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用于生产碳五平台化学品5-氨基戊酸和戊二酸的谷氨酸棒杆菌系统代谢工程

Systems metabolic engineering of Corynebacterium glutamicum for the production of the carbon-5 platform chemicals 5-aminovalerate and glutarate.

作者信息

Rohles Christina Maria, Gießelmann Gideon, Kohlstedt Michael, Wittmann Christoph, Becker Judith

机构信息

Institute of Systems Biotechnology, Saarland University, Saarbrücken, Germany.

出版信息

Microb Cell Fact. 2016 Sep 13;15(1):154. doi: 10.1186/s12934-016-0553-0.

Abstract

BACKGROUND

The steadily growing world population and our ever luxurious life style, along with the simultaneously decreasing fossil resources has confronted modern society with the issue and need of finding renewable routes to accommodate for our demands. Shifting the production pipeline from raw oil to biomass requires efficient processes for numerous platform chemicals being produced with high yield, high titer and high productivity.

RESULTS

In the present work, we established a de novo bio-based production process for the two carbon-5 platform chemicals 5-aminovalerate and glutarate on basis of the lysine-hyperproducing strain Corynebacterium glutamicum LYS-12. Upon heterologous implementation of the Pseudomonas putida genes davA, encoding 5-aminovaleramidase and davB, encoding lysine monooxygenase, 5-aminovalerate production was established. Related to the presence of endogenous genes coding for 5-aminovalerate transaminase (gabT) and glutarate semialdehyde dehydrogenase, 5-aminovalerate was partially converted to glutarate. Moreover, residual L-lysine was secreted as by-product. The issue of by-product formation was then addressed by deletion of the lysE gene, encoding the L-lysine exporter. Additionally, a putative gabT gene was deleted to enhance 5-aminovalerate production. To fully exploit the performance of the optimized strain, fed-batch fermentation was carried out producing 28 g L(-1) 5-aminovalerate with a maximal space-time yield of 0.9 g L(-1) h(-1).

CONCLUSIONS

The present study describes the construction of a recombinant microbial cell factory for the production of carbon-5 platform chemicals. Beyond a basic proof-of-concept, we were able to specifically increase the production flux of 5-aminovalerate thereby generating a strain with excellent production performance. Additional improvement can be expected by removal of remaining by-product formation and bottlenecks, associated to the terminal pathway, to generate a strain being applicable as centerpiece for a bio-based production of 5-aminovalerate.

摘要

背景

世界人口稳步增长,我们的生活方式日益奢华,同时化石资源不断减少,这使现代社会面临寻找可再生途径以满足我们需求的问题和需求。将生产流程从原油转向生物质需要高效的工艺来大量生产高产量、高滴度和高生产率的多种平台化学品。

结果

在本研究中,我们基于赖氨酸高产菌株谷氨酸棒杆菌LYS-12建立了从头生物基生产两种C5平台化学品5-氨基戊酸和戊二酸的工艺。在异源表达恶臭假单胞菌编码5-氨基戊酰胺酶的davA基因和编码赖氨酸单加氧酶的davB基因后,建立了5-氨基戊酸的生产。由于存在编码5-氨基戊酸转氨酶(gabT)和戊二醛半醛脱氢酶的内源基因,5-氨基戊酸部分转化为戊二酸。此外,残留的L-赖氨酸作为副产物分泌。然后通过缺失编码L-赖氨酸输出蛋白的lysE基因来解决副产物形成的问题。此外,删除了一个假定的gabT基因以提高5-氨基戊酸的产量。为了充分发挥优化菌株的性能,进行了补料分批发酵,生产出28 g L⁻¹的5-氨基戊酸,最大时空产率为0.9 g L⁻¹ h⁻¹。

结论

本研究描述了用于生产C5平台化学品的重组微生物细胞工厂的构建。除了基本的概念验证外,我们能够特异性地增加5-氨基戊酸的生产通量,从而产生具有优异生产性能的菌株。通过去除与终端途径相关的剩余副产物形成和瓶颈,有望进一步改进,以产生一种可作为基于生物的5-氨基戊酸生产核心的菌株。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/ed7f/5020477/f595df112e2e/12934_2016_553_Fig1_HTML.jpg

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