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理解并利用大肠杆菌中甘油的微需氧代谢。

Understanding and harnessing the microaerobic metabolism of glycerol in Escherichia coli.

作者信息

Durnin Guyton, Clomburg James, Yeates Zeno, Alvarez Pedro J J, Zygourakis Kyriacos, Campbell Paul, Gonzalez Ramon

机构信息

Department of Chemical and Biomolecular Engineering, Rice University, 6100 Main Street, MS-362, P.O. Box 1892, Houston, Texas 77251-1892, USA.

出版信息

Biotechnol Bioeng. 2009 May 1;103(1):148-61. doi: 10.1002/bit.22246.

Abstract

Given its availability, low prices, and high degree of reduction, glycerol has become an ideal feedstock for the production of reduced compounds. The anaerobic fermentation of glycerol by Escherichia coli could be an excellent platform for this purpose but it requires expensive nutrients such as tryptone and yeast extract. In this work, microaerobic conditions were used as a means of eliminating the need for rich nutrients. Availability of low amounts of oxygen enabled redox balance while preserving the ability to synthesize reduced products. A fermentation balance analysis showed approximately 95% recovery of carbon and reducing equivalents. The pathways involved in glycerol dissimilation were identified using different genetic and biochemical approaches. Respiratory (GlpK-GlpD/GlpABC) and fermentative (GldA-DhaKLM) routes mediated the conversion of glycerol to glycolytic intermediates. Although pyruvate formate-lyase (PFL) and pyruvate dehydrogenase contributed to the synthesis of acetyl-CoA from pyruvate, most of the carbon flux proceeded through PFL. The pathways mediating the synthesis of acetate and ethanol were required for the efficient utilization of glycerol. The microaerobic metabolism of glycerol was harnessed by engineering strains for the co-production of ethanol and hydrogen (EH05 [pZSKLMgldA]), and ethanol and formate (EF06 [pZSKLMgldA]). High ethanol yields were achieved by genetic manipulations that reduced the synthesis of by-products succinate, acetate, and lactate. Co-production of hydrogen required the use of acidic pH while formate co-production was facilitated by inactivation of the enzyme formate-hydrogen lyase. High rates of product synthesis were realized by overexpressing glycerol dehydrogenase (GldA) and dihydroxyacetone kinase (DhaKLM). Engineered strains efficiently produced ethanol and hydrogen and ethanol and formate from glycerol in a minimal medium without rich supplements.

摘要

鉴于甘油的可得性、低价格以及高还原度,它已成为生产还原化合物的理想原料。大肠杆菌对甘油的厌氧发酵可能是实现这一目的的绝佳平台,但这需要昂贵的营养物质,如胰蛋白胨和酵母提取物。在这项研究中,微需氧条件被用作消除对丰富营养物质需求的一种手段。少量氧气的存在实现了氧化还原平衡,同时保留了合成还原产物的能力。发酵平衡分析表明,碳和还原当量的回收率约为95%。使用不同的遗传和生化方法确定了甘油异化过程中涉及的途径。呼吸途径(GlpK-GlpD/GlpABC)和发酵途径(GldA-DhaKLM)介导了甘油向糖酵解中间产物的转化。尽管丙酮酸甲酸裂解酶(PFL)和丙酮酸脱氢酶有助于丙酮酸合成乙酰辅酶A,但大部分碳通量是通过PFL进行的。介导乙酸和乙醇合成的途径是甘油高效利用所必需的。通过构建工程菌株来利用甘油的微需氧代谢,实现乙醇和氢气的联产(EH05 [pZSKLMgldA])以及乙醇和甲酸的联产(EF06 [pZSKLMgldA])。通过减少副产物琥珀酸、乙酸和乳酸的合成的基因操作实现了高乙醇产量。联产氢气需要使用酸性pH,而甲酸联产则通过使甲酸氢裂解酶失活来促进。通过过量表达甘油脱氢酶(GldA)和二羟基丙酮激酶(DhaKLM)实现了高产物合成速率。工程菌株能够在不添加丰富营养成分的基本培养基中,从甘油高效生产乙醇和氢气以及乙醇和甲酸。

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