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Liver-on-chip model and application in predictive genotoxicity and mutagenicity of drugs

遗传毒性 甲基磺酸盐 微核 体内 DNA损伤 甲基磺酸乙酯 彗星试验 分子生物学 微核试验 化学 药理学 生物化学 毒理 生物 遗传学 突变 DNA 基因 毒性 有机化学
作者
Benjamin T. Kopp,A. Khawam,K. Di Perna,D. Lenart,M. Vinette,Rufino Silva,Thalita B. Zanoni,C. Rore,Gareth Guenigault,Emily Richardson,Tomasz Kostrzewski,A. Boswell,Phong Nguyen Van,Carrie R. Valentine,Jonas Salk,A Hamel
出处
期刊:Mutation Research [Elsevier]
卷期号:896: 503762-503762 被引量:10
标识
DOI:10.1016/j.mrgentox.2024.503762
摘要

Currently, there is no test system, whether in vitro or in vivo, capable of examining all endpoints required for genotoxicity evaluation used in pre-clinical drug safety assessment. The objective of this study was to develop a model which could assess all the required endpoints and possesses robust human metabolic activity, that could be used in a streamlined, animal-free manner. Liver-on-chip (LOC) models have intrinsic human metabolic activity that mimics the in vivo environment, making it a preferred test system. For our assay, the LOC was assembled using primary human hepatocytes or HepaRG cells, in a MPS-T12 plate, maintained under microfluidic flow conditions using the PhysioMimix® Microphysiological System (MPS), and co-cultured with human lymphoblastoid (TK6) cells in transwells. This system allows for interaction between two compartments and for the analysis of three different genotoxic endpoints, i.e. DNA strand breaks (comet assay) in hepatocytes, chromosome loss or damage (micronucleus assay) and mutation (Duplex Sequencing) in TK6 cells. Both compartments were treated at 0, 24 and 45 hours with two direct genotoxicants: methyl methanesulfonate (MMS) and ethyl methanesulfonate (EMS), and two genotoxicants requiring metabolic activation: benzo[a]pyrene (B[a]P) and cyclophosphamide (CP). Assessment of cytochrome activity, RNA expression, albumin, urea and lactate dehydrogenase production, demonstrated functional metabolic capacities. Genotoxicity responses were observed for all endpoints with MMS and EMS. Increases in the micronucleus and mutations (MF) frequencies were also observed with CP, and %Tail DNA with B[a]P, indicating the metabolic competency of the test system. CP did not exhibit an increase in the %Tail DNA, which is in line with in vivo data. However, B[a]P did not exhibit an increase in the % micronucleus and MF, which might require an optimization of the test system. In conclusion, this proof-of-principle experiment suggests that LOC-MPS technology is a promising tool for in vitro hazard identification genotoxicants.
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