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取代对苯醌和对苯二酚的体外生物测定中的毒性效应会受到与细胞测定介质的反应的影响而改变。

Toxic effects of substituted p-benzoquinones and hydroquinones in in vitro bioassays are altered by reactions with the cell assay medium.

机构信息

Eawag, Swiss Federal Institute of Aquatic Science and Technology, Duebendorf CH-8600, Switzerland; Department of Chemistry and Bioscience, Aalborg University, Aalborg 9220, Denmark.

Department of Cell Toxicology, UFZ - Helmholtz Centre for Environmental Research, Leipzig 04318, Germany; Center for Applied Geoscience, Eberhard Karls University of Tübingen, Schnarrenbergstr. 94-96, Tübingen 72076, Germany.

出版信息

Water Res. 2021 Sep 1;202:117415. doi: 10.1016/j.watres.2021.117415. Epub 2021 Jul 7.

Abstract

Substituted para-benzoquinones and hydroquinones are ubiquitous transformation products that arise during oxidative water treatment of phenolic precursors, for example through ozonation or chlorination. The benzoquinone structural motive is associated with mutagenicity and carcinogenicity, and also with induction of the oxidative stress response through the Nrf2 pathway. For either endpoint, toxicological data for differently substituted compounds are scarce. In this study, oxidative stress response, as indicated by the AREc32 in vitro bioassay, was induced by differently substituted para-benzoquinones, but also by the corresponding hydroquinones. Bioassays that indicate defense against genotoxicity (p53RE-bla) and DNA repair activity (UmuC) were not activated by these compounds. Stability tests conducted under incubation conditions, but in the absence of cell lines, showed that tested para-benzoquinones reacted rapidly with constituents of the incubation medium. Compounds were abated already in phosphate buffer, but even faster in biological media, with reactions attributed to amino- and thiol-groups of peptides, proteins, and free amino acids. The products of these reactions were often the corresponding substituted hydroquinones. Conversely, differently substituted hydroquinones were quantitatively oxidized to p-benzoquinones over the course of the incubation. The observed induction of the oxidative stress response was attributed to hydroquinones that are presumably oxidized to benzoquinones inside the cells. Despite the instability of the tested compounds in the incubation medium, the AREc32 in vitro bioassay could be used as an unspecific sum parameter to detect para-benzoquinones and hydroquinones in oxidatively treated waters.

摘要

取代对苯二酚和对苯醌是在酚类前体的氧化水处理过程中产生的普遍转化产物,例如通过臭氧化或氯化。苯醌结构基与致突变性和致癌性有关,也与通过 Nrf2 途径诱导氧化应激反应有关。对于任一终点,具有不同取代基的化合物的毒理学数据都很缺乏。在这项研究中,不同取代的对苯醌会诱导氧化应激反应,如 AREc32 体外生物测定所示,但也会诱导相应的对苯二酚。指示针对遗传毒性的防御(p53RE-bla)和 DNA 修复活性(UmuC)的生物测定未被这些化合物激活。在孵育条件下但在没有细胞系的情况下进行的稳定性测试表明,测试的对苯醌与孵育介质的成分迅速反应。在磷酸盐缓冲液中,化合物已经被衰减,但在生物介质中更快,反应归因于肽、蛋白质和游离氨基酸的氨基和巯基。这些反应的产物通常是相应的取代对苯二酚。相反,不同取代的对苯二酚在孵育过程中被定量氧化为对苯醌。观察到的氧化应激反应的诱导归因于可能在细胞内氧化为苯醌的对苯二酚。尽管测试化合物在孵育介质中的不稳定性,但 AREc32 体外生物测定可作为一种非特异性的总和参数,用于检测氧化处理水中的对苯醌和对苯二酚。

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