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在人肝脏DNA中鉴定乙醛加合物并将其定量为N2-乙基脱氧鸟苷。

Identification of an acetaldehyde adduct in human liver DNA and quantitation as N2-ethyldeoxyguanosine.

作者信息

Wang Mingyao, Yu Nanxiong, Chen Li, Villalta Peter W, Hochalter J Bradley, Hecht Stephen S

机构信息

The Cancer Center, University of Minnesota, Mayo Mail Code 806, 420 Delaware Street SE, Minneapolis, Minnesota 55455, USA.

出版信息

Chem Res Toxicol. 2006 Feb;19(2):319-24. doi: 10.1021/tx0502948.

Abstract

Acetaldehyde, an ubiquitous mutagen and carcinogen, could be involved in human cancer etiology. Because DNA adducts are important in carcinogenesis, we have used liquid chromatography-electrospray ionization-tandem mass spectrometry (LC-ESI-MS/MS) to explore the presence in human liver DNA of the major acetaldehyde DNA adduct, N2-ethylidenedeoxyguanosine (1). DNA was isolated and enzymatically hydrolyzed in the presence of NaBH3CN, which quantitatively converts adduct 1 to N2-ethyldeoxyguanosine (N2-ethyl-dGuo, 2). [15N5]N2-Ethyl-dGuo was synthesized and used as an internal standard. Adduct 2 was enriched from the hydrolysate by solid phase extraction and analyzed by LC-ESI-MS/MS. Clear peaks were observed for adduct 2 in analyses of human liver DNA, calf thymus DNA, and rat liver DNA. These peaks were not observed, or were much smaller, when the NaBH3CN step was omitted. When the DNA was subjected to neutral thermal hydrolysis prior to NaBH3CN treatment, adduct 2 was not observed. Control experiments using [13C2]acetaldehyde demonstrated that adducts 1 and 2 were not formed as artifacts during DNA isolation and analysis. These results strongly indicate that adduct 1 is present in human liver DNA and demonstrate that it can be quantified as adduct 2. Levels of adduct 2 measured in 12 human liver samples were 534 +/- 245 fmol/micromol dGuo (mean +/- SD). The results of this study establish the presence of an acetaldehyde adduct in human liver DNA and suggest that it is a commonly occurring endogenous DNA adduct.

摘要

乙醛是一种普遍存在的诱变剂和致癌物,可能参与人类癌症的病因形成。由于DNA加合物在致癌过程中很重要,我们使用液相色谱 - 电喷雾电离 - 串联质谱法(LC - ESI - MS/MS)来探究人类肝脏DNA中主要的乙醛DNA加合物N2 - 乙叉脱氧鸟苷(1)的存在情况。分离DNA并在NaBH3CN存在下进行酶促水解,NaBH3CN可将加合物1定量转化为N2 - 乙基脱氧鸟苷(N2 - ethyl - dGuo,2)。合成了[15N5]N2 - Ethyl - dGuo并用作内标。通过固相萃取从水解产物中富集加合物2,并通过LC - ESI - MS/MS进行分析。在对人类肝脏DNA、小牛胸腺DNA和大鼠肝脏DNA的分析中观察到了加合物2的清晰峰。当省略NaBH3CN步骤时,未观察到这些峰,或者峰要小得多。当DNA在NaBH3CN处理之前进行中性热水解时,未观察到加合物2。使用[13C2]乙醛进行的对照实验表明,在DNA分离和分析过程中不会作为假象形成加合物1和2。这些结果有力地表明加合物1存在于人类肝脏DNA中,并证明它可以作为加合物2进行定量。在12个人类肝脏样本中测得的加合物2水平为534±245 fmol/μmol dGuo(平均值±标准差)。本研究结果证实了人类肝脏DNA中存在乙醛加合物,并表明它是一种常见的内源性DNA加合物。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/9448/3199962/de4aa48c0d01/nihms63261f1.jpg

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