Fedtke N, Boucheron J A, Turner M J, Swenberg J A
Chemical Industry Institute of Toxicology, Department of Biochemical Toxicology and Pathobiology, Research Triangle Park, NC 27709.
Carcinogenesis. 1990 Aug;11(8):1279-85. doi: 10.1093/carcin/11.8.1279.
A sensitive assay for quantitative determination of the vinyl chloride (VC)-induced cyclic DNA adduct N2,3-ethenoguanine (EG) was developed. The method is based on the detection of EG as its di-pentafluorobenzyl derivative (3,5-PFB2-EG). This compound exhibited good gas chromatographic properties and was detected with high sensitivity by gas chromatography with electron capture detection (limit of detection 300 amol/microliters injected solution) or with negative ion chemical ionization mass spectrometry monitoring the [M-181]-fragment ion at m/z 354 (GC-NICI-MS, limit of detection 190 amol/microliters injected solution). EG, its 13C-labeled analog [13C4]-EG and 3,5-PFB2-EG were synthesized and characterized by UV and fluorescence spectrophotometry, 1H- and 13C-NMR spectroscopy and mass spectrometry. The standards were used to optimize the isolation of EG and its derivatization with pentafluorobenzyl bromide (electrophore labeling) at fmol quantities. DNA solutions were spiked with EG, the DNA was depurinated by mild acid hydrolysis, and EG was isolated from the hydrolysates by low-pressure strong cation exchange chromatography with subsequent C18 solid-phase extraction. The extracted EG was electrophore labeled and 3,5-PFB2-EG was detected using GC-NICI-MS. [13C4]EG served as internal standard. 3,5-PFB2-EG was quantitated relative to its 13C-labeled analog by measuring the ion ratio m/z 354/358. The limit of detection for the complete method was 60 fmol EG/mumols guanine. The method was applied to liver DNA from young Sprague-Dawley rats exposed to 600 p.p.m. VC from day 10 through day 14 after birth. The EG concentration in these samples was 1.8 +/- 0.3 pmol/mumols guanine.
开发了一种用于定量测定氯乙烯(VC)诱导的环状DNA加合物N2,3 - 乙烯基鸟嘌呤(EG)的灵敏检测方法。该方法基于将EG检测为其二 - 五氟苄基衍生物(3,5 - PFB2 - EG)。该化合物具有良好的气相色谱性质,通过带有电子捕获检测的气相色谱法(检测限为每微升进样溶液300 amol)或通过负离子化学电离质谱法监测质荷比为354的[M - 181] - 碎片离子(GC - NICI - MS,检测限为每微升进样溶液190 amol)进行高灵敏度检测。合成了EG、其13C标记的类似物[13C4] - EG和3,5 - PFB2 - EG,并通过紫外和荧光分光光度法、1H - 和13C - NMR光谱法以及质谱法对其进行了表征。这些标准品用于以飞摩尔量优化EG的分离及其与五氟苄基溴的衍生化反应(电泳标记)。向DNA溶液中加入EG,通过温和的酸水解使DNA脱嘌呤,然后通过低压强阳离子交换色谱法从水解产物中分离出EG,随后进行C18固相萃取。对提取的EG进行电泳标记,并使用GC - NICI - MS检测3,5 - PFB2 - EG。[13C4]EG用作内标。通过测量质荷比354/358的离子比率,相对于其13C标记的类似物对3,5 - PFB2 - EG进行定量。该完整方法的检测限为60 fmol EG/μmol鸟嘌呤。该方法应用于出生后第10天至第14天暴露于600 ppm VC的幼年Sprague - Dawley大鼠的肝脏DNA。这些样品中EG的浓度为1.8±0.3 pmol/μmol鸟嘌呤。
