Kim Seong Keun, Lee Dae-Hee, Kim Oh Cheol, Kim Jihyun F, Yoon Sung Ho
Synthetic Biology and Bioengineering Research Center, Korea Research Institute of Bioscience and Biotechnology (KRIBB) , Daejeon 34141, Republic of Korea.
Biosystems and Bioengineering Program, University of Science and Technology (UST) , Daejeon 34113, Republic of Korea.
ACS Synth Biol. 2017 Sep 15;6(9):1766-1773. doi: 10.1021/acssynbio.7b00102. Epub 2017 May 31.
Most inducible expression systems suffer from growth defects, leaky basal induction, and inhomogeneous expression levels within a host cell population. These difficulties are most prominent with the overproduction of membrane proteins that are toxic to host cells. Here, we developed an Escherichia coli inducible expression system for membrane protein production based on titrated expression of a mutant lac repressor (mLacI). Performance of the mLacI inducible system was evaluated in conjunction with commonly used lac operator-based expression vectors using a T7 or tac promoter. Remarkably, expression of a target gene can be titrated by the dose-dependent addition of l-rhamnose, and the expression levels were homogeneous in the cell population. The developed system was successfully applied to overexpress three membrane proteins that were otherwise difficult to produce in E. coli. This gene expression control system can be easily applied to a broad range of existing protein expression systems and should be useful in constructing genetic circuits that require precise output signals.
大多数诱导型表达系统存在生长缺陷、基础诱导渗漏以及宿主细胞群体内表达水平不均一的问题。这些困难在对宿主细胞有毒性的膜蛋白过量表达时最为突出。在此,我们基于突变型乳糖阻遏蛋白(mLacI)的滴定表达,开发了一种用于大肠杆菌中膜蛋白生产的诱导型表达系统。使用T7或tac启动子,结合常用的基于乳糖操纵子的表达载体,对mLacI诱导系统的性能进行了评估。值得注意的是,通过剂量依赖性添加L-鼠李糖可以滴定目标基因的表达,并且细胞群体中的表达水平是均一的。所开发的系统成功应用于三种原本难以在大肠杆菌中生产的膜蛋白的过表达。这种基因表达控制系统可以很容易地应用于广泛的现有蛋白质表达系统,并且在构建需要精确输出信号的遗传回路中应该会很有用。
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