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暴露于环境水平臭氧的烟草烟雾芳胺对培养的人肺细胞DNA损伤的诱导作用。

Induction of DNA damage in cultured human lung cells by tobacco smoke arylamines exposed to ambient levels of ozone.

作者信息

Kozumbo W J, Agarwal S

机构信息

Center for Environmental Medicine and Lung Biology, University of North Carolina, Chapel Hill 27599.

出版信息

Am J Respir Cell Mol Biol. 1990 Dec;3(6):611-8. doi: 10.1165/ajrcmb/3.6.611.

Abstract

Ozone (O3) is a powerful oxidizing component of air pollution that may react with other air pollutants before or after inhalation. Because ozonized compounds can be mutagenic to bacteria, we examined whether ambient O3 levels can transform tobacco smoke arylamines into products that are genotoxic to human lung cells. To test this possibility, aqueous solutions of 1-naphthylamine (1-NA) were first exposed to air or O3 in the absence of cells and then used to treat cultured human lung cells, i.e., the diploid fibroblasts CCD-18Lu and the transformed type II epithelial cells A549. DNA single-strand breaks were assayed by DNA alkaline elution. Neither air-exposed 1-NA nor O3-exposed buffer or water were DNA-damaging. However, exposure of 1-NA (15 microM) to O3 (0.1 ppm; 1 h) produced 400 rad equivalents of DNA breaks in either cell type. Although maximal induction of DNA breaks depended upon arylamine concentration, the rates at which DNA-damaging products were formed (activated) and subsequently deactivated depended upon O3 concentration. O3-activated 1-NA was stable for at least 4 h and could damage cellular DNA at 4 degrees C. During ozonization, hydroperoxides were formed at levels equivalent to between 2 and 20 microM of hydrogen peroxide and were eliminated by treatment with catalase. However, failure of catalase and superoxide dismutase to block formation of DNA breaks indicated that neither hydrogen peroxide nor superoxide anions were involved in breaking DNA.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

臭氧(O₃)是空气污染中一种强大的氧化成分,在吸入之前或之后可能与其他空气污染物发生反应。由于臭氧氧化的化合物可能对细菌具有致突变性,我们研究了环境臭氧水平是否能将烟草烟雾中的芳胺转化为对人肺细胞具有遗传毒性的产物。为了测试这种可能性,首先将1-萘胺(1-NA)的水溶液在无细胞的情况下暴露于空气或臭氧中,然后用于处理培养的人肺细胞,即二倍体成纤维细胞CCD-18Lu和转化的II型上皮细胞A549。通过DNA碱性洗脱法检测DNA单链断裂情况。暴露于空气的1-NA、暴露于臭氧的缓冲液或水均不会造成DNA损伤。然而,将1-NA(15微摩尔)暴露于臭氧(0.1 ppm;1小时)会在两种细胞类型中产生相当于400拉德当量的DNA断裂。虽然DNA断裂的最大诱导程度取决于芳胺浓度,但形成(激活)并随后失活DNA损伤产物的速率取决于臭氧浓度。臭氧激活的1-NA至少4小时内稳定,且在4℃时可损伤细胞DNA。在臭氧氧化过程中,形成的氢过氧化物水平相当于2至20微摩尔过氧化氢,并通过过氧化氢酶处理而消除。然而,过氧化氢酶和超氧化物歧化酶未能阻止DNA断裂的形成,这表明过氧化氢和超氧阴离子均未参与DNA断裂。(摘要截短至250字)

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