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从水母发光蛋白到荧光团的生物发光共振能量转移:一种用于多分析物检测的人工水母。

Bioluminescence resonance energy transfer from aequorin to a fluorophore: an artificial jellyfish for applications in multianalyte detection.

作者信息

Deo Sapna K, Mirasoli Mara, Daunert Sylvia

机构信息

Department of Chemistry, University of Kentucky, Lexington, KY 40506-0055, USA.

出版信息

Anal Bioanal Chem. 2005 Apr;381(7):1387-94. doi: 10.1007/s00216-005-3081-z. Epub 2005 Feb 25.

Abstract

In nature, the green light emission observed in the jellyfish Aequorea victoria is a result of a non-radiative energy transfer from the excited-state aequorin to the green fluorescent protein. In this work, we have modified the photoprotein aequorin by attaching selected fluorophores at a unique site on the protein. This will allow for in vitro transfer of bioluminescent energy from aequorin to the fluorophore thus creating an "artificial jellyfish". The fluorophores are selected such that the excitation spectrum of the fluorophore overlaps with the emission spectrum of aequorin. By modifying aequorin with different fluorophores, bioluminescent labels with different emission maxima are produced, which will allow for the simultaneous detection of multiple analytes. By examining the X-ray crystal structure of the protein, four different sites for introduction of the unique cysteine residue were evaluated. Two fluorophores with differing emission maxima were attached individually to the mutants through the sulfhydryl group of the cysteine molecule. Two of the fluorophore-labeled mutants showed a peak corresponding to fluorophore emission thus indicating resonance energy transfer from aequorin to the fluorophore.

摘要

在自然界中,在维多利亚多管发光水母中观察到的绿色光发射是激发态水母发光蛋白向绿色荧光蛋白进行非辐射能量转移的结果。在这项工作中,我们通过在蛋白上的一个独特位点连接选定的荧光团对光蛋白水母发光蛋白进行了修饰。这将使得生物发光能量在体外从水母发光蛋白转移到荧光团,从而创造出一种“人工水母”。所选择的荧光团的激发光谱与水母发光蛋白的发射光谱重叠。通过用不同的荧光团修饰水母发光蛋白,产生了具有不同发射最大值的生物发光标记物,这将允许同时检测多种分析物。通过研究该蛋白的X射线晶体结构,评估了引入独特半胱氨酸残基的四个不同位点。两种具有不同发射最大值的荧光团通过半胱氨酸分子的巯基分别连接到突变体上。两种荧光团标记的突变体显示出与荧光团发射相对应的峰,从而表明从水母发光蛋白到荧光团的共振能量转移。

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