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工程改造大肠杆菌以实现甘油向乙醇及副产物的高效转化。

Engineering Escherichia coli for the efficient conversion of glycerol to ethanol and co-products.

作者信息

Shams Yazdani Syed, Gonzalez Ramon

机构信息

Department of Chemical and Biomolecular Engineering, Rice University, Houston, TX, USA.

出版信息

Metab Eng. 2008 Nov;10(6):340-51. doi: 10.1016/j.ymben.2008.08.005. Epub 2008 Sep 9.

Abstract

Given its availability, low prices, and high degree of reduction, glycerol has become an ideal feedstock for producing reduced compounds via anaerobic fermentation. We recently identified environmental conditions enabling the fermentative metabolism of glycerol in E. coli, along with the pathways and mechanisms mediating this metabolic process. In this work, we used the knowledge base created in previous studies to engineer E. coli for the efficient conversion of crude glycerol to ethanol. Our strategy capitalized on the high degree of reduction of carbon in glycerol, thus enabling the production of not only ethanol but also co-products hydrogen and formate. Two strains were created for the co-production of ethanol-hydrogen and ethanol-formate: SY03 and SY04, respectively. High ethanol yields were achieved in both strains by minimizing the synthesis of by-products succinate and acetate through mutations that inactivated fumarate reductase (DeltafrdA) and phosphate acetyltransferase (Deltapta), respectively. Strain SY04, which produced ethanol-formate, also contained a mutation that inactivated formate-hydrogen lyase (DeltafdhF), thus preventing the conversion of formate to CO(2) and H(2). High rates of glycerol utilization and product synthesis were achieved by simultaneous overexpression of glycerol dehydrogenase (gldA) and dihydroxyacetone kinase (dhaKLM), which are the enzymes responsible for the conversion of glycerol to glycolytic intermediate dihydroxyacetone phosphate. The resulting strains, SY03 (pZSKLMgldA) and SY04 (pZSKLMgldA), produced ethanol-hydrogen and ethanol-formate from unrefined glycerol at yields exceeding 95% of the theoretical maximum and specific rates in the order of 15-30 mmol/gcell/h. These yields and productivities are superior to those reported for the conversion of glycerol to ethanol-H(2) or ethanol-formate by other organisms and equivalent to those achieved in the production of ethanol from sugars using E. coli.

摘要

鉴于甘油的可得性、低价格以及高还原度,它已成为通过厌氧发酵生产还原型化合物的理想原料。我们最近确定了能使大肠杆菌进行甘油发酵代谢的环境条件,以及介导这一代谢过程的途径和机制。在这项工作中,我们利用先前研究建立的知识库对大肠杆菌进行工程改造,以实现将粗甘油高效转化为乙醇。我们的策略利用了甘油中碳的高还原度,从而不仅能够生产乙醇,还能生产副产物氢气和甲酸盐。构建了两株分别用于联产乙醇 - 氢气和乙醇 - 甲酸盐的菌株:SY03和SY04。通过分别使延胡索酸还原酶(DeltafrdA)和磷酸乙酰转移酶(Deltapta)失活的突变来最小化副产物琥珀酸和乙酸的合成,在这两株菌株中均实现了高乙醇产量。产生乙醇 - 甲酸盐的菌株SY04还含有使甲酸氢裂解酶(DeltafdhF)失活的突变,从而防止甲酸盐转化为CO₂和H₂。通过同时过表达甘油脱氢酶(gldA)和二羟基丙酮激酶(dhaKLM)实现了高甘油利用率和产物合成速率,这两种酶负责将甘油转化为糖酵解中间产物磷酸二羟基丙酮。所得菌株SY03(pZSKLMgldA)和SY04(pZSKLMgldA)从未精炼甘油中生产乙醇 - 氢气和乙醇 - 甲酸盐的产量超过理论最大值的95%,比生产率约为15 - 30 mmol/g细胞/小时。这些产量和生产率优于其他生物体将甘油转化为乙醇 - H₂或乙醇 - 甲酸盐的报道,并且与使用大肠杆菌从糖生产乙醇所达到的产量和生产率相当。

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