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对映体特异性生物转化率的全氟辛烷磺酸 (PFOS)-前体通过细胞色素 P450 同工酶和人肝微粒体。

Isomer-specific biotransformation rates of a perfluorooctane sulfonate (PFOS)-precursor by cytochrome P450 isozymes and human liver microsomes.

机构信息

Division of Analytical and Environmental Toxicology, Department of Laboratory Medicine, University of Alberta, Canada.

出版信息

Environ Sci Technol. 2009 Nov 15;43(22):8566-72. doi: 10.1021/es901915f.

DOI:10.1021/es901915f
PMID:20028053
Abstract

The exposure sources of perfluorooctane sulfonate (PFOS) in humans and wildlife are not well characterized. Human biomonitoring data show that PFOS profiles may consist of up to approximately 50% branched isomers, despite the fact that historical direct manufacturing of PFOS generally resulted in products containing no more than approximately 30% branched isomers. These observations cannot be explained based on what is known about the pharmacokinetics of branched PFOS isomers; thus, here we examined the relative isomer-specific biotransformation rates of a model PFOS-precursor (N-ethylperfluorooctane sulfonamide, NEtFOSA) with human microsomes and recombinant human cytochrome P450s (CYPs) 2C9 and 2C19. Using solid phase microextraction-gas chromatography-electron capture detection to monitor NEtFOSA disappearance, and liquid chromatography-tandem mass spectrometry to monitor product formation, we showed that, in general, human microsomes and CYP isozymes transformed the branched isomers more rapidly than linear NEtFOSA. Among branched isomers, perfluoroalkyl branching geometry significantly influenced the rate of biotransformation. As a result, PFOS isomer patterns in biota exposed predominantly to precursors could be much different than expected from the isomer pattern of the precursor. While these data are suggestive that the relatively high abundance of branched PFOS isomers present in some humans, or wildlife, may be explained by substantial exposure to PFOS-precursors, in vivo studies with other relevant PFOS-precursors are warranted to validate this as a biomarker of exposure source.

摘要

全氟辛烷磺酸(PFOS)在人类和野生动物中的暴露源尚未得到很好的描述。人体生物监测数据表明,PFOS 谱可能由多达约 50%的支链异构体组成,尽管历史上直接制造 PFOS 通常导致产品中不超过约 30%的支链异构体。这些观察结果无法根据我们对支链 PFOS 异构体药代动力学的了解来解释;因此,在这里我们研究了模型 PFOS 前体(N-乙基全氟辛烷磺酰胺,NEtFOSA)与人微粒体和重组人细胞色素 P450(CYP)2C9 和 2C19 的相对异构体特异性生物转化率。使用固相微萃取-气相色谱-电子捕获检测监测 NEtFOSA 的消失,并用液相色谱-串联质谱监测产物形成,我们表明,通常情况下,人微粒体和 CYP 同工酶比线性 NEtFOSA 更快地转化支链异构体。在支链异构体中,全氟烷基分支几何形状显著影响生物转化速率。因此,主要暴露于前体的生物群中 PFOS 异构体模式可能与前体的异构体模式有很大不同。虽然这些数据表明,一些人类或野生动物中存在的相对高丰度的支链 PFOS 异构体可能是由于大量暴露于 PFOS 前体所致,但需要进行其他相关 PFOS 前体的体内研究来验证这一点作为暴露源的生物标志物。

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