Regulation of Promoter-CAT Stress Genes in HepG2 Cells by Suspensions of Particles from Ambient Air

Renaud Vincent , Patrick Goegan , Gala Johnson , Jeffrey R. Brook , Prem Kumarathasan , Léo Bouthillier , Richard T. Burnett
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引用次数: 57

Abstract

A panel of HepG2-derived cell lines (CAT-Tox [L] assay, Xenometrix), harboring stress genes consisting of a sequence for chloramphenicol acetyltransferase (CAT) under the transcriptional regulation from mammalian promoters and response elements, was exposed for 18–24 hr to aqueous suspensions of urban dusts (SRM-1648, SRM-1649, EHC-93) or PM2.5 particles (particulate matter < 2.5 μm). Expression of CAT protein was measured by enzyme-linked immunosorbent assay. Induction of the CAT genes was verified with benzo[a]pyrene (CYP1A1, cytochrome P450 1A1 promoter; GSTYa, glutathione transferase subunit Ya promoter; XRE, xenobiotic response element), cadmium sulfate, and copper sulfate (HMTIIa, metallothionein IIa promoter; HSP70, heat shock protein 70 promoter). The urban dust suspensions were active on CYP1A1, GSTYa, and XRE cell lines. SRM-1648 and SRM-1649 were twice as potent as EHC-93 per unit mass in inducing the xenobiotic-dependent responses, which correlated with contents in polycyclic aromatic hydrocarbons. These three reference particles, as well as six PM2.5 preparations collected on hi-vol filters in the Great Lakes basin, were also found to induce HMTIIa and HSP70, the magnitude of the responses correlating closely with the amount of soluble copper in the particulate preparations. The results indicate that bioavailable chemical species in the unfractionated particles can directly and quantitatively induce xenobiotic, metal, and stress-dependent responses in a target cell model, resulting in patterns of gene induction consistent with the chemical compositions of the environmental materials. We propose that cell culture models could be helpful for toxicodynamic inferences in adjunct to environmental monitoring and exposure assessments.

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环境空气颗粒悬浮液对HepG2细胞启动子- cat应激基因的调控
将一组hepg2衍生的细胞系(CAT- tox [L] assay, Xenometrix)暴露于城市粉尘(SRM-1648, SRM-1649, EHC-93)或PM2.5颗粒(颗粒物和污染物)的水悬浮液中18-24小时,其中含有由哺乳动物启动子和应答元件转录调控的氯霉素乙酰转移酶(CAT)序列组成的应激基因。2.5μm)。酶联免疫吸附法检测CAT蛋白表达。用苯并[a]芘(CYP1A1,细胞色素P450 1A1启动子;GSTYa,谷胱甘肽转移酶亚基Ya启动子;XRE,异种反应元件)、硫酸镉、硫酸铜(HMTIIa,金属硫蛋白IIa启动子;热休克蛋白70启动子)。城市粉尘悬浮液对CYP1A1、GSTYa和XRE细胞均有活性。SRM-1648和SRM-1649诱导的外源依赖性反应与多环芳烃含量相关,是单位质量EHC-93的2倍。这三种参考颗粒以及五大湖流域高容量过滤器收集的六种PM2.5制剂也可以诱导HMTIIa和HSP70,其响应的大小与颗粒制剂中可溶性铜的含量密切相关。结果表明,未分离颗粒中的生物可利用化学物质可以在靶细胞模型中直接和定量地诱导外源、金属和应力依赖性反应,导致基因诱导模式与环境材料的化学成分一致。我们建议细胞培养模型可以辅助环境监测和暴露评估进行毒理学推断。
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