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非诺贝特酸介导的光过敏反应的机制研究:与血清白蛋白的光反应性

Mechanistic Studies on the Photoallergy Mediated by Fenofibric Acid: Photoreactivity with Serum Albumins.

作者信息

Vayá Ignacio, Andreu Inmaculada, Monje Vicente T, Jiménez M Consuelo, Miranda Miguel A

机构信息

Departamento de Química/Instituto de Tecnología Química UPV-CSIC, Universitat Politècnica de València , Camino de Vera s/n, 46022 Valencia, Spain.

Unidad Mixta de Investigación IIS La Fe-UPV, Hospital Universitari i Politècnic La Fe , Avenida de Fernando Abril Martorell 106, 46026 Valencia, Spain.

出版信息

Chem Res Toxicol. 2016 Jan 19;29(1):40-6. doi: 10.1021/acs.chemrestox.5b00357. Epub 2015 Dec 17.

DOI:10.1021/acs.chemrestox.5b00357
PMID:26633742
Abstract

The photoreactivity of fenofibric acid (FA) in the presence of human and bovine serum albumins (HSA and BSA, respectively) has been investigated by steady-state irradiation, fluorescence, and laser flash photolysis (LFP). Spectroscopic measurements allowed for the determination of a 1:1 stoichiometry for the FA/SA complexes and pointed to a moderate binding of FA to the proteins; by contrast, the FA photoproducts were complexed more efficiently with SAs. Covalent photobinding to the protein, which is directly related to the photoallergic properties of the drug, was detected after long irradiation times and was found to be significantly higher in the case of BSA. Intermolecular FA-amino acid and FA-albumin irradiations resulted in the formation of photoproducts arising from coupling between both moieties, as indicated by mass spectrometric analysis. Mechanistic studies using model drug-amino acid linked systems indicated that the key photochemical step involved in photoallergy is formal hydrogen atom transfer from an amino acid residue to the excited benzophenone chromophore of FA or (more likely) its photoproducts. This results in the formation of caged radical pairs followed by C-C coupling to give covalent photoaducts.

摘要

通过稳态辐照、荧光和激光闪光光解(LFP)研究了非诺贝特酸(FA)在人血清白蛋白(HSA)和牛血清白蛋白(BSA)存在下的光反应活性。光谱测量确定了FA/SA复合物的化学计量比为1:1,并表明FA与蛋白质的结合较弱;相比之下,FA光产物与SA的结合更有效。长时间辐照后检测到与蛋白质的共价光结合,这与药物的光过敏特性直接相关,并且发现BSA的共价光结合明显更高。质谱分析表明,分子间FA-氨基酸和FA-白蛋白辐照导致两个部分之间偶联形成光产物。使用模型药物-氨基酸连接系统的机理研究表明,光过敏中涉及的关键光化学步骤是从氨基酸残基到FA或(更可能)其光产物的激发二苯甲酮发色团的正式氢原子转移。这导致笼形自由基对的形成,随后通过C-C偶联产生共价光加合物。

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