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A cost-effective polyphosphate-based metabolism fuels an all E. coli cell-free expression system

机译:具有成本效益的基于多磷酸盐的新陈代谢为整个大肠杆菌无细胞表达系统提供了燃料

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摘要

A new cost-effective metabolism providing an ATP-regeneration system for cell-free protein synthesis is presented. Hexametaphosphate, a polyphosphate molecule, is used as phosphate donor together with maltodextrin, a polysaccharide used as carbon source to stimulate glycolysis. Remarkably, addition of enzymes is not required for this metabolism, which is carried out by endogenous catalysts present in the Escherichia coli crude extract. This new ATP regeneration system allows efficient recycling of inorganic phosphate, a strong inhibitor of protein synthesis. We show that up to 1.34-1.65 mg/mL of active reporter protein is synthesized in batch-mode reaction after 5 h of incubation. Unlike typical hybrid in vitro protein synthesis systems based on bacteriophage transcription, expression is carried out through E. colt promoters using only the endogenous transcription-translation molecular machineries provided by the extract. We demonstrate that traditional expensive energy regeneration systems, such as creatine phosphate, phosphoenolpyruvate or phosphoglycerate, can be replaced by a cost-effective metabolic scheme suitable for cell-free protein synthesis applications. Our work also shows that cell-free systems are useful platforms for metabolic engineering. (C) 2014 International Metabolic Engineering Society. Published by Elsevier Inc. All rights reserved.
机译:提出了一种新的具有成本效益的新陈代谢方法,为无细胞蛋白质合成提供了ATP再生系统。六磷酸六磷酸酯(一种多磷酸盐分子)与麦芽糊精(一种用作碳源以刺激糖酵解的多糖)一起用作磷酸盐供体。显着地,该代谢不需要添加酶,这是通过存在于大肠杆菌粗提物中的内源性催化剂来进行的。这种新的ATP再生系统可有效回收无机磷酸盐(一种强力的蛋白质合成抑制剂)。我们显示,孵育5小时后,以批处理模式反应可合成高达1.34-1.65 mg / mL的活性报道蛋白。与典型的基于噬菌体转录的杂交体外蛋白质合成系统不同,仅通过提取物提供的内源转录-翻译分子机制通过大肠杆菌启动子进行表达。我们证明了传统的昂贵的能量再生系统,例如磷酸肌酸,磷酸烯醇丙酮酸或磷酸甘油酸,可以被适合无细胞蛋白质合成应用的具有成本效益的代谢方案所取代。我们的工作还表明,无细胞系统是代谢工程的有用平台。 (C)2014年国际代谢工程学会。由Elsevier Inc.出版。保留所有权利。

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