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在大肠杆菌突变菌株的中心需氧代谢途径中代谢通量的重新分布,这些菌株缺失了用于合成乙酸异戊酯的ackA-pta和poxB途径。

Redistribution of metabolic fluxes in the central aerobic metabolic pathway of E. coli mutant strains with deletion of the ackA-pta and poxB pathways for the synthesis of isoamyl acetate.

作者信息

Dittrich Cheryl R, Vadali Ravishankar V, Bennett George N, San Ka-Yiu

机构信息

Department of Bioengineering, Rice University, Houston, Texas 77005, USA.

出版信息

Biotechnol Prog. 2005 Mar-Apr;21(2):627-31. doi: 10.1021/bp049730r.

Abstract

Although the bacterium E. coli is chosen as the host in many bioprocesses, products derived from the central aerobic metabolic pathway often compete with the acetate-producing pathways poxB and ackA-pta for glucose as the substrate. As such, a significant portion of the glucose may be excreted as acetate, wasting substrate that could have otherwise been used for the desired product. The production of the ester isoamyl acetate from acetyl-CoA by ATF2, a yeast alcohol acetyl transferase, was used as a model system to demonstrate the beneficial effects of reducing acetate production. All strains tested for ester production also overexpressed panK, a native E. coli gene that previous studies have shown to increase free intracellular CoA levels when fed with pantothenic acid. A recombinant E. coli strain with a deletion in ackA-pta produces less acetate and more isoamyl acetate than the wild-type E. coli strain. When both acetate-producing pathways were deleted, the acetate production was greatly reduced. However, pyruvate began to accumulate, so that the overall ester production remained largely unchanged. To produce more ester, a previously established strategy of increasing the flux from pyruvate to acetyl-CoA was adopted by overexpressing pyruvate dehydrogenase. The ester production was then 80% higher in the poxB, ackA-pta strain (0.18 mM) than that found in the single ackA-pta mutant (0.10 mM), which also overexpressed PDH.

摘要

尽管在许多生物过程中选择大肠杆菌作为宿主,但源自中心需氧代谢途径的产物通常会与产乙酸途径poxB和ackA-pta竞争葡萄糖作为底物。因此,很大一部分葡萄糖可能会以乙酸盐的形式排出,浪费了原本可用于所需产物的底物。酵母醇乙酰转移酶ATF2由乙酰辅酶A生产乙酸异戊酯用作模型系统,以证明减少乙酸盐产生的有益效果。所有测试酯生产的菌株也过表达了panK,这是一种天然的大肠杆菌基因,先前的研究表明,当提供泛酸时,该基因会增加细胞内游离辅酶A的水平。与野生型大肠杆菌菌株相比,ackA-pta基因缺失的重组大肠杆菌菌株产生的乙酸盐更少,乙酸异戊酯更多。当两条产乙酸途径都缺失时,乙酸盐的产生大大减少。然而,丙酮酸开始积累,因此总的酯产量基本保持不变。为了生产更多的酯,通过过表达丙酮酸脱氢酶采用了先前建立的增加从丙酮酸到乙酰辅酶A通量的策略。在poxB、ackA-pta菌株(0.18 mM)中,酯产量比同样过表达PDH的单ackA-pta突变体(0.10 mM)高80%。

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