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Detection of green fluorescent protein in a single bacterium by capillary electrophoresis with laser-induced fluorescence

机译:激光诱导荧光的毛细管电泳检测单个细菌中的绿色荧光蛋白

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Green fluorescence protein (GFP) is a common reporter used to monitor protein expression in single cells. However, autofluorescence from endogenous components can mask the signal from GFP, particularly at low expression levels in prokaryotes. We employ capillary electrophoresis with laser-induced fluorescence for the analysis of the expression of green fluorescent protein in a single bacterium. Capillary electrophoresis separates GFP from native cellular autofluorescent components, reducing the background signal and improving detection limits. Our system provides 100 ymol (60 copies) limits of detection for GFP. To demonstrate the performance of this instrument, we employ a model system of Deinococcus radiodurans that has been engineered to express GFP under the control of the recA promoter. We report resolution and detection of GFP and autofluorescent components in a single D. radiodurans bacterium. This paper presents the first example of expression of GFP in D. radiodurans and the first detection of GFP in a single bacterium by capillary electrophoresis.
机译:绿色荧光蛋白(GFP)是用于监测单个细胞中蛋白表达的常见报告基因。但是,内源性成分的自发荧光可以掩盖来自GFP的信号,特别是在原核生物中的低表达水平下。我们采用毛细管电泳和激光诱导的荧光来分析单个细菌中绿色荧光蛋白的表达。毛细管电泳将GFP与天然细胞自身荧光成分分开,从而减少了背景信号并提高了检测限。我们的系统为GFP提供100 ymol(60拷贝)的检测限。为了证明该仪器的性能,我们采用了放射杜鹃球菌的模型系统,该模型系统经过工程设计以在recA启动子的控制下表达GFP。我们报告在一个单一的D. radiodurans细菌中的分辨率和GFP和自发荧光成分的检测。本文介绍了第一个示例在GFP中的表达,并通过毛细管电泳在单个细菌中首次检测到了GFP。

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