Centre for Drug Safety Science, Department of Pharmacology and Therapeutics, University of Liverpool, Liverpool, United Kingdom.
GSK, BioStatistics, Stevenage, United Kingdom.
Elife. 2023 Jun 6;12:e78187. doi: 10.7554/eLife.78187.
Evidence supports an important link between mitochondrial DNA (mtDNA) variation and adverse drug reactions such as idiosyncratic drug-induced liver injury (iDILI). Here, we describe the generation of HepG2-derived transmitochondrial cybrids, to investigate the impact of mtDNA variation on mitochondrial (dys)function and susceptibility to iDILI. This study created 10 cybrid cell lines, each containing distinct mitochondrial genotypes of haplogroup H or haplogroup J backgrounds.
HepG2 cells were depleted of mtDNA to make rho zero cells, before the introduction of known mitochondrial genotypes using platelets from healthy volunteers (n=10), thus generating 10 transmitochondrial cybrid cell lines. The mitochondrial function of each was assessed at basal state and following treatment with compounds associated with iDILI; flutamide, 2-hydroxyflutamide, and tolcapone, and their less toxic counterparts bicalutamide and entacapone utilizing ATP assays and extracellular flux analysis.
Whilst only slight variations in basal mitochondrial function were observed between haplogroups H and J, haplogroup-specific responses were observed to the mitotoxic drugs. Haplogroup J showed increased susceptibility to inhibition by flutamide, 2-hydroxyflutamide, and tolcapone, via effects on selected mitochondrial complexes (I and II), and an uncoupling of the respiratory chain.
This study demonstrates that HepG2 transmitochondrial cybrids can be created to contain the mitochondrial genotype of any individual of interest. This provides a practical and reproducible system to investigate the cellular consequences of variation in the mitochondrial genome, against a constant nuclear background. Additionally, the results show that inter-individual variation in mitochondrial haplogroup may be a factor in determining sensitivity to mitochondrial toxicants.
This work was supported by the Centre for Drug Safety Science supported by the Medical Research Council, United Kingdom (Grant Number G0700654); and GlaxoSmithKline as part of an MRC-CASE studentship (grant number MR/L006758/1).
有证据表明线粒体 DNA(mtDNA)变异与药物不良反应之间存在重要联系,例如特异质药物性肝损伤(iDILI)。在这里,我们描述了 HepG2 衍生的传递线粒体细胞杂种的产生,以研究 mtDNA 变异对线粒体(功能障碍)和易感性 iDILI 的影响。本研究创建了 10 个细胞杂种系,每个细胞杂种系都包含源自单倍群 H 或单倍群 J 的不同线粒体基因型。
HepG2 细胞被耗尽 mtDNA 以制造 rho 零细胞,然后使用来自健康志愿者的血小板(n=10)引入已知的线粒体基因型,从而产生 10 个传递线粒体细胞杂种系。在基础状态下和在用与 iDILI 相关的化合物处理后(氟他胺、2-羟基氟他胺和托卡朋及其毒性较小的对应物比卡鲁胺和恩他卡朋),利用 ATP 测定法和细胞外通量分析评估每个细胞杂种系的线粒体功能。
尽管在单倍群 H 和 J 之间观察到基础线粒体功能只有轻微的变化,但对线粒体毒性药物观察到了单倍群特异性反应。单倍群 J 对氟他胺、2-羟基氟他胺和托卡朋的抑制作用更敏感,通过对选定的线粒体复合物(I 和 II)的作用以及呼吸链的解偶联。
本研究表明,可以创建 HepG2 传递线粒体细胞杂种系来包含任何感兴趣个体的线粒体基因型。这提供了一种实用且可重复的系统,可在恒定的核背景下研究线粒体基因组变异的细胞后果。此外,结果表明,线粒体单倍群的个体间变异可能是决定对线粒体毒物敏感性的一个因素。
这项工作得到了英国医学研究理事会(MRC)资助的药物安全科学中心(Grant Number G0700654)和葛兰素史克公司的支持,作为 MRC-CASE 学生奖学金的一部分(grant number MR/L006758/1)。
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