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利用荧光共振能量转移对配体-受体相互作用进行实时监测。

Real-time monitoring of ligand-receptor interactions with fluorescence resonance energy transfer.

作者信息

Dogra Navneet, Reyes Julia C, Garg Nishi, Kohli Punit

机构信息

Department of Chemistry and Biochemistry, Southern Illinois University, USA.

出版信息

J Vis Exp. 2012 Aug 20(66):e3805. doi: 10.3791/3805.

Abstract

FRET is a process whereby energy is non-radiatively transferred from an excited donor molecule to a ground-state acceptor molecule through long-range dipole-dipole interactions. In the present sensing assay, we utilize an interesting property of PDA: blue-shift in the UV-Vis electronic absorption spectrum of PDA (Figure 1) after an analyte interacts with receptors attached to PDA. This shift in the PDA absorption spectrum provides changes in the spectral overlap (J) between PDA (acceptor) and rhodamine (donor) that leads to changes in the FRET efficiency. Thus, the interactions between analyte (ligand) and receptors are detected through FRET between donor fluorophores and PDA. In particular, we show the sensing of a model protein molecule streptavidin. We also demonstrate the covalent-binding of bovine serum albumin (BSA) to the liposome surface with FRET mechanism. These interactions between the bilayer liposomes and protein molecules can be sensed in real-time. The proposed method is a general method for sensing small chemical and large biochemical molecules. Since fluorescence is intrinsically more sensitive than colorimetry, the detection limit of the assay can be in sub-nanomolar range or lower. Further, PDA can act as a universal acceptor in FRET, which means that multiple sensors can be developed with PDA (acceptor) functionalized with donors and different receptors attached on the surface of PDA liposomes.

摘要

荧光共振能量转移(FRET)是一种能量通过长程偶极-偶极相互作用从激发态供体分子非辐射转移到基态受体分子的过程。在本传感分析中,我们利用了聚多巴胺(PDA)的一个有趣特性:当分析物与附着在PDA上的受体相互作用后,PDA的紫外-可见电子吸收光谱发生蓝移(图1)。PDA吸收光谱的这种变化导致了PDA(受体)与罗丹明(供体)之间光谱重叠(J)的改变,进而导致FRET效率的变化。因此,通过供体荧光团与PDA之间的FRET来检测分析物(配体)与受体之间的相互作用。特别地,我们展示了对模型蛋白分子链霉亲和素的传感。我们还通过FRET机制证明了牛血清白蛋白(BSA)与脂质体表面的共价结合。双层脂质体与蛋白质分子之间的这些相互作用可以实时检测。所提出的方法是一种用于传感小分子化学物质和大分子生物化学物质的通用方法。由于荧光本质上比比色法更灵敏,该分析方法的检测限可以在亚纳摩尔范围或更低。此外,PDA可以在FRET中充当通用受体,这意味着可以用供体功能化的PDA(受体)以及附着在PDA脂质体表面的不同受体开发多种传感器。

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