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二硝基甲苯体内处理后大鼠肝细胞中DNA非预定合成的诱导。

Induction of unscheduled DNA synthesis in rat hepatocytes following in vivo treatment with dinitrotoluene.

作者信息

Mirsalis J C, Butterworth B E

出版信息

Carcinogenesis. 1982;3(3):241-5. doi: 10.1093/carcin/3.3.241.

Abstract

The purpose of this study was to examine the induction of unscheduled DNA synthesis (UDS) by the potent hepatocarcinogen technical grade dinitrotoluene (tgDNT; 76% 2, 4-DNT, 19% 2, 6-DNT) using the in vivo-in vitro hepatocyte DNA repair assay, Male Fischer-344 rats were treated by gavage and hepatocytes were isolated by liver perfusion and cultured with [3H] thymidine. UDS was measured by quantitative autoradiography as net grains/nucleus (NG); greater than or equal to 5 NG was considered positive. Controls consistently had -3 to -6 NG. A dose-related increase in UDS was observed 12 h after treatment, with 200 mg/kg tgDNT producing 26 NG. AZ 50-fold increase in the number of cells in S-phase was observed at 48 h after treatment. This increase in S-phase cells could be suppressed in the presence of 10-20 mM hydroxyurea (HU), while the same levels of HU did not affect the level of UDS at 12 h after treatment, 2,4-DNT produced only a weak response, in contrast to 2,6-DNT which was a potent inducer of UDS. Treatment of female rats with tgDNT yielded only modest increases in UDS and DNA replication relative to males. These results are consistent with the carcinogenicity studies and indicate that tgDNT is a potent genotoxic agent, with 2,6-DNT contributing the major portion of the effect.

摘要

本研究的目的是使用体内-体外肝细胞DNA修复试验,检测强效肝癌致癌物工业级二硝基甲苯(tgDNT;76% 2,4-二硝基甲苯,19% 2,6-二硝基甲苯)对非程序性DNA合成(UDS)的诱导作用。雄性Fischer-344大鼠经口灌胃给药,通过肝脏灌注分离肝细胞,并与[3H]胸腺嘧啶核苷一起培养。通过定量放射自显影术测量UDS,以净颗粒数/细胞核(NG)表示;大于或等于5 NG被视为阳性。对照组的NG值始终为-3至-6。给药后12小时观察到UDS呈剂量相关增加,200 mg/kg tgDNT产生26 NG。给药后48小时观察到S期细胞数量增加了50倍。在存在10-20 mM羟基脲(HU)的情况下,S期细胞的这种增加可被抑制,而相同水平的HU在给药后12小时不影响UDS水平。与强效诱导UDS的2,6-二硝基甲苯相比,2,4-二硝基甲苯仅产生微弱反应。与雄性大鼠相比,用tgDNT处理雌性大鼠后,UDS和DNA复制仅适度增加。这些结果与致癌性研究一致,表明tgDNT是一种强效的遗传毒性剂,其中2,6-二硝基甲苯起主要作用。

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