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吖啶橙-十二烷基苯磺酸钠-蛋白质体系中吖啶橙二聚体的形成与解聚研究

Study on the formation and depolymerization of acridine orange dimer in acridine orange-sodium dodecyl benzene sulfonate-protein system.

作者信息

Wang Fei, Yang Jinghe, Wu Xia, Wang Xiaobo, Feng Lishun, Jia Zhen, Guo Changying

机构信息

Key Laboratory of Colloid and Interface Chemistry (Shandong University), Ministry of Education, School of Chemistry and Chemical Engineering, Shandong University, Jinan 250100, PR China.

出版信息

J Colloid Interface Sci. 2006 Jun 15;298(2):757-64. doi: 10.1016/j.jcis.2006.01.028. Epub 2006 Feb 3.

Abstract

Experiment indicates that the fluorescence of acridine orange (AO) can be greatly quenched by anionic surfactant sodium dodecyl benzene sulfonate (SDBS), but when protein is added into the AO-SDBS system, the fluorescence intensity of the latter is enhanced. It is considered that SDBS can promote the formation of AO dimer, resulting in the quenching of the fluorescence of AO. When bovine serum albumin (BSA) is added into AO-SDBS system, BSA and SDBS can interact and form negative micelle-like cluster complex with "aromatic ring stacking," which destroys the formation conditions of AO dimer and makes some AO dimers turn into monomer, resulting in the fluorescence enhancement of AO-SDBS system. Whereas the positive AO and residual AO dimer are dissolved in the negative BSA-SDBS cluster through electrostatic and hydrophobic forces and form a large association. Here, the fluorescence enhancement of AO-SDBS is considered to originate from the hydrophobic microenvironment provided by BSA and SDBS, the depolymerization of AO dimer and intermolecular energy transfer between BSA and AO.

摘要

实验表明,吖啶橙(AO)的荧光可被阴离子表面活性剂十二烷基苯磺酸钠(SDBS)大幅猝灭,但当向AO-SDBS体系中加入蛋白质时,后者的荧光强度增强。据认为,SDBS可促进AO二聚体的形成,导致AO荧光猝灭。当将牛血清白蛋白(BSA)加入AO-SDBS体系时,BSA与SDBS可相互作用并形成具有“芳香环堆积”的负胶束状簇合物,这破坏了AO二聚体的形成条件,使一些AO二聚体转变为单体,导致AO-SDBS体系荧光增强。而带正电的AO和残余的AO二聚体通过静电和疏水作用力溶解于带负电的BSA-SDBS簇合物中并形成大的缔合物。在此,AO-SDBS的荧光增强被认为源于BSA和SDBS提供的疏水微环境、AO二聚体的解聚以及BSA与AO之间的分子间能量转移。

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