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两种荧光探针在人血清白蛋白I位点的协同结合:该蛋白质作为一种支架促进荧光共振能量转移。

Concomitant binding of two fluorescent probes at site-I of human serum albumin: The protein acting as a scaffold enabling fluorescence resonance energy transfer.

作者信息

Ximenes Valdecir Farias

机构信息

Department of Chemistry, Faculty of Sciences, UNESP - São Paulo State University, 17033-360 Bauru, São Paulo, Brazil.

出版信息

J Photochem Photobiol B. 2022 Sep;234:112542. doi: 10.1016/j.jphotobiol.2022.112542. Epub 2022 Aug 10.

DOI:10.1016/j.jphotobiol.2022.112542
PMID:35973286
Abstract

Human serum albumin (HSA) is the primary drug carrier in the blood plasma. Here, I aimed to show that two ligands can be accommodated simultaneously in the binding site-I of HSA. To do so, I studied the interaction inside the protein among site-I ligands of HSA via fluorescence resonance energy transfer (FRET), synchronous fluorescence, red edge excitation shift (REES), and induced circular dichroism (ICD). Warfarin (WAR), coumarin-153 (C153), 6-(p-toluidino)-2-naphthalenesulfonic acid sodium salt (TNS), dansylglycine (DGY), and 4-(dicyanomethylene)-2-methyl-6-(4-dimethylaminostyryl)-4H-pyran (DCM) were enrolled in the investigation. I found that WAR can transfer energy to C153 only in the presence of the protein. In addition, the presence of WAR at site-I altered the protein microenvironment felt by C153. The alteration was detected by measuring the synchronous fluorescence, REES, and ICD in C153. The findings were validated by measuring the energy transfer from TNS to DCM and the alteration in synchronous fluorescence and REES. FRET was not observed using WAR as donor and DGY as acceptor. The result is consistent, as DGY is a site-II ligand at a higher WAR distance. In all studied cases, the effects were only observed in the presence of HSA. In conclusion, the protein acted as a scaffold approximating the ligands. These findings prove that more than one ligand can simultaneously be complex at site-I of HSA.

摘要

人血清白蛋白(HSA)是血浆中的主要药物载体。在此,我的目的是证明两个配体可以同时容纳在HSA的结合位点I中。为此,我通过荧光共振能量转移(FRET)、同步荧光、红边激发位移(REES)和诱导圆二色性(ICD)研究了HSA的位点I配体之间在蛋白质内部的相互作用。华法林(WAR)、香豆素-153(C153)、6-(对甲苯胺基)-2-萘磺酸钠盐(TNS)、丹磺酰甘氨酸(DGY)和4-(二氰基亚甲基)-2-甲基-6-(4-二甲基氨基苯乙烯基)-4H-吡喃(DCM)被纳入研究。我发现只有在蛋白质存在的情况下,WAR才能将能量转移到C153。此外,位点I处WAR的存在改变了C153所感受到的蛋白质微环境。通过测量C153中的同步荧光、REES和ICD检测到了这种改变。通过测量从TNS到DCM的能量转移以及同步荧光和REES的变化验证了这些发现。未观察到以WAR为供体、DGY为受体的FRET。结果是一致的,因为DGY是距离WAR较远的位点II配体。在所有研究的情况下,只有在HSA存在时才观察到这些效应。总之,蛋白质起到了使配体接近的支架作用。这些发现证明不止一个配体可以同时在HSA的位点I处形成复合物。

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