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用双酚A二缩水甘油醚处理的C3H小鼠中DNA加合物的分子剂量测定

Molecular dosimetry of DNA adducts in C3H mice treated with bisphenol A diglycidylether.

作者信息

Steiner S, Hönger G, Sagelsdorff P

机构信息

Ciba-Geigy Ltd, Toxicology Services, Cell Biology, Basel, Switzerland.

出版信息

Carcinogenesis. 1992 Jun;13(6):969-72. doi: 10.1093/carcin/13.6.969.

DOI:10.1093/carcin/13.6.969
PMID:1600618
Abstract

The formation of a glycidaldehyde-DNA adduct in skin of C3H mice treated with [14C]bisphenol A diglycidylether has been previously reported and it was assumed that the modification occurred on guanine residues. We were interested in elucidating the structure of this glycidaldehyde-DNA adduct by using a non-radioactive approach. Male C3H mice were treated with a single topical dose of 2 mg bisphenol A diglycidylether in acetone for 48, 96 or 192 h. An additional two mice were treated with 2 mg glycidaldehyde in acetone for 24 h. Epidermal DNA was isolated and enzymatically digested to nucleoside-3'-monophosphates. Aliquots of the DNA hydrolysates were separated on HPLC using a reverse-phase column with a potassium dihydrogen phosphate/methanol gradient. Fluorescence analysis of the eluent indicated the presence of a fluorescent DNA adduct, which was identified as hydroxymethylethenodeoxyadenosine-3'-monophosphate by comparison with a synthetic reference standard. Amounts of adducts were determined by fluorescence measurements using a calibration curve obtained with the authentic adduct standard. Irrespective of duration of exposure, all DNA hydrolysates of treated mice contained similar amounts of the deoxyadenosine adduct. The alkylation frequency was 0.1-0.8 and 166 adducts/10(6) normal nucleotides for the treatment with bisphenol A diglycidylether and glycidaldehyde respectively. The limit of detection using 500 micrograms DNA samples for analysis was approximately 0.03 adducts/10(6) normal nucleotides.

摘要

先前已有报道,用[14C]双酚A二缩水甘油醚处理的C3H小鼠皮肤中会形成缩水甘油醛 - DNA加合物,并且推测这种修饰发生在鸟嘌呤残基上。我们感兴趣的是通过使用非放射性方法来阐明这种缩水甘油醛 - DNA加合物的结构。雄性C3H小鼠用2毫克双酚A二缩水甘油醚的丙酮溶液单次局部给药,处理48、96或192小时。另外两只小鼠用2毫克缩水甘油醛的丙酮溶液处理24小时。分离表皮DNA并酶解为核苷 - 3'-单磷酸。DNA水解产物的等分试样在HPLC上使用带有磷酸二氢钾/甲醇梯度的反相柱进行分离。洗脱液的荧光分析表明存在一种荧光DNA加合物,通过与合成参考标准品比较,鉴定为羟甲基乙烯基脱氧腺苷 - 3'-单磷酸。通过使用由真实加合物标准品获得的校准曲线进行荧光测量来确定加合物的量。无论暴露持续时间如何,处理过的小鼠的所有DNA水解产物都含有相似量的脱氧腺苷加合物。双酚A二缩水甘油醚和缩水甘油醛处理的烷基化频率分别为0.1 - 0.8和166个加合物/10(6)个正常核苷酸。使用500微克DNA样品进行分析的检测限约为0.03个加合物/10(6)个正常核苷酸。

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Expression and DNA methylation changes in human breast epithelial cells after bisphenol A exposure.双酚 A 暴露后人类乳腺上皮细胞的表达和 DNA 甲基化变化。
Int J Oncol. 2012 Jul;41(1):369-77. doi: 10.3892/ijo.2012.1444. Epub 2012 Apr 20.
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Bisphenol A directly targets tubulin to disrupt spindle organization in embryonic and somatic cells.双酚A直接作用于微管蛋白,破坏胚胎细胞和体细胞中的纺锤体组织。
ACS Chem Biol. 2008 Mar 20;3(3):167-79. doi: 10.1021/cb700210u. Epub 2008 Jan 29.
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Prenatal bisphenol A exposure induces preneoplastic lesions in the mammary gland in Wistar rats.孕期暴露于双酚A会在Wistar大鼠的乳腺中诱发癌前病变。
Environ Health Perspect. 2007 Jan;115(1):80-6. doi: 10.1289/ehp.9282.
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Determination of bisphenol A and related aromatic compounds released from bis-GMA-based composites and sealants by high performance liquid chromatography.采用高效液相色谱法测定双酚A基复合材料和密封剂中释放的双酚A及相关芳香族化合物。
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