Mediating role of metabolic activation in in vitro cytotoxicity assays.

Molecular toxicology Pub Date : 1987-09-01
H Babich, N Martin-Alguacil, E Borenfreund
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Abstract

Enzymatic activation of polycyclic aromatic hydrocarbons (PAHs) and its effect on cytotoxicity were studied using the neutral red viability assay as the end point. Benzo[a]pyrene was progressively cytotoxic to human hepatoma (HepG2) cells over a 1- to 3-d period, and after induction of monooxygenase activity with a polychlorobiphenyl (PCB) mixture (Arochlor 1254), cytotoxicity was increased about threefold. Concomitant with Arochlor exposure was an increase in the activity of 7-ethoxycoumarin odeethylase, which could be inhibited by exposure to alpha-naphthoflavone. Human keratinocytes (NHEK), but not fibroblasts (HFF), were sensitive to the cytotoxicity of benzo[a]pyrene. However, preexposure of the keratinocytes to Arochlor did not increase their sensitivity to benzo[a]pyrene. Neither the keratinocytes, fibroblasts, nor HepG2 cells were sensitive to acenaphthene. Addition of hamster or rat hepatic S9 mix, however, resulted in toxicity from benzo[a]pyrene and acenaphthene. 7,12-Dimethylbenz[a]anthracene was only mildly cytotoxic to the fibroblasts, and its cytotoxicity was not enhanced in the presence of rat or hamster S9 mix. Exposure of the HepG2 cells to 7,12-dimethylbenz[a]anthracene showed progressive toxicity over a 1- to 3-d period. Prior exposure of the HepG2 cells to Arochlor did not enhance their sensitivity to 7,12-dimethylbenz[a]anthracene. Human keratinocytes were sensitive to 7,12-dimethylbenz[a]anthracene, with cytotoxicity markedly increasing over a 1- to 3-d period.

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代谢激活在体外细胞毒性试验中的中介作用。
以中性红活力法为终点,研究了多环芳烃(PAHs)的酶促活性及其对细胞毒性的影响。苯并[a]芘对人肝癌(HepG2)细胞具有1- 3-d的渐进式细胞毒性,并且在用多氯联苯(PCB)混合物(Arochlor 1254)诱导单加氧酶活性后,细胞毒性增加约三倍。与芳香氯接触同时发生的是7-乙氧基香豆素去乙基酶活性的增加,这种活性可以被暴露于α -萘黄酮抑制。人角质形成细胞(NHEK),而非成纤维细胞(HFF),对苯并[a]芘的细胞毒性敏感。然而,角化细胞预先暴露于芳香烃并没有增加它们对苯并[a]芘的敏感性。角质形成细胞、成纤维细胞和HepG2细胞对苊均不敏感。然而,添加仓鼠或大鼠肝脏S9混合物导致苯并[a]芘和苊的毒性。7,12-二甲基苯[a]蒽仅对成纤维细胞具有轻度细胞毒性,并且在大鼠或仓鼠S9混合物存在时其细胞毒性未增强。HepG2细胞暴露于7,12-二甲基苯[a]蒽中,在1- 3-d时间内显示出进行性毒性。先前暴露于芳香氯的HepG2细胞没有增强其对7,12-二甲基苯[a]蒽的敏感性。人角质形成细胞对7,12-二甲基苯[a]蒽敏感,细胞毒性在1- 3-d期间显著增加。
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