Gavina Jennilee M A, Rubab Mamoona, Zhang Huijuan, Zhu Jiping, Nong Andy, Feng Yong-Lai
Exposure and Biomonitoring Division, Health Canada, AL: 0800C, EHC, Tunney's Pasture, Ottawa, Ontario, Canada K1A 0K9.
J Environ Monit. 2011 Nov;13(11):3145-55. doi: 10.1039/c1em10511f. Epub 2011 Oct 19.
DNA damage represents a potential biomarker for determining the exposure risk to chemicals and may provide early warning data for identifying chemical hazards to human health. Here, we have demonstrated a simple chromatography-based method that can be used to rapidly screen for the presence of chemical hazards as well as to determine parameters relevant to hazard assessment. In this proof-of-principle study, a simple in vitro system was used to determine the interaction of pollutants and probable carcinogens, phenyl glycidyl ether (PGE), tetrachlorohydroquinone (Cl(4)HQ), methylmethane sulfonate (MMS), styrene-7,8-oxide (SO), and benzo[a]pyrene-7,8-dihydrodiol-9,10-epoxide (BPDE), a metabolite of benzo[a]pyrene (B[a]P), with single- and double-stranded DNA probes. Differences in potency and reaction kinetics were studied for chemical and DNA type. A relative interaction potency equivalency (PEQ) of a chemical was determined by ratio of interaction potency of a chemical to BPDE as the reference chemical in the reaction with single- and double-stranded oligodeoxynucleotides. PEQs were found to be BPDE > PGE > SO > MMS > Cl(4)HQ for single-stranded oligodeoxynucleotides while they were found to be BPDE > PGE > Cl(4)HQ > MMS > SO for double-stranded oligodeoxynucleotides. Kinetics evaluation revealed that BPDE reacted with both DNA probes at a significantly faster rate, as compared to the remaining test chemicals. Equilibrium was reached within an hour for BPDE, but required a minimum of 48 h for the remaining chemicals. First-order rate constants were (1.61 ± 0.2) × 10(-3) s(-1) and (3.18 ± 0.4) × 10(-4) s(-1) for reaction of BPDE with double- and single-stranded DNA, respectively. The remaining chemicals possessed rate constants from 2 to 13 × 10(-6) s(-1) with a relative kinetic order for reaction with DNA of BPDE ≫ MMS > SO > PGE > Cl(4)HQ for ds-DNA and BPDE ≫ SO ≈ Cl(4)HQ ≈ MMS > PGE for ss-DNA. We further found that the reaction potency, defined by dose-response between chemical pollutants and DNA, depends on the form of DNA present for reaction. Noteworthy, we found that relative PEQ did not follow the same kinetic trends. However, our preliminary findings suggest that reaction kinetics, in combination with relative interaction potency, may be a significant parameter that can be used to evaluate the hazard level of environmental pollutants.
DNA损伤是确定化学物质暴露风险的潜在生物标志物,可为识别化学物质对人类健康的危害提供早期预警数据。在此,我们展示了一种基于色谱的简单方法,可用于快速筛查化学危害的存在,并确定与危害评估相关的参数。在这项原理验证研究中,使用了一个简单的体外系统来确定污染物与可能的致癌物苯基缩水甘油醚(PGE)、四氯对苯二酚(Cl(4)HQ)、甲磺酸甲酯(MMS)、苯乙烯-7,8-氧化物(SO)以及苯并[a]芘的代谢物苯并[a]芘-7,8-二氢二醇-9,10-环氧化物(BPDE)与单链和双链DNA探针的相互作用。研究了化学物质和DNA类型在效力和反应动力学方面的差异。通过化学物质与BPDE在与单链和双链寡脱氧核苷酸反应中的相互作用效力之比,确定了化学物质的相对相互作用效力当量(PEQ)。对于单链寡脱氧核苷酸,发现PEQ顺序为BPDE > PGE > SO > MMS > Cl(4)HQ,而对于双链寡脱氧核苷酸,顺序为BPDE > PGE > Cl(4)HQ > MMS > SO。动力学评估表明,与其余测试化学物质相比,BPDE与两种DNA探针的反应速度明显更快。BPDE在一小时内达到平衡,但其余化学物质至少需要48小时。BPDE与双链和单链DNA反应的一级速率常数分别为(1.61 ± 0.2) × 10(-3) s(-1)和(3.18 ± 0.4) × 10(-4) s(-1)。其余化学物质的速率常数为2至13 × 10(-6) s(-1),与双链DNA反应的相对动力学顺序为BPDE ≫ MMS > SO > PGE > Cl(4)HQ,与单链DNA反应的顺序为BPDE ≫ SO ≈ Cl(4)HQ ≈ MMS > PGE。我们进一步发现,由化学污染物与DNA之间的剂量反应定义的反应效力取决于反应中存在的DNA形式。值得注意的是,我们发现相对PEQ并不遵循相同的动力学趋势。然而,我们的初步研究结果表明,反应动力学与相对相互作用效力相结合,可能是用于评估环境污染物危害水平的一个重要参数。
