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通过在荧光开启型方酸-蒽醌三联体中破坏电子转移来测定万古霉素。

Vancomycin Determination by Disrupting Electron-Transfer in a Fluorescence Turn-On Squaraine-Anthraquinone Triad.

机构信息

Division of Chemistry and Biological Chemistry, School of Physical and Mathematical Sciences , Nanyang Technological University , 21 Nanyang Link , Singapore 637371.

出版信息

ACS Sens. 2018 Jun 22;3(6):1156-1163. doi: 10.1021/acssensors.8b00188. Epub 2018 Jun 7.

DOI:10.1021/acssensors.8b00188
PMID:29792330
Abstract

A highly sensitive and selective probe for Vancomycin (Van) in aqueous and serum samples is developed in this study. The probe is based on a triad consisting of a near-infrared squaraine dye (Seta-640) conjugated to two anthraquinone molecules via Lys-d-Ala-d-Ala peptides. In the absence of Van, the close proximity and efficient electron-transfer from the excited Seta-640 dye to anthraquinone result in significant fluorescence quenching of the dye ("off"-state). When Van is added, the antibiotic molecules bind with high affinity to the -d-Ala-d-Ala ligands in a 2:1 stoichiometry (Van:triad), resulting in fluorescence recovery that is as high as 30 times ("on"-state). Even though bound Van enhances the fluorescence by reducing the rate of (intrinsic) polarity-induced nonradiative decay process, this effect plays only a minor role. Instead, the main reason behind the observed fluorescence recovery after drug binding is the effective inhibition of electron-transfer; plausibly arising from a steric-induced lengthening of the spatial separation between electron donor and acceptor. The probe has detection limits of 7.0 and 96.9 nM in buffer and human serum, respectively, operates in the clinically relevant range, is insensitive to Van crystalline degradation product (CDP-1), and is easy to operate by using a commonly available fluorescence spectrometer.

摘要

本研究开发了一种在水相和血清样品中检测万古霉素(Van)的高灵敏和高选择性探针。该探针基于三联体结构,由近红外方酸染料(Seta-640)通过赖氨酸-d-丙氨酸-d-丙氨酸肽连接两个蒽醌分子组成。在没有 Van 的情况下,由于受激 Seta-640 染料与蒽醌之间的紧密接近和有效电子转移,导致染料的荧光显著猝灭(“关”态)。当添加 Van 时,抗生素分子以 2:1 的化学计量比(Van:三联体)与-d-Ala-d-Ala 配体高亲和力结合,导致荧光恢复高达 30 倍(“开”态)。尽管结合的 Van 通过降低由极性诱导的非辐射衰减过程的速率来增强荧光,但这种效应仅起次要作用。相反,药物结合后观察到的荧光恢复的主要原因是电子转移的有效抑制;可能是由空间分离的立体诱导延长引起的。该探针在缓冲液和人血清中的检测限分别为 7.0 和 96.9 nM,在临床相关范围内工作,对 Van 晶体降解产物(CDP-1)不敏感,并且使用常用的荧光光谱仪即可轻松操作。

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