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Green fluorescent protein is superior to blue fluorescent protein as a quantitative reporter of promoter activity in E. coli

机译:作为大肠杆菌中启动子活性的定量报告物,绿色荧光蛋白优于蓝色荧光蛋白

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摘要

Fluorescent proteins related to and derived from green fluorescent protein (GFP) are widely used as tools for investigating a wide range of biological processes. In particular, GFP and its relatives have been used extensively as qualitative reporters of gene expression in many different organisms, but relatively few studies have investigated fluorescent proteins as quantitative reporters of gene expression. GFP has some limitations as a reporter gene, including possible toxicity when expressed at high levels. Therefore, it would be useful if other fluorescent proteins could be identified for use as quantitative reporters. Toward this end, we investigated BFP as a quantitative reporter of promoter activity in E. coli and directly compared it with GFPuv using a set of well-characterized synthetic constitutive promoters. The fluorescence produced in E. coli strains expressing GFPuv or BFP grown on solid medium was quantified using a CCD camera and fluorimetry. GFPuv consistently gave more reliable and statistically significant results than did BFP in all assays. Correspondingly, we found that the signal-to-noise ratio for GFPuv fluorescence is substantially higher than for BFP. We conclude that, under the conditions assessed in this study, GFPuv is superior to BFP as a quantitative reporter of promoter activity in E. coli.
机译:与绿色荧光蛋白(GFP)相关并衍生自绿色荧光蛋白(GFP)的荧光蛋白被广泛用作研究各种生物学过程的工具。特别是,GFP及其近亲已被广泛用作许多不同生物体中基因表达的定性报告基因,但相对较少的研究已经研究了荧光蛋白作为基因表达的定量报告基因。 GFP作为报告基因有一些局限性,包括高水平表达时可能产生的毒性。因此,如果可以鉴定其他荧光蛋白用作定量报告基因,将是有用的。为此,我们调查了BFP作为大肠杆菌中启动子活性的定量报告者,并使用一组功能齐全的合成组成型启动子直接将其与GFPuv进行比较。使用CCD相机和荧光法定量在固体培养基上生长的表达GFPuv或BFP的大肠杆菌菌株中产生的荧光。在所有分析中,GFPuv始终提供比BFP更可靠和统计学上显着的结果。相应地,我们发现GFPuv荧光的信噪比明显高于BFP。我们得出的结论是,在本研究评估的条件下,GFPuv作为大肠杆菌中启动子活性的定量报告者优于BFP。

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