在Crabtree阴性的酿酒酵母中高效的基于转录组的非乙醇化学物质的生物合成。

Zhen Yao, Yufeng Guo, Huan Wang, Yun Chen, Qinhong Wang, Jens Nielsen, Zongjie Dai
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引用次数: 1

摘要

背景:由于Crabtree效应,酿酒酵母在氧气和过量葡萄糖存在的情况下产生大量乙醇,导致碳的损失,用于非乙醇化学物质的生物合成。在本研究中,我们探索了新构建的Crabtree阴性酿酒酵母作为底盘细胞的潜力,用于生物合成各种非乙醇化合物。结果:为了解Crabtree阴性酿酒葡萄球菌sZJD-28的代谢特征,将其转录谱与Crabtree阳性酿酒葡萄球菌cn . pk113 - 11c进行了比较。记者GO项分析显示,在sZJD-28中,与翻译过程相关的基因下调,而与碳代谢相关的基因显著上调。为了验证Crabtree阴性菌株的碳代谢可能增加,然后对sZJD-28和cn . pk113 - 11c进行了非乙醇化学物质的生产,这些化学物质来自不同的代谢节点。在丙酮酸节点,szjd -28菌株的2,3-丁二醇和乳酸产量显著高于CEN菌株。以pk113 - 11c为基础的基因,滴度分别提高16.8倍和1.65倍,特异性滴度(mg/L/OD)分别提高4.5倍和0.65倍。同样,对莽草酸衍生对香豆酸,基于szjd -28的菌株的滴度比CEN高0.68倍。以pk113 - 11c为基础,特异性滴度提高0.98倍。而两种乙酰辅酶a衍生物法脂烯和番茄红素的滴度分别增加了0.21倍和1.88倍。从丙二酰辅酶a来看,szjd -28菌株的3-羟丙酸和脂肪酸滴度分别是CEN的0.19倍和0.76倍。分别基于pk113 - 11c。事实上,由于没有残留的葡萄糖,产品的收率也提高了同样的倍。分批补料发酵进一步表明,基于szjd -28的菌株28-FFA-E的游离脂肪酸滴度达到6295.6 mg/L,最高报道的酿酒酵母特异性滴度为247.7 mg/L/OD。结论:与CEN比较。在PK113-11C中,阴性菌株sZJD-28表现出了显著不同的转录谱,并且由于碳和能量来源转向代谢物生物合成,在非乙醇化学物质的生物合成中具有明显的优势。因此,这一发现表明,一株Crabtree阴性酿酒葡萄球菌菌株可能是一种有希望的用于各种化学物质生物合成的底盘细胞。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

A highly efficient transcriptome-based biosynthesis of non-ethanol chemicals in Crabtree negative Saccharomyces cerevisiae.

A highly efficient transcriptome-based biosynthesis of non-ethanol chemicals in Crabtree negative Saccharomyces cerevisiae.

A highly efficient transcriptome-based biosynthesis of non-ethanol chemicals in Crabtree negative Saccharomyces cerevisiae.

A highly efficient transcriptome-based biosynthesis of non-ethanol chemicals in Crabtree negative Saccharomyces cerevisiae.

Background: Owing to the Crabtree effect, Saccharomyces cerevisiae produces a large amount of ethanol in the presence of oxygen and excess glucose, leading to a loss of carbon for the biosynthesis of non-ethanol chemicals. In the present study, the potential of a newly constructed Crabtree negative S. cerevisiae, as a chassis cell, was explored for the biosynthesis of various non-ethanol compounds.

Results: To understand the metabolic characteristics of Crabtree negative S. cerevisiae sZJD-28, its transcriptional profile was compared with that of Crabtree positive S. cerevisiae CEN.PK113-11C. The reporter GO term analysis showed that, in sZJD-28, genes associated with translational processes were down-regulated, while those related to carbon metabolism were significantly up-regulated. To verify a potential increase in carbon metabolism for the Crabtree negative strain, the production of non-ethanol chemicals, derived from different metabolic nodes, was then undertaken for both sZJD-28 and CEN.PK113-11C. At the pyruvate node, production of 2,3-butanediol and lactate in sZJD-28-based strains was remarkably higher than that of CEN.PK113-11C-based ones, representing 16.8- and 1.65-fold increase in titer, as well as 4.5-fold and 0.65-fold increase in specific titer (mg/L/OD), respectively. Similarly, for shikimate derived p-coumaric acid, the titer of sZJD-28-based strain was 0.68-fold higher than for CEN.PK113-11C-based one, with a 0.98-fold increase in specific titer. While farnesene and lycopene, two acetoacetyl-CoA derivatives, showed 0.21- and 1.88-fold increases in titer, respectively. From malonyl-CoA, the titer of 3-hydroxypropionate and fatty acids in sZJD-28-based strains were 0.19- and 0.76-fold higher than that of CEN.PK113-11C-based ones, respectively. In fact, yields of products also improved by the same fold due to the absence of residual glucose. Fed-batch fermentation further showed that the titer of free fatty acids in sZJD-28-based strain 28-FFA-E reached 6295.6 mg/L with a highest reported specific titer of 247.7 mg/L/OD in S. cerevisiae.

Conclusions: Compared with CEN.PK113-11C, the Crabtree negative sZJD-28 strain displayed a significantly different transcriptional profile and obvious advantages in the biosynthesis of non-ethanol chemicals due to redirected carbon and energy sources towards metabolite biosynthesis. The findings, therefore, suggest that a Crabtree negative S. cerevisiae strain could be a promising chassis cell for the biosynthesis of various chemicals.

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