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酿酒酵母中维生素B12依赖性的发展。

Development of vitamin B12 dependency in Saccharomyces cerevisiae.

作者信息

Lehner Sandra, Boles Eckhard

机构信息

Institute of Molecular Biosciences, Faculty of Biological Sciences, Goethe University Frankfurt, Frankfurt am Main 60438, Germany.

出版信息

FEMS Yeast Res. 2023 Jan 4;23. doi: 10.1093/femsyr/foad020.

DOI:10.1093/femsyr/foad020
PMID:36941127
Abstract

For decades, the industrial vitamin B12 (cobalamin) production has been based on bacterial producer strains. Due to limited methods for strain optimization and difficult strain handling, the desire for new vitamin B12-producing hosts has risen. As a vitamin B12-independent organism with a big toolbox for genomic engineering and easy-to-handle cultivation conditions, Saccharomyces cerevisiae has high potential for heterologous vitamin B12 production. However, the B12 synthesis pathway is long and complex. To be able to easily engineer and evolve B12-producing recombinant yeast cells, we have developed an S. cerevisiae strain whose growth is dependent on vitamin B12. For this, the B12-independent methionine synthase Met6 of yeast was replaced by a B12-dependent methionine synthase MetH from Escherichia coli. Adaptive laboratory evolution, RT-qPCR, and overexpression experiments show that additional high-level expression of a bacterial flavodoxin/ferredoxin-NADP+ reductase (Fpr-FldA) system is essential for in vivo reactivation of MetH activity and growth. Growth of MetH-containing yeast cells on methionine-free media is only possible with the addition of adenosylcobalamin or methylcobalamin. A heterologous vitamin B12 transport system turned out to be not necessary for the uptake of cobalamins. This strain should be a powerful chassis to engineer B12-producing yeast cells.

摘要

几十年来,工业上生产维生素B12(钴胺素)一直基于细菌生产菌株。由于菌株优化方法有限且菌株处理困难,人们对新型维生素B12生产宿主的需求日益增加。酿酒酵母作为一种不依赖维生素B12的生物体,拥有用于基因组工程的丰富工具且培养条件易于操作,在异源生产维生素B12方面具有很高的潜力。然而,B12合成途径漫长而复杂。为了能够轻松地对生产B12的重组酵母细胞进行工程改造和进化,我们构建了一种生长依赖于维生素B12的酿酒酵母菌株。为此,将酵母中不依赖B12的甲硫氨酸合酶Met6替换为来自大肠杆菌的依赖B12的甲硫氨酸合酶MetH。适应性实验室进化、RT-qPCR和过表达实验表明,额外高水平表达细菌黄素氧还蛋白/铁氧还蛋白-NADP+还原酶(Fpr-FldA)系统对于MetH活性的体内再激活和生长至关重要。含MetH的酵母细胞只有在添加腺苷钴胺素或甲基钴胺素的情况下才能在无甲硫氨酸的培养基上生长。结果表明,异源维生素B12转运系统对于钴胺素的摄取并非必需。该菌株应该是工程改造生产B12的酵母细胞的强大底盘。

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