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首页> 外文期刊>Electronic Journal of Biotechnology >Engineering Escherichia coli for autoinducible production of n-butanol
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Engineering Escherichia coli for autoinducible production of n-butanol

机译:工程性大肠杆菌,用于自动诱导生产正丁醇

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Background: Escherichia coli does not produce n-butanol naturally, but can be butanologenic when related enzymes were expressed using inducible elements on plasmids. In this study we attempted to confer E. coli strain capability of automatic excretion of the chemical by employing a native anaerobic promoter. Also, a novel DNA kit was designed for PCR preparation of linear DNA fragments to perform strain modification. The kit is primarily composed of two mother vectors, co-transformation of linear DNAs into E. coli can simultaneously introduce two butanol synthetic operons into the chromosome and create two in-frame gene deletions at targeted native loci. Results: E. coli strain Bw2V carries plasmid pCNA-PHC and pENA-TA, both utilizes native anaerobic promoter Phya for the expression of butanol synthetic enzymes. When Bw2V was subjected in anaerobic fermentation using medium containing extra glucose, the accumulated n-butanol in the broth was up to 2.8?g/L in bioreactor; as the genetic element expressing the same pathway was introduced into the genome, the titer of butanol was 1.4?g/L. Conclusions: The expression system using Phya is effective in applications that involve expression plasmids as also applicable in ectopic expression as single copy on the chromosome. Results imply that Phya can be subjected for broader application in bioproduction of more feedstock chemicals.
机译:背景:大肠杆菌不会自然产生正丁醇,但是当使用质粒上的可诱导元件表达相关酶时,可能会产生丁醇。在这项研究中,我们尝试通过使用天然厌氧启动子赋予大肠杆菌菌株化学物质自动排泄的能力。同样,设计了一种新颖的DNA试剂盒,用于PCR制备线性DNA片段以进行菌株修饰。该试剂盒主要由两个母载体组成,线性DNA共同转化为大肠杆菌可同时将两个丁醇合成操纵子引入染色体,并在目标天然基因座处产生两个框内基因缺失。结果:大肠杆菌菌株Bw2V携带质粒pCNA-PHC和pENA-TA,两者均利用天然厌氧启动子Phya来表达丁醇合成酶。当使用含过量葡萄糖的培养基对Bw2V进行厌氧发酵时,在生物反应器中肉汤中积累的正丁醇高达2.8?g / L。当将表达相同途径的遗传元件引入基因组时,丁醇的效价为1.4?g / L。结论:使用Phya的表达系统在涉及表达质粒的应用中是有效的,该应用也可作为染色体上的单拷贝应用于异位表达。结果表明,Phya可以在更多原料化学物质的生物生产中得到更广泛的应用。

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