Alveolar organoids: development of an in vitro assay to facilitate pulmonary toxicity assessments

Jooyeon Lee, Hyosin Baek, Seok-Ho Hong, Jong-Hee Lee, Seung-jun Wang, Ji Young Lee, Myung Ha Song, Se-Ran Yang
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Abstract

Animal experiments have been performed to predict toxicity in humans in many fields, including toxicology, medicine, and pharmacology, and have contributed to increasing life expectancy. However, animal testing has been a controversial issue for over 100 years due to ethical concerns, and inter-species differences pose limitations for understanding human responses to toxicity. In recent years, many researchers have developed in vitro and in silico alternatives to using animals (e.g., 3-dimensional [3D] organoid culture, organs-on-a-chip, and advanced computer modeling). In this study, we generated 3D alveolar organoids (AOs) for pulmonary toxicity testing following exposure to chemicals, instead of animal models or two-dimensional culture of a single cell type. After human induced pluripotent stem cells were cultured with differentiation medium corresponding to each step for 14 days in 6-well plates, AOs were generated by forced aggregation and cultured with differentiation medium. The AOs were exposed to acrolein and sodium chromate for 24, 72, and 120 hours, and we determined the cytotoxicity of these chemicals using the MTT assay. Exposure to acrolein and sodium chromate for 24 hours decreased proliferation, but the organoid size did not change considerably. However, long-term exposure to acrolein and sodium chromate significantly decreased the organoid size. These findings suggest that AOs could facilitate acute toxicity assessments based on measurements of cell viability in AOs, as well as sub-chronic toxicity assessments based on measurements of both size and viability.
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肺泡类器官:一种促进肺毒性评估的体外测定方法的发展
动物实验已经在许多领域进行,包括毒理学、医学和药理学,以预测对人类的毒性,并有助于提高预期寿命。然而,由于伦理问题,动物试验一直是一个有争议的问题超过100年,物种间的差异对理解人类对毒性的反应构成了限制。近年来,许多研究人员已经开发出体外和计算机替代动物的方法(例如,三维类器官培养、芯片上的器官和先进的计算机建模)。在这项研究中,我们生成了3D肺泡类器官(AOs),用于暴露于化学物质后的肺毒性测试,而不是动物模型或单一细胞类型的二维培养。将人诱导多能干细胞在6孔板上用相应步骤的分化培养基培养14天后,强制聚集生成AOs,再用分化培养基培养。将AOs暴露于丙烯醛和铬酸钠24,72和120小时,我们使用MTT法测定这些化学物质的细胞毒性。丙烯醛和铬酸钠作用24小时可降低细胞增殖,但类器官大小没有明显变化。然而,长期暴露于丙烯醛和铬酸钠会显著降低类器官的大小。这些发现表明,AOs可以促进基于AOs中细胞活力测量的急性毒性评估,以及基于尺寸和活力测量的亚慢性毒性评估。
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