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用于评估职业性接触1,3 - 丁二烯的生物标志物。

Biomarkers for assessing occupational exposures to 1,3-butadiene.

作者信息

Albertini R J, Sram R J, Vacek P M, Lynch J, Wright M, Nicklas J A, Boogaard P J, Henderson R F, Swenberg J A, Tates A D, Ward J B

机构信息

Genetic Toxicology Laboratory, University of Vermont, 32 N. Prospect Street, Burlington, VT 05401, USA.

出版信息

Chem Biol Interact. 2001 Jun 1;135-136:429-53. doi: 10.1016/s0009-2797(01)00181-8.

Abstract

The overall objective of this study was to evaluate a continuum of biomarkers in blood and urine for their sensitivities as indicators of low level occupational exposures to 1,3 butadiene (BD). The study design was largely cross-sectional, with biological samples collected within a short timeframe. Personal 8-h BD exposure measures were made on several occasions over a 60-day period for each potentially exposed worker in order provide maximum accuracy for this independent variable and to accommodate the different expression intervals of the several biomarkers. Co-exposures to styrene, toluene and benzene were also measured. The study included 24 BD monomer production workers (mean BD exposure=0.642 mg/m(3)), 34 polymerization workers (mean BD exposure=1.794 mg/m(3)) and 25 controls (mean BD exposure=0.023 mg/m(3)). The several biomarkers were measured by a consortium of investigators at different locations in the US and Europe. These biomarkers included: (1) metabolic genotypes (CYP2E1, EH, GST M1, GST T1, ADH2, ADH3), determined in Prague and Burlington, VT; (2) urinary M1 and M2 metabolites (1,2-dihydroxy-4-[N-acetylcysteinyl]-butane and 1-hydroxy-2-[N-acetylcysteinyl]-3-butene, respectively), determined in Albuquerque, NM and Leiden; (3) hemoglobin adducts (N-[2-dihydroxy-3-butenyl]valine=HBVal and N-[2,3,4-trihydroxybutyl]valine=THBVal), determined in Amsterdam and Chapel Hill, NC, respectively; (4) HPRT mutations determined by autoradiographic assay in Galveston, TX, with slides re-read in Burlington, VT; (6) hypoxanthine-guanine phosphoribosyltransferase (HPRT) mutations determined by cloning assay in Leiden with mutational spectra characterized in Burlington, VT; (7) sister chromatid exchanges and chromosome aberrations determined by standard methods and FISH analysis in Prague. Urinary M1 and M2 metabolites and HBVal and THBVal hemoglobin adducts were all significantly correlated with BD exposure levels, with adducts being the most highly associated. No significant relationships were observed between BD exposures and HPRT mutations or any of the cytogenetic endpoints, regardless of method of assay.

摘要

本研究的总体目标是评估血液和尿液中的一系列生物标志物,以确定其作为低水平职业接触1,3 - 丁二烯(BD)指标的敏感性。研究设计主要为横断面研究,在短时间内收集生物样本。在60天内,对每位潜在接触工人进行了多次个人8小时BD暴露测量,以便为该自变量提供最大准确性,并适应几种生物标志物不同的表达间隔。同时还测量了苯乙烯、甲苯和苯的共同暴露情况。该研究包括24名BD单体生产工人(平均BD暴露量 = 0.642 mg/m³)、34名聚合工人(平均BD暴露量 = 1.794 mg/m³)和25名对照组人员(平均BD暴露量 = 0.023 mg/m³)。几种生物标志物由美国和欧洲不同地点的一组研究人员进行测量。这些生物标志物包括:(1)代谢基因型(CYP2E1、EH、GST M1、GST T1、ADH2、ADH3),在布拉格和佛蒙特州伯灵顿测定;(2)尿液中的M1和M2代谢物(分别为1,2 - 二羟基 - 4 - [N - 乙酰半胱氨酰基] - 丁烷和1 - 羟基 - 2 - [N - 乙酰半胱氨酰基] - 3 - 丁烯),在新墨西哥州阿尔伯克基和莱顿测定;(3)血红蛋白加合物(N - [2 - 二羟基 - 3 - 丁烯基]缬氨酸 = HBVal和N - [2,3,4 - 三羟基丁基]缬氨酸 = THBVal),分别在阿姆斯特丹和北卡罗来纳州教堂山测定;(4)通过放射自显影法在得克萨斯州加尔维斯顿测定HPRT突变,玻片在佛蒙特州伯灵顿重新读取;(6)通过克隆法在莱顿测定次黄嘌呤 - 鸟嘌呤磷酸核糖转移酶(HPRT)突变,并在佛蒙特州伯灵顿对突变谱进行表征;(7)通过标准方法和荧光原位杂交分析在布拉格测定姐妹染色单体交换和染色体畸变。尿液中的M1和M2代谢物以及HBVal和THBVal血红蛋白加合物均与BD暴露水平显著相关,其中加合物的相关性最高。无论采用何种检测方法,均未观察到BD暴露与HPRT突变或任何细胞遗传学终点之间存在显著关系。

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