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用于在单细胞水平上对细菌细胞内氧化还原状态进行监测的基于荧光蛋白的荧光共振能量转移传感器。

Fluorescent protein-based FRET sensor for intracellular monitoring of redox status in bacteria at single cell level.

作者信息

Abraham Bobin George, Santala Ville, Tkachenko Nikolai V, Karp Matti

机构信息

Department of Chemistry and Bioengineering, Tampere University of Technology, P.O. Box 541, 33101, Tampere, Finland,

出版信息

Anal Bioanal Chem. 2014 Nov;406(28):7195-204. doi: 10.1007/s00216-014-8165-1. Epub 2014 Sep 16.

Abstract

Monitoring of intracellular redox status in a bacterial cell provides vital information about the physiological status of the cell, which can be exploited in several applications such as metabolic engineering and computational modeling. Fluorescent protein-based genetically encoded sensors can be used to monitor intracellular oxidation/reduction status. This study reports the development of a redox sensor for intracellular measurements using fluorescent protein pairs and the phenomenon of Förster resonance energy transfer (FRET). For the development of the sensor, fluorescent proteins Citrine and Cerulean were genetically modified to carry reactive cysteine residues on the protein surface close to the chromophore and a constructed FRET pair was fused using a biotinylation domain as a linker. In oxidized state, the FRET pairs are in close proximity by labile disulfide bond formation resulting in higher FRET efficiency. In reducing environment, the FRET is diminished due to the increased distance between FRET pairs providing large dynamic measurement range to the sensor. Intracellular studies in Escherichia coli mutants revealed the capability of the sensor in detecting real-time redox variations at single cell level. The results were validated by intensity based and time resolved measurements. The functional immobilization of the fluorescent protein-based FRET sensor at solid surfaces for in vitro applications was also demonstrated.

摘要

监测细菌细胞内的氧化还原状态可提供有关细胞生理状态的重要信息,这些信息可用于代谢工程和计算建模等多种应用。基于荧光蛋白的基因编码传感器可用于监测细胞内的氧化/还原状态。本研究报告了一种利用荧光蛋白对和Förster共振能量转移(FRET)现象进行细胞内测量的氧化还原传感器的开发。为了开发该传感器,对荧光蛋白柠檬黄和天蓝色进行了基因改造,使其在靠近发色团的蛋白质表面携带反应性半胱氨酸残基,并使用生物素化结构域作为连接子构建了一个FRET对。在氧化状态下,FRET对通过不稳定的二硫键形成紧密靠近,导致更高的FRET效率。在还原环境中,由于FRET对之间距离增加,FRET减弱,为传感器提供了较大动态测量范围。在大肠杆菌突变体中的细胞内研究揭示了该传感器在单细胞水平检测实时氧化还原变化的能力。结果通过基于强度和时间分辨测量得到验证。还展示了基于荧光蛋白的FRET传感器在固体表面的功能固定化用于体外应用。

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