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通过Red/ET重组构建启动子文库的大肠杆菌菌株为转录微调铺平了道路。

Escherichia coli strains with promoter libraries constructed by Red/ET recombination pave the way for transcriptional fine-tuning.

作者信息

Braatsch Stephan, Helmark Søren, Kranz Harald, Koebmann Brian, Jensen Peter Ruhdal

机构信息

Gene Bridges GmbH, Commercial Centre, Im Neuenheimer Feld 584, Heidelberg, Germany.

出版信息

Biotechniques. 2008 Sep;45(3):335-7. doi: 10.2144/000112907.

Abstract

System-oriented applications of genetic engineering, such as metabolic engineering, often require the serial optimization of enzymatic reaction steps, which can be achieved by transcriptional fine-tuning. However, approaches to changing gene expression are usually limited to deletion and/or strong overexpression and rarely match the desired optimal transcript levels. A solution to this all-or-nothing approach has been the use of a synthetic promoter library (SPL) that is based on randomized sequences flanking the consensus -10 and -35 promoter regions and allows for fine-tuning of bacterial gene expression. Red/ET recombination perfectly complements SPL technology, since it enables easy modification of the Escherichia coli genome and can be accomplished with linear DNA (i.e., the SPL). To demonstrate the synergistic use of Red/ET and SPL for metabolic engineering applications, we replaced the native promoter of a genomic localized phosphoglucose isomerase (pgi)-lacZ reporter construct by an SPL. Using these technologies together, we were able to rapidly identify synthetic promoter sequences that resulted in activity range of 25% to 570% of the native pgi-promoter.

摘要

基因工程的面向系统的应用,如代谢工程,通常需要对酶促反应步骤进行系列优化,这可通过转录微调来实现。然而,改变基因表达的方法通常局限于缺失和/或强过表达,很少能达到所需的最佳转录水平。解决这种非此即彼方法的一个办法是使用基于共有-10和-35启动子区域侧翼随机序列的合成启动子文库(SPL),它能对细菌基因表达进行微调。Red/ET重组与SPL技术完美互补,因为它能轻松修饰大肠杆菌基因组,并且可以用线性DNA(即SPL)来完成。为了证明Red/ET和SPL在代谢工程应用中的协同使用,我们用一个SPL替换了基因组定位的磷酸葡萄糖异构酶(pgi)-lacZ报告构建体的天然启动子。将这些技术结合使用,我们能够快速鉴定出导致活性范围为天然pgi启动子活性的25%至570%的合成启动子序列。

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