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Human Ntera2 cells as a predictive in vitro test system for developmental neurotoxicity

机译:人类Ntera2细胞作为发育性神经毒性的预测性体外测试系统

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Developmental neurotoxicity (DNT) of environmental chemicals is a serious threat to human health. Current DNT testing guidelines propose investigations in rodents, which require large numbers of animals. With regard to the "3Rs" (reduction, replacement, and refinement) of animal testing, alternative testing strategies are needed in order to refine and reduce animal experiments and allow faster and less expensive screening. The goal of this study was to establish components for a human cell-based test system to assess DNT potential of chemicals at an early stage of brain development. A human neural precursor cell line should be tested for suitability for semi-automated high-throughput DNT screening. We established assays suitable for detecting disturbances in two basic processes of brain development in 96-well scale: neuronal differentiation and migration using the human Ntera2 (NT2) cell line. We assessed the effects of four test compounds with well-established DNT potential in comparison with three compounds without specific DNT potential. We found that human NT2 cell cultures treated with the morphogen, retinoic acid, imitate neuronal differentiation, and migration in vitro. The developmental neurotoxicants methylmercury chloride, sodium arsenite, sodium valproate, and methylazoxymethanol significantly reduced the expression of the neuronal marker β-tubulin type III and decreased the migration distance in developing NT2 cells. Both endpoints, differentiation and migration, can be read out directly in a standard fluorescence plate reader, enabling high-throughput screening. We conclude that NT2 cell tests are likely to become valuable components of a human cell-based modular in vitro DNT test systems.
机译:环境化学品的发育性神经毒性(DNT)对人类健康构成严重威胁。当前的DNT测试指南建议对需要大量动物的啮齿动物进行调查。关于动物测试的“ 3R”(减少,替代和完善),需要其他测试策略以完善和减少动物实验并允许更快,更便宜的筛查。这项研究的目的是为基于人体细胞的测试系统建立组件,以评估大脑发育早期化学物质的DNT潜力。应测试人类神经前体细胞系是否适合半自动化高通量DNT筛选。我们建立了适合检测96孔规模的大脑发育的两个基本过程中的障碍的检测方法:使用人Ntera2(NT2)细胞系进行神经元分化和迁移。与没有特定DNT电位的三种化合物相比,我们评估了具有良好DNT电位的四种测试化合物的效果。我们发现用吗啡原,视黄酸处理的人NT2细胞培养物可模仿神经元分化和体外迁移。发育中的神经毒性物质氯化甲基汞,亚砷酸钠,丙戊酸钠和甲基丙氧基甲醇显着降低了神经元标志物III型微管蛋白的表达,并缩短了正在发育的NT2细胞的迁移距离。分化和迁移这两个终点都可以在标准荧光板读数器中直接读出,从而实现高通量筛选。我们得出结论,NT2细胞测试可能会成为基于人细胞的模块化体外DNT测试系统的重要组成部分。

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