Lack of effect of piperonyl butoxide on unscheduled DNA synthesis in precision-cut human liver slices

Jenny A. Beamand , Roger J. Price , John C. Phillips , William H. Butler , G.Denys Glynne Jones , Tom G. Osimitz , Karl L. Gabriel , Fred J. Preiss , Brian G. Lake
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引用次数: 31

Abstract

In this study the effect of piperonyl butoxide (PBO) on unscheduled DNA synthesis in precision-cut human liver slices has been examined. Liver slices prepared from tissue samples from five human donors were cultured in medium containing [3H]thymidine and 0–2.5 mM PBO using a dynamic organ culture system. After 24 h the liver slices were processed for autoradiographic examination of UDS. As positive controls, liver slices were also cultured with three known genotoxic agents, namely 2-acetylaminofluorene (2-AAF), aflatoxin B1 (AFB1) and 2-amino-1-methyl-6-phenylimidazo[4,5-b]pyridine (PhIP). UDS was quantified as the net grain count in centrilobular hepatocytes and as the percentage of centrilobular hepatocyte nuclei with >5 and >10 net grains. Compared to control liver slice cultures PBO had no effect on UDS. In contrast, treatment with 0.02 and 0.05 mM 2-AAF, 0.002 and 0.02 and 0.02 mM AFB1 and 0.005 and 0.05 mM PhIP produced significant increases in net grain counts of centrilobular hepatocytes. The greatest induction of UDS was observed in liver slices treated with 0.05 mM PhIP. Treatment with 2-AAF, AFB1 and PhIP also produced increases in the number of centrilobular hepatocyte nuclei with >5 and >10 net grains. At the concentrations examined neither PBO, 2-AAF nor PhIP had any significant effect on replicative DNA synthesis in 24 h cultured human liver slices. In cultured liver slices treated with 0.02, but not 0.002, mM AFB1 a significant reduction in the rate of replicative DNA synthesis was observed. These results demonstrate that PBO does not induce UDS in cultured human liver slices. However, all three positive control compounds produced marked significant increases in UDS, thus confirming the functional viability of the human liver slice

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胡椒酰丁醇对精确切割人类肝脏切片非预定DNA合成的影响
本研究考察了胡椒酰丁醇(PBO)对精确切割的人肝切片非预定DNA合成的影响。采用动态器官培养系统,在含有[3H]胸腺嘧啶和0-2.5 mM PBO的培养基中培养5名人类供体组织样品制备的肝脏切片。24 h后处理肝片进行UDS放射自显影检查。作为阳性对照,肝脏切片也用3种已知的基因毒性药物进行培养,即2-乙酰氨基芴(2-AAF)、黄曲霉毒素B1 (AFB1)和2-氨基-1-甲基-6-苯咪唑[4,5-b]吡啶(PhIP)。以小叶中心型肝细胞的净粒数和小叶中心型肝细胞核中净粒数为5粒和10粒的百分比进行定量。与对照组肝片培养相比,PBO对UDS无影响。相比之下,0.02和0.05 mM 2-AAF、0.002和0.02和0.02 mM AFB1以及0.005和0.05 mM PhIP处理的小叶中心肝细胞净粒数显著增加。0.05 mM PhIP处理的肝片对UDS的诱导作用最大。用2-AAF、AFB1和PhIP处理也使小叶中心肝细胞核数量增加,分别增加了5和10净粒。在检测的浓度下,PBO、2-AAF和PhIP对培养24 h的人肝片的复制性DNA合成均无显著影响。在培养的肝片中,用0.02而不是0.002处理,mM AFB1显著降低了复制DNA的合成率。这些结果表明PBO在培养的人肝片中不诱导UDS。然而,所有三种阳性对照化合物均显著增加了UDS,从而证实了人肝片的功能活力
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