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Quantitative Imaging of Gene Expression in Individual Bacterial Cells by Chemiluminescence

机译:化学发光定量分析单个细菌细胞中基因的表达

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Recent gene expression studies at the single bacterial cell level have primarily used green fluorescent protein (GFP) as the reporter. However, fluorescence monitoring has intrinsic limitations, such as GFP maturation time, high background, and photobleaching. To overcome those problems, we introduce the alternative approach of chemi-luminescence (CL) detection with firefly luciferase as the probe. Firefly luciferase is roughly 100 times more efficient and is faster in generating CL than bacterial luciferase but requires the introduction of luciferin, a species that is not native to bacteria. The difficulty of luciferin diffusion into the cells was solved by making use of cell membrane leakage during bacteria dehydration. In this scheme, the overall sensitivity of the system approaches the single protein molecule level. Quantitative studies of gene expression in BL21 and XLU102 bacteria can thus be performed.
机译:最近在单个细菌细胞水平上的基因表达研究主要使用绿色荧光蛋白(GFP)作为报告基因。但是,荧光监测具有固有的局限性,例如GFP成熟时间,高背景和光漂白。为了克服这些问题,我们介绍了使用萤火虫荧光素酶作为探针进行化学发光(CL)检测的另一种方法。萤火虫萤光素酶的效率比细菌萤光素酶高约100倍,并且产生CL的速度更快,但需要引入萤光素,而萤光素不是细菌固有的。通过在细菌脱水过程中利用细胞膜渗漏来解决萤光素扩散到细胞中的困难。在此方案中,系统的整体灵敏度接近单个蛋白质分子水平。因此可以对BL21和XLU102细菌中的基因表达进行定量研究。

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