphenol A, 4-hydroxy-2',3,4',5,6'-pentachlorobiphenyl) and phenol (pentachlorophenol, 2,4,6-triiodophenol) compounds suspected of being thyroid-disrupting environmental chemicals induced partial agonistic and/or complex competitive/uncompetitive antagonistic responses in PC-DR-LUC cells at micromolar concentrations. A cell viability test indicated that these effects were not related to cytotoxicity of the chemicals. These results suggest that the PC-DR-LUC assay could be a valuable tool for the large-scale screening for thyroid receptor agonists and antagonists in vitro, and for detecting thyroid disruptors in the environment.
机译:环境污染物与甲状腺内分泌轴的相互作用受到了广泛关注,特别是因为甲状腺激素(THs)在哺乳动物大脑发育中起着重要作用。为了筛选作用于三碘甲状腺氨酸(T3)信号通路的化合物,我们开发了一种新的报告基因试验,该试验在TH受体(TR)的控制下表达荧光素酶。表达SV的启动子控制的荧光素酶基因可稳定转染表达禽源TR的α1-亚型的PC12细胞,并通过四间隔直接重复(DR4)甲状腺反应元件(TRE)进行增强。所得的PC-DR-LUC细胞用于优化多孔微孔板中的T3分析。该测定法高度灵敏(30 pM T3)且可重复,对TH类似物的反应预期。几种卤代酚醛(3,3',5,5'-四溴双酚A,3,3',5,5'-四氯双酚A,4-羟基-2',3,4',5,6'-五氯联苯)和怀疑是破坏甲状腺的环境化学物质的苯酚(五氯苯酚,2,4,6-三碘苯酚)化合物以微摩尔浓度在PC-DR-LUC细胞中引起部分激动和/或复杂的竞争/非竞争性拮抗作用。细胞活力测试表明,这些作用与化学物质的细胞毒性无关。这些结果表明,PC-DR-LUC测定法可能是一种有价值的工具,可用于大规模体外筛选甲状腺受体激动剂和拮抗剂,以及检测环境中的甲状腺干扰物。

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