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用于甲状腺激素信号环境干扰物的多层级体内定量检测套件。

A multi-tiered, in vivo, quantitative assay suite for environmental disruptors of thyroid hormone signaling.

作者信息

Mengeling Brenda J, Wei Yuzhu, Dobrawa Lucia N, Streekstra Mischa, Louisse Jochem, Singh Vikrant, Singh Latika, Lein Pamela J, Wulff Heike, Murk Albertinka J, Furlow J David

机构信息

Department of Neurobiology, Physiology, and Behavior, College of Biological Sciences, University of California, Davis 95616-8519, USA.

Marine Animal Ecology Group, Wageningen University, The Netherlands, Wageningen University, P.O. Box 38, 6700 AH Wageningen, The Netherlands.

出版信息

Aquat Toxicol. 2017 Sep;190:1-10. doi: 10.1016/j.aquatox.2017.06.019. Epub 2017 Jun 21.

DOI:10.1016/j.aquatox.2017.06.019
PMID:28662416
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5558850/
Abstract

The essential role of thyroid hormone (TH) signaling in mammalian development warrants the examination of man-made chemicals for its disruption. Among vertebrate species, the molecular components of TH signaling are highly conserved, including the thyroid hormone receptors (TRs), their heterodimer binding partners the retinoid-X receptors (RXRs), and their DNA recognition sequences (TREs). This molecular conservation allows examination of potential TH disruption in the tractable, in vivo model system of amphibian metamorphosis. Metamorphosis requires TH signaling for both instigation and progression, and it provides dramatic and well-characterized phenotypes involving different cell fates. Here we describe a quantitative, precocious-metamorphosis assay suite we developed using one-week post-fertilization (PF) Xenopus laevis tadpoles in order to assess disruption of TH signaling. Tadpoles at this developmental stage (Nieuwkoop-Faber (NF)-48) are competent to respond to TH hormone, although not yet producing TH, along many metamorphic pathways, and they are uniform in size. This allowed us to quantify changes in morphology associated with natural metamorphosis (e.g. gill and tail resorption, brain expansion, and craniofacial remodeling) after five days of treatment. Using the same tadpoles from morphological measurements, we quantified a 20-fold increase in TH-induced cellular proliferation in the rostral head region by whole-mount immunocytochemistry. At the molecular level, we used F3-generation tadpoles from a transgenic X. laevis line, which expresses luciferase under the control of a native TRE, to assess the ability of compounds to disrupt TR function. The luciferase reporter showed over 10-fold activation by physiologic concentrations of TH. We used the synthetic TR antagonist NH-3 to demonstrate the feasibility of our assay suite to measure inhibition of TH activity at the level of the receptor. Finally, we assessed the capabilities of suspected TH-disrupting chemicals tetrabrominated diphenyl ether 47 (BDE-47) and tetrabromobisphenol A (TBBPA). We found that BDE-47 displays general toxicity rather than TH disruption, as it did not increase brain width nor affect the TRE-luciferase reporter. However, TBBPA, a suspected TR antagonist, although not effective in antagonizing cell proliferation, significantly inhibited the TRE-luciferase reporter, suggesting that it bears closer scrutiny as a TH disruptor. Overall the assay suite has important advantages over the classical tadpole metamorphosis assays with respect to the uniformity of animal size, small test volume, reproducibility, and short test period. The assays are performed before endogenous TH production and free feeding start, which further reduces complexity and variability.

摘要

甲状腺激素(TH)信号传导在哺乳动物发育中起着至关重要的作用,这使得人们有必要对人造化学物质对其的干扰作用进行研究。在脊椎动物物种中,TH信号传导的分子成分高度保守,包括甲状腺激素受体(TRs)、它们的异二聚体结合伴侣视黄醛X受体(RXRs)以及它们的DNA识别序列(TREs)。这种分子保守性使得在易于处理的两栖动物变态的体内模型系统中检测潜在的TH干扰成为可能。变态既需要TH信号传导来启动,也需要其来推进,并且它会产生涉及不同细胞命运的显著且特征明确的表型。在此,我们描述了一套定量的早熟变态分析方法,该方法是我们利用受精后一周(PF)的非洲爪蟾蝌蚪开发的,用于评估TH信号传导的干扰情况。处于这个发育阶段(Nieuwkoop-Faber(NF)-48)的蝌蚪能够沿着许多变态途径对TH激素做出反应,尽管它们自身尚未产生TH,而且它们的大小是一致的。这使我们能够在处理五天后量化与自然变态相关的形态变化(例如鳃和尾巴的吸收、大脑扩张以及颅面重塑)。利用来自形态测量的相同蝌蚪,我们通过全片免疫细胞化学方法量化了TH诱导的吻部头部区域细胞增殖增加了20倍。在分子水平上,我们使用了来自转基因非洲爪蟾品系的F3代蝌蚪,该品系在天然TRE的控制下表达荧光素酶,以评估化合物干扰TR功能的能力。荧光素酶报告基因显示在生理浓度的TH作用下有超过10倍的激活。我们使用合成的TR拮抗剂NH-3来证明我们的分析方法在受体水平测量TH活性抑制的可行性。最后,我们评估了疑似TH干扰化学物质四溴二苯醚47(BDE-47)和四溴双酚A(TBBPA)的能力。我们发现BDE-47表现出一般毒性而非TH干扰,因为它没有增加脑宽也没有影响TRE-荧光素酶报告基因。然而,TBBPA作为一种疑似TR拮抗剂,尽管在拮抗细胞增殖方面无效,但显著抑制了TRE-荧光素酶报告基因,这表明它作为TH干扰物值得更深入的研究。总体而言,与经典的蝌蚪变态分析相比,该分析方法在动物大小的一致性、小测试体积、可重复性和短测试周期方面具有重要优势。这些分析是在内源性TH产生和自由摄食开始之前进行的,这进一步降低了复杂性和变异性。

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