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Butyrate Production in Engineered Escherichia coli With Synthetic Scaffolds

机译:人工合成工程支架在丁酸生产中的应用

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Butyrate pathway was constructed in recombinant Escherichia coli using the genes from Clostridium acetobutylicum and Treponema denticola. However, the pathway constructed from exogenous enzymes did not efficiently convert carbon flux to butyrate. Three steps of the productivity enhancement were attempted in this study. First, pathway engineering to delete metabolic pathways to by-products successfully improved the butyrate production. Second, synthetic scaffold protein that spatially co-localizes enzymes was introduced to improve the efficiency of the heterologous pathway enzymes, resulting in threefold improvement in butyrate production. Finally, further optimizations of inducer concentrations and pH adjustment were tried. The final titer of butyrate was 4.3 and 7.2 g/L under batch and fed-batch cultivation, respectively. This study demonstrated the importance of synthetic scaffold protein as a useful tool for optimization of heterologous butyrate pathway in E. coli. Biotechnol. Bioeng. 2013;110: 2790–2794.
机译:利用丙酮丁醇梭菌和密螺旋体的基因在重组大肠杆菌中构建丁酸途径。但是,由外源酶构建的途径不能有效地将碳通量转化为丁酸。在这项研究中尝试了提高生产率的三个步骤。首先,消除副产物代谢途径的途径工程成功地提高了丁酸盐的产量。其次,引入了在空间上共定位酶的合成支架蛋白,以提高异源途径酶的效率,从而使丁酸酯产量提高了三倍。最后,尝试了进一步优化诱导剂浓度和调节pH。在分批和补料分批培养下,丁酸的最终滴度分别为4.3 g / L和7.2 g / L。这项研究证明了合成支架蛋白作为优化大肠杆菌异源丁酸途径的有用工具的重要性。生物技术。生恩2013; 110:2790-2794。

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