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Enhanced production of polysialic acid by metabolic engineering of Escherichia coli

机译:通过大肠杆菌的代谢工程提高多唾液酸的产量

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摘要

A number of reports have described the production of polysialic acid (PSA), focusing on the fermentation and purification of PSA. However, little work has been done to strengthen the synthetic pathway of PSA to improve PSA production. In this study, an efficient process for enhanced production of PSA using a recombinant Escherichia coli strain was developed. To improve the PSA production efficiency, the key enzymes of PSA synthetic pathway were overexpressed separately or in combination, including N-acetylneuraminate (Neu5Ac) 7-O(or 9-O)-acetyltransferase (NeuD), CMP-Neu5Ac synthetase (NeuA), and alpha-Neu5Ac alpha-2,8-sialyltransferase (NeuS). The PSA production was significantly improved by coexpression of NeuD and NeuA. In terms of the efficiency, NeuD was considered as the most important factor. Secondly, the competing pathway of intermediate Neu5Ac was blocked by nanA deletion. The efficient PSA-producing strain E. coli SA9 Delta nanA/pDB1S-DA was constructed, and 16.15 +/- 1.45 g/L PSA was obtained in the fed-batch culture. The production of PSA by engineered strain was increased by 85 % compared to the original strain. These results provide evidence for improvement of PSA production by regulation of the PSA biosynthetic pathway. The high productivity of our process should make it a promising cost-effective resource for PSA.
机译:许多报告描述了聚唾液酸(PSA)的生产,着重于PSA的发酵和纯化。但是,加强PSA的合成途径以提高PSA产量的工作很少。在这项研究中,开发了使用重组大肠杆菌菌株提高PSA产量的有效方法。为了提高PSA的生产效率,PSA合成途径的关键酶被单独或组合过量表达,包括N-乙酰神经氨酸(Neu5Ac)7-O(或9-O)-乙酰基转移酶(NeuD),CMP-Neu5Ac合成酶(NeuA) ,以及alpha-Neu5Ac alpha-2,8-唾液酸转移酶(NeuS)。通过NeuD和NeuA的共表达可显着提高PSA的产量。在效率方面,NeuD被认为是最重要的因素。其次,中间体Neu5Ac的竞争途径被nanA缺失所阻断。构建了有效产生PSA的菌株大肠杆菌SA9 Delta nanA / pDB1S-DA,在分批补料培养中获得了16.15 +/- 1.45 g / L PSA。与原始菌株相比,工程菌株产生的PSA产量提高了85%。这些结果提供了通过调节PSA生物合成途径来改善PSA生产的证据。我们过程的高生产率应使其成为PSA的有前途的成本效益资源。

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