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HepG2 悬滴球状体体外毒理学的表征和可重复性。

Characterization and reproducibility of HepG2 hanging drop spheroids toxicology in vitro.

机构信息

Department of Pharmacology, Faculty of Health Sciences, School of Medicine, University of Pretoria, Private Bag X323, Arcadia, 0007, South Africa.

Department of Pharmacology, Faculty of Health Sciences, School of Medicine, University of Pretoria, Private Bag X323, Arcadia, 0007, South Africa.

出版信息

Toxicol In Vitro. 2018 Aug;50:86-94. doi: 10.1016/j.tiv.2018.02.013. Epub 2018 Feb 21.

DOI:10.1016/j.tiv.2018.02.013
PMID:29476884
Abstract

Hepatotoxicity remains a major challenge in drug development despite preclinical toxicity screening using hepatocytes of human origin. To overcome some limitations of reproducing the hepatic phenotype, more structurally and functionally authentic cultures in vitro can be introduced by growing cells in 3D spheroid cultures. Characterisation and reproducibility of HepG2 spheroid cultures using a high-throughput hanging drop technique was performed and features contributing to potential phenotypic variation highlighted. Cultured HepG2 cells were seeded into Perfecta 3D® 96-well hanging drop plates and assessed over time for morphology, viability, cell cycle distribution, protein content and protein-mass profiles. Divergent aspects which were assessed included cell stocks, seeding density, volume of culture medium and use of extracellular matrix additives. Hanging drops are advantageous due to no complex culture matrix being present, enabling background free extractions for downstream experimentation. Varying characteristics were observed across cell stocks and batches, seeding density, culture medium volume and extracellular matrix when using immortalized HepG2 cells. These factors contribute to wide-ranging cellular responses and highlights concerns with respect to generating a reproducible phenotype in HepG2 hanging drop spheroids.

摘要

尽管使用源自人类的肝细胞进行了临床前毒性筛选,但肝毒性仍然是药物开发中的一个主要挑战。为了克服重现肝表型的一些限制,可以通过在 3D 球体培养中培养细胞来引入更具结构和功能真实性的体外培养。使用高通量悬滴技术对 HepG2 球体培养物进行了表征和重现性研究,并突出了导致潜在表型变异的特征。将培养的 HepG2 细胞接种到 Perfecta 3D®96 孔悬滴板中,并随时间评估形态、活力、细胞周期分布、蛋白质含量和蛋白质质量谱。评估的不同方面包括细胞库、接种密度、培养基体积和细胞外基质添加剂的使用。由于不存在复杂的培养基质,悬滴具有优势,可为下游实验提供无背景的提取。在使用永生化 HepG2 细胞时,细胞库和批次、接种密度、培养基体积和细胞外基质之间存在不同的特征。这些因素导致广泛的细胞反应,并突出了在 HepG2 悬滴球体中产生可重现表型的问题。

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