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生物活性黄酮中的激发态分子内质子转移为其与靶蛋白的结合提供了可用于识别的荧光观察指标。

Excited-state intramolecular proton transfer in a bioactive flavonoid provides fluorescence observables for recognizing its engagement with target proteins.

机构信息

Department of Chemical and Geological Sciences, University of Modena and Reggio Emilia (UNIMORE), Via Campi 103, 41125 Modena, Italy.

Department of Life Sciences, University of Modena and Reggio Emilia (UNIMORE), Via Campi 103, 41125 Modena, Italy.

出版信息

Photochem Photobiol Sci. 2019 Sep 1;18(9):2270-2280. doi: 10.1039/c9pp00026g. Epub 2019 Mar 22.

DOI:10.1039/c9pp00026g
PMID:30900698
Abstract

A benzothiophene-substituted chromenone with promising activity against Leishmania and Trypanosoma species exhibits peculiar fluorescence properties useful for identifying its complexes with target proteins in the microorganism proteomes. The emission spectra, anisotropy and time profiles of this flavonoid strongly change when moving from the free to the protein-bound forms. The same two types of emission are observed in organic solvents and their mixtures with water, with the relative band intensities depending on the solvent ability to establish hydrogen bonds with the solute. The regular emission prevails in protic solvents, while in aprotic solvents the anomalously red-shifted emission occurs from a zwitterionic tautomeric form, produced in the excited state by proton transfer within the intramolecularly H-bonded form. This interpretation finds support from an experimental and theoretical investigation of the conformational preferences of this compound in the ground and lowest excited state, with a focus on the relative twisting about the chromenone-benzothiophene interconnecting bond. An analysis of the absorption and emission spectra and of the photophysical properties of the two emitting tautomers highlights the relevance of the local microenvironment, particularly of the intra- and intermolecular hydrogen bonds in which this bioactive compound is involved, in determining both its steady-state and time-resolved fluorescence behaviour.

摘要

一种具有抗利什曼原虫和锥虫属物种活性的苯并噻吩取代色烯酮,具有独特的荧光性质,可用于鉴定其与微生物蛋白质组中靶蛋白的复合物。当从游离形式转变为蛋白质结合形式时,这种类黄酮的发射光谱、各向异性和时间分布会发生强烈变化。在有机溶剂及其与水的混合物中,观察到相同的两种类型的发射,其相对带强度取决于溶剂与溶质形成氢键的能力。在质子溶剂中,规则发射占主导地位,而在非质子溶剂中,异常红移发射则来自于分子内氢键形成的内酰胺互变异构体,该互变异构体通过质子转移在激发态中产生。这种解释得到了实验和理论研究的支持,这些研究关注的是该化合物在基态和最低激发态下的构象偏好,重点是关于色烯酮-苯并噻吩连接键的相对扭转。对两种发射互变异构体的吸收和发射光谱以及光物理性质的分析,突出了局部微环境的相关性,特别是涉及该生物活性化合物的分子内和分子间氢键,对其稳态和时间分辨荧光行为都有影响。

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