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Engineering transcription factors with novel DNA-binding specificity using comparative genomics

机译:使用比较基因组学设计具有新型DNA结合特异性的转录因子

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The transcriptional program for a gene consists of the promoter necessary for recruiting RNA polymerase along with neighboring operator sites that bind different activators and repressors. From a synthetic biology perspective, if the DNA-binding specificity of these proteins can be changed, then they can be used to reprogram gene expression in cells. While many experimental methods exist for generating such specificity-altering mutations, few computational approaches are available, particularly in the case of bacterial transcription factors. In a previously published computational study of nitrogen oxide metabolism in bacteria, a small number of amino-acid residues were found to determine the specificity within the CRP (cAMP receptor protein)/FNR (fumarate and nitrate reductase regulatory protein) family of transcription factors. By analyzing how these amino acids vary in different regulators, a simple relationship between the identity of these residues and their target DNA-binding sequence was constructed. In this article, we experimentally tested whether this relationship could be used to engineer novel DNA-protein interactions. Using Escherichia coli CRP as a template, we tested eight designs based on this relationship and found that four worked as predicted. Collectively, these results in this work demonstrate that comparative genomics can inform the design of bacterial transcription factors.
机译:基因的转录程序由募集RNA聚合酶所需的启动子以及结合不同激活子和阻遏子的邻近操纵子位点组成。从合成生物学的角度来看,如果可以改变这些蛋白质的DNA结合特异性,则可以将它们用于重新编程细胞中的基因表达。尽管存在许多产生这种改变特异性的实验方法,但是很少有计算方法可用,特别是在细菌转录因子的情况下。在先前发表的细菌中氮氧化物代谢的计算研究中,发现少量氨基酸残基决定了转录因子CRP(cAMP受体蛋白)/ FNR(富马酸酯和硝酸还原酶调节蛋白)家族的特异性。通过分析这些氨基酸在不同调节剂中的变化方式,构建了这些残基的身份与其靶标DNA结合序列之间的简单关系。在本文中,我们通过实验测试了这种关系是否可用于工程化新型DNA-蛋白质相互作用。使用大肠杆菌CRP作为模板,我们基于这种关系测试了8个设计,发现其中4个按预期工作。总的来说,这项工作中的这些结果表明,比较基因组学可以指导细菌转录因子的设计。

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