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Calibrating Transcriptional Activity Using Constitutive Synthetic Promoters in Mutants for Global Regulators in Escherichia coli

机译:使用突变体中的本构合成启动子校准大肠埃希菌的转录活性。

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The engineering of synthetic circuits in cells relies on the use of well-characterized biological parts that would perform predicted functions under the situation considered, and many efforts have been taken to set biological standards that could define the basic features of these parts. However, since most synthetic biology projects usually require a particular cellular chassis and set of growth conditions, defining standards in the field is not a simple task as gene expression measurements could be affected severely by genetic background and culture conditions. In this study, we addressed promoter parameterization in bacteria in different genetic backgrounds and growth conditions. We found that a small set of constitutive promoters of different strengths controlling a short-lived GFP reporter placed in a low-copy number plasmid produces remarkably reproducible results that allow for the calibration of promoter activity over different genetic backgrounds and physiological conditions, thus providing a simple way to set standards of promoter activity in bacteria. Based on these results, we proposed the utilization of synthetic constitutive promoters as tools for calibration for the standardization of biological parts, in a way similar to the use of DNA and protein ladders in molecular biology as references for comparison with samples of interest.
机译:细胞中合成电路的工程设计依赖于充分使用的生物学部件的使用,这些生物学部件将在所考虑的情况下执行预测的功能,并且已经进行了许多努力来设置可以定义这些部件的基本特征的生物学标准。但是,由于大多数合成生物学项目通常都需要特定的细胞结构和生长条件,因此在现场确定标准并非易事,因为基因表达测量可能会受到遗传背景和培养条件的严重影响。在这项研究中,我们研究了不同遗传背景和生长条件下细菌中启动子的参数化。我们发现,控制短寿命GFP报道分子的一小部分不同强度的组成型启动子被放置在低拷贝数质粒中,产生了可重现的结果,可在不同的遗传背景和生理条件下对启动子活性进行校准,从而提供了一个设定细菌中启动子活性标准的简单方法。基于这些结果,我们提出了利用合成组成型启动子作为校准生物部分标准化的工具,其方式类似于在分子生物学中使用DNA和蛋白质阶梯作为与感兴趣样品进行比较的参考。

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