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探究8:2氟调聚物丙烯酸酯的体外蛋白质组半胱氨酸反应活性。

Querying the In Vitro Proteome Cysteine Reactivity of 8:2 Fluorotelomer Acrylate.

作者信息

Hall David Ross, Gauthier Jeremy, Peng Hui

机构信息

Department of Chemistry, University of Toronto, Toronto, Ontario M5S 1A1, Canada.

School of the Environment, University of Toronto, Toronto, Ontario M5S 1A1, Canada.

出版信息

Environ Sci Technol. 2023 Sep 5;57(35):13015-13024. doi: 10.1021/acs.est.3c02930. Epub 2023 Aug 22.

DOI:10.1021/acs.est.3c02930
PMID:37607404
Abstract

Despite the phase out of legacy per- and polyfluoroalkyl substances (PFAS), fluorotelomer-based polymers (FTP) have been used for many applications, notably textile surface coatings. FTPs are of a health concern due to their breakdown into legacy PFAS and the co-occurrence of fluorotelomer acrylate (FTAC) monomers, of which the latter may potentially react with cellular thiols. To evaluate this hypothesis, we employed fluorous-solid-phase extraction (FSPE), to enrich peptides covalently modified by 8:2 fluorotelomer acrylate (8:2 FTAC) and coupled it to a modified nano-liquid chromatography method for the identification of in vitro protein adducts using bottom-up data-dependent proteomics analysis. Using this method, over 100 unique peptides were detected with 8:2 FTAC modifications, although none of the modified cysteine residues were annotated active site nucleophiles. In parallel, a synthetic CF-iodoacetamide (F-IAM) chemical probe was used to gauge the upper bound of PFAS-thiol reactivity. Over seven hundred peptides were detected with modifications but only 9 of 28 annotated active site cysteines in this dataset were modified by F-IAM. Further exploration of the impacts of 8:2 FTAC adducts on protein function revealed that 8:2 FTAC modification promotes protein aggregation in vitro. These results suggest that 8:2 FTAC may exhibit significant proteome thiol reactivity and imply a more general mechanism of toxicity of PFAS-induced protein aggregation.

摘要

尽管传统的全氟和多氟烷基物质(PFAS)已逐步淘汰,但基于氟调聚物的聚合物(FTP)仍被用于许多应用,尤其是纺织品表面涂层。由于FTP会分解为传统的PFAS,且同时存在氟调聚物丙烯酸酯(FTAC)单体,因此其对健康存在潜在威胁,后者可能会与细胞中的硫醇发生反应。为了验证这一假设,我们采用了氟固相萃取(FSPE)技术来富集经8:2氟调聚物丙烯酸酯(8:2 FTAC)共价修饰的肽段,并将其与一种改进的纳米液相色谱方法相结合,通过自下而上的数据依赖蛋白质组学分析来鉴定体外蛋白质加合物。使用该方法,共检测到100多个带有8:2 FTAC修饰的独特肽段,不过所有修饰的半胱氨酸残基均未被注释为活性位点亲核试剂。同时,使用一种合成的CF-碘乙酰胺(F-IAM)化学探针来评估PFAS与硫醇反应活性的上限。在该数据集中,共检测到700多个带有修饰的肽段,但其中28个注释的活性位点半胱氨酸中只有9个被F-IAM修饰。对8:2 FTAC加合物对蛋白质功能影响的进一步探索表明,8:2 FTAC修饰会促进体外蛋白质聚集。这些结果表明,8:2 FTAC可能具有显著的蛋白质组硫醇反应活性,并暗示了PFAS诱导蛋白质聚集的更普遍毒性机制。

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