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野生型和工程化酿酒酵母菌株中线粒体外部 NADH 脱氢酶 Nde1 对甘油代谢的影响。

Involvement of the external mitochondrial NADH dehydrogenase Nde1 in glycerol metabolism by wild-type and engineered Saccharomyces cerevisiae strains.

机构信息

Department of Life Sciences and Chemistry, Jacobs University Bremen gGmbH, Campus Ring 1, 28759 Bremen, Germany.

出版信息

FEMS Yeast Res. 2019 May 1;19(3). doi: 10.1093/femsyr/foz026.

Abstract

Glycerol is an attractive substrate for microbial fermentations due to its higher degree of reduction compared to glucose. The replacement of the native FAD-dependent glycerol catabolic pathway in Saccharomyces cerevisiae by an artificial NADH-delivering dihydroxyacetone (DHA) pathway is supposed to facilitate the capturing of electrons in fermentation products. This requires that the electrons from the cytosolic NADH are not exclusively transferred to oxygen. However, the external NADH dehydrogenases (Nde1/2) and the L-glycerol 3-phosphate shuttle (composed of Gpd1/2 and Gut2), both coupled to the respiratory chain, are known to contribute to cytosolic NAD+ regeneration during growth on non-fermentable carbon sources. In order to evaluate the role of these mechanisms during growth on glycerol, we deleted GPD1/2, GUT2 as well as NDE1/2, separately and in combinations in both the glycerol-utilizing wild-type strain CBS 6412-13A and the corresponding engineered strain CBS DHA in which glycerol is catabolized by the DHA pathway. Particularly, the nde1Δ mutants showed a significant reduction in growth rate and the nde1∆ nde2∆ double deletion mutants did not grow at all in synthetic glycerol medium. The current work also demonstrates a positive impact of deleting NDE1 on the production of the fermentation product 1,2-propanediol in an accordingly engineered S. cerevisiae strain.

摘要

甘油相对于葡萄糖具有更高的还原程度,因此是微生物发酵的有吸引力的底物。通过用人工提供 NADH 的二羟丙酮 (DHA) 途径替代酿酒酵母中天然的依赖 FAD 的甘油分解代谢途径,应该可以促进发酵产物中电子的捕获。这需要细胞溶胶中的 NADH 电子不是专一地转移到氧气上。然而,已知与呼吸链偶联的外部 NADH 脱氢酶 (Nde1/2) 和 L-甘油 3-磷酸穿梭系统 (由 Gpd1/2 和 Gut2 组成),在非发酵碳源上生长时,有助于细胞溶胶中 NAD+的再生。为了评估这些机制在利用甘油生长过程中的作用,我们分别删除了 GPD1/2、GUT2 以及 NDE1/2,并且在利用甘油的野生型菌株 CBS 6412-13A 和相应的工程菌株 CBS DHA 中分别和组合删除了这些基因,在该工程菌株中甘油通过 DHA 途径进行分解代谢。特别是,nde1Δ 突变体的生长速率显著降低,而 nde1∆ nde2∆ 双缺失突变体在合成甘油培养基中根本无法生长。目前的工作还表明,在相应工程化的酿酒酵母菌株中删除 NDE1 对发酵产物 1,2-丙二醇的生产有积极影响。

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