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异戊烯氧化物对培养的大鼠淋巴细胞的致断裂性。

Clastogenicity of isoamylene oxide to rat lymphocytes in culture.

作者信息

Gollapudi B B, Linscombe V A, Wilmer J W

机构信息

Dow Chemical Company, Midland, MI 48674, USA.

出版信息

Mutat Res. 1995 Jun;347(1):9-12. doi: 10.1016/0165-7992(95)90025-x.

Abstract

The mutagenic activity of the aliphatic epoxide isoamylene oxide (2-methyl-2,3-epoxybutane) is not readily detectable in the standard Ames test. In this study, the clastogenic potential of isoamylene oxide was evaluated using an in vitro mammalian cell culture system. Approximately 48 h after establishing primary cultures of rat lymphocyte cultures, the cells were treated for 4 h with various concentrations of isoamylene oxide (50, 166.7, 500,, 1666.7, and 5000 micrograms/ml in the initial assay and 500, 1000, 2000, 3000, 4000, and 5000 micrograms/ml in the confirmatory assay). The cultures were harvested 24 h after termination of the treatment. Based upon the mitotic indices, cultures treated with the three highest concentrations in both the initial and confirmatory assays were evaluated to estimate the chromosomal aberration frequencies. Isoamylene oxide demonstrated a strong clastogenic activity in this assay: up to 29% aberrant cells (without gaps) were observed at the highest concentration analyzed. The presence of an external metabolic activation system (S9) did not seem to influence the magnitude of the response at the dose levels analyzed.

摘要

在标准艾姆斯试验中,脂肪族环氧化物异戊烯氧化物(2-甲基-2,3-环氧丁烷)的诱变活性不易检测到。在本研究中,使用体外哺乳动物细胞培养系统评估了异戊烯氧化物的致断裂潜力。在建立大鼠淋巴细胞原代培养物约48小时后,用不同浓度的异戊烯氧化物(初始试验中为50、166.7、500、1666.7和5000微克/毫升,确认试验中为500、1000、2000、3000、4000和5000微克/毫升)处理细胞4小时。处理终止后24小时收获培养物。根据有丝分裂指数,对初始试验和确认试验中用三个最高浓度处理的培养物进行评估,以估计染色体畸变频率。在该试验中,异戊烯氧化物表现出很强的致断裂活性:在分析的最高浓度下,观察到高达29%的异常细胞(无裂隙)。在所分析的剂量水平下,外部代谢激活系统(S9)的存在似乎并未影响反应的强度。

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