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在微型 3D 细胞培养平台上进行高内涵成像分析。

High-content imaging assays on a miniaturized 3D cell culture platform.

机构信息

Department of Chemical and Biomedical Engineering, Cleveland State University, 455 Fenn Hall, 1960 East 24th Street, Cleveland, OH 44115-2214, USA.

Department of Chemical and Biomedical Engineering, Cleveland State University, 455 Fenn Hall, 1960 East 24th Street, Cleveland, OH 44115-2214, USA.

出版信息

Toxicol In Vitro. 2018 Aug;50:147-159. doi: 10.1016/j.tiv.2018.02.014. Epub 2018 Mar 6.

Abstract

The majority of high-content imaging (HCI) assays have been performed on two-dimensional (2D) cell monolayers for its convenience and throughput. However, 2D-cultured cell models often do not represent the in vivo characteristics accurately and therefore reduce the predictability of drug toxicity/efficacy in vivo. Recently, three-dimensional (3D) cell-based HCI assays have been demonstrated to improve predictability, but its use is limited due to difficulty in maneuverability and low throughput in cell imaging. To alleviate these issues, we have developed miniaturized 3D cell culture on a micropillar/microwell chip and demonstrated high-throughput HCI assays for mechanistic toxicity. Briefly, Hep3B human hepatoma cell line was encapsulated in a mixture of alginate and fibrin gel on the micropillar chip, cultured in 3D, and exposed to six model compounds in the microwell chip for rapidly assessing mechanistic hepatotoxicity. Several toxicity parameters, including DNA damage, mitochondrial impairment, intracellular glutathione level, and cell membrane integrity were measured on the chip, and the IC values of the compounds at different readouts were determined to investigate the mechanism of toxicity. Overall, the Z' factors were between 0.6 and 0.8 for the HCI assays, and the coefficient of variation (CV) were below 20%. These results indicate high robustness and reproducibility of the HCI assays established on the miniaturized 3D cell culture chip. In addition, it was possible to determine the predominant mechanism of toxicity using the 3D HCI assays. Therefore, our miniaturized 3D cell culture coupled with HCI assays has great potential for high-throughput screening (HTS) of compounds and mechanistic toxicity profiling.

摘要

大多数高内涵成像(HCI)测定都是在二维(2D)细胞单层上进行的,因为这样比较方便且通量高。然而,2D 培养的细胞模型往往不能准确地代表体内特征,从而降低了体内药物毒性/疗效的可预测性。最近,已经证明了基于三维(3D)细胞的 HCI 测定可以提高预测能力,但由于在细胞成像中操作困难和通量低,其应用受到限制。为了解决这些问题,我们开发了一种在微柱/微槽芯片上进行的小型化 3D 细胞培养方法,并展示了用于机制毒性的高通量 HCI 测定。简而言之,将 Hep3B 人肝癌细胞系包裹在微柱芯片上的藻酸盐和纤维蛋白凝胶混合物中,在 3D 中培养,并在微槽芯片中暴露于六种模型化合物,以快速评估机制肝毒性。在芯片上测量了几个毒性参数,包括 DNA 损伤、线粒体损伤、细胞内谷胱甘肽水平和细胞膜完整性,并确定了化合物在不同读出值下的 IC 值,以研究毒性机制。总体而言,HCI 测定的 Z'值在 0.6 到 0.8 之间,变异系数(CV)低于 20%。这些结果表明,在小型化 3D 细胞培养芯片上建立的 HCI 测定具有很高的稳健性和重现性。此外,使用 3D HCI 测定可以确定毒性的主要机制。因此,我们的小型化 3D 细胞培养与 HCI 测定相结合,具有用于化合物高通量筛选(HTS)和机制毒性分析的巨大潜力。

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本文引用的文献

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