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在藻酸盐微胶囊中培养的HepG2球体,作为使用海马XFe24分析仪探索线粒体和糖酵解代谢的模型。

HepG2 spheroids cultured in alginate microcapsules as a model for exploring mitochondrial and glycolytic metabolism using the Seahorse XFe24 Analyzer.

作者信息

Ghiraldelli Miranda Raul, Machado Ivo F, Rolo Anabela Pinto, Dorta Daniel Junqueira, Palmeira Carlos Manuel Marques

机构信息

School of Pharmaceutical Science of Ribeirão Preto, University of São Paulo, São Paulo, SP, Brazil.

Department of Life Sciences, of the University of Coimbra, Coimbra, Portugal.

出版信息

Toxicol Mech Methods. 2025 May;35(4):413-421. doi: 10.1080/15376516.2024.2447740. Epub 2025 Jan 6.

DOI:10.1080/15376516.2024.2447740
PMID:39757864
Abstract

Mitochondria are affected by chemical substances and play a critical role in drug-induced liver injury (DILI). Chemical substances can have a significant impact on various cellular processes, such as the disruption of oxidative phosphorylation, oxidative stress, and alteration of glucose metabolism. Given the consequences of these effects, it is crucial to understand the molecular pathways of chemical substances in the context of hepatotoxicity to prevent and treat DILI. In this regard, the Seahorse XFe24 Analyzer is a valuable tool for assessing mitochondrial bioenergetics and glucose metabolism. The Mito Stress Test and Glycolytic Rate Assay allow real-time assessment of the metabolic state after chemical exposure. Additionally, HepG2 spheroids have emerged as an important alternative tool for assessing hepatotoxicity, as they provide results that are more comparable to those found in humans than monolayer cultures or animal tests (such as rodent tests). By integrating these two powerful tools, it is possible to bridge the gap between animal and human tests, resulting in more reliable results in the assessment of human hepatotoxicity and DILI. However, because of the high variability in characteristics between 3D cultures (such as spheroids and organoids), XF analyzer assays are not well optimized for use with HepG2 spheroids. Here, we describe a streamlined and optimized protocol for performing the Mito Stress Test and Glycolytic Rate Assay using HepG2 spheroids cultured in alginate microcapsules in the Seahorse XFe24 Analyzer.

摘要

线粒体受化学物质影响,在药物性肝损伤(DILI)中起关键作用。化学物质可对各种细胞过程产生重大影响,如氧化磷酸化的破坏、氧化应激以及葡萄糖代谢的改变。鉴于这些影响的后果,了解化学物质在肝毒性背景下的分子途径对于预防和治疗DILI至关重要。在这方面,Seahorse XFe24分析仪是评估线粒体生物能量学和葡萄糖代谢的宝贵工具。线粒体应激试验和糖酵解速率测定可实时评估化学物质暴露后的代谢状态。此外,HepG2球状体已成为评估肝毒性的重要替代工具,因为与单层培养或动物试验(如啮齿动物试验)相比,它们提供的结果与人类中的结果更具可比性。通过整合这两种强大的工具,可以弥合动物试验和人体试验之间的差距,从而在评估人类肝毒性和DILI时获得更可靠的结果。然而,由于3D培养物(如球状体和类器官)之间的特征高度可变,XF分析仪检测方法并未针对HepG2球状体进行优化。在此,我们描述了一种简化且优化的方案,用于在Seahorse XFe24分析仪中对培养在藻酸盐微胶囊中的HepG2球状体进行线粒体应激试验和糖酵解速率测定。

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