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利用Förster共振能量转移对量子点进行毛细管内探测以及荧光蛋白的自组装和置换。

In-capillary probing of quantum dots and fluorescent protein self-assembly and displacement using Förster resonance energy transfer.

作者信息

Wang Jianhao, Fan Jie, Li Jinchen, Liu Li, Wang Jianpeng, Jiang Pengju, Liu Xiaoqian, Qiu Lin

机构信息

School of Pharmaceutical Engineering and Life Science, Changzhou University, Changzhou, Jiangsu, People's Republic of China.

Key Laboratory of Synthetic Biology, Shanghai Institutes for Biological Sciences, Chinese Academy of Sciences, Shanghai, People's Republic of China.

出版信息

J Sep Sci. 2017 Feb;40(4):933-939. doi: 10.1002/jssc.201600937. Epub 2016 Dec 30.

DOI:10.1002/jssc.201600937
PMID:27935249
Abstract

Herein, a Förster resonance energy transfer system was designed, which consisted of CdSe/ZnS quantum dots donor and mCherry fluorescent protein acceptor. The quantum dots and the mCherry proteins were conjugated to permit Förster resonance energy transfer. Capillary electrophoresis with fluorescence detection was used for the analyses for the described system. The quantum dots and mCherry were sequentially injected into the capillary, while the real-time fluorescence signal of donor and acceptor was simultaneously monitored by two channels with fixed wavelength detectors. An effective separation of complexes from free donor and acceptor was achieved. Results showed quantum dots and hexahistidine tagged mCherry had high affinity and the assembly was affected by His -mCherry/quantum dot molar ratio. The kinetics of the self-assembly was calculated using the Hill equation. The microscopic dissociation constant values for out of- and in-capillary assays were 10.49 and 23.39 μM, respectively. The capillary electrophoresis with fluorescence detection that monitored ligands competition assay further delineated the different binding capacities of histidine containing peptide ligands for binding sites on quantum dots. This work demonstrated a novel approach for the improvement of Förster resonance energy transfer for higher efficiency, increased sensitivity, intuitionistic observation, and low sample requirements of the in-capillary probing system.

摘要

在此,设计了一种福斯特共振能量转移系统,其由CdSe/ZnS量子点供体和mCherry荧光蛋白受体组成。量子点和mCherry蛋白进行了共轭以实现福斯特共振能量转移。采用带荧光检测的毛细管电泳对所述系统进行分析。将量子点和mCherry依次注入毛细管中,同时通过两个具有固定波长检测器的通道同步监测供体和受体的实时荧光信号。实现了复合物与游离供体和受体的有效分离。结果表明量子点和六聚组氨酸标记的mCherry具有高亲和力,且组装受His-mCherry/量子点摩尔比的影响。使用希尔方程计算自组装的动力学。毛细管外和毛细管内测定的微观解离常数分别为10.49和23.39 μM。监测配体竞争试验的带荧光检测的毛细管电泳进一步描绘了含组氨酸的肽配体对量子点上结合位点的不同结合能力。这项工作展示了一种新颖的方法,用于改进福斯特共振能量转移,以实现更高的效率、更高的灵敏度、直观的观察以及毛细管内探测系统对样品的低要求。

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