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三羧酸循环基因破坏对酿酒酵母中琥珀酸生产的影响。

Effect of gene disruptions of the TCA cycle on production of succinic acid in Saccharomyces cerevisiae.

作者信息

Arikawa Y, Kuroyanagi T, Shimosaka M, Muratsubaki H, Enomoto K, Kodaira R, Okazaki M

机构信息

Food Technology Research Institute of Nagano Prefecture, 205-1 Nishibanba, Kurita, Nagano City 380-0921, Japan.

出版信息

J Biosci Bioeng. 1999;87(1):28-36. doi: 10.1016/s1389-1723(99)80004-8.

Abstract

Succinate is the main taste component produced by yeasts during sake (Japanese rice wine) fermentation. The pathway leading to accumulation of succinate was examined in liquid culture in the presence of a high concentration (15%) of glucose under aerobic and anaerobic conditions using a series of Saccharomyces cerevisiae strains in which various genes that encode the expression of enzymes required in TCA cycle were disrupted. When cultured in YPD medium containing 15% glucose under aerobic conditions, the KGD1 (alpha-ketoglutarate dehydrogenase) gene disrupted mutant produced a lower level of succinate than the wild-type strain, while the SDH1 (succinate dehydrogenase) gene-disrupted mutant produced an increased level of succinate. On the other hand, the FUM1 (fumarase) gene disrupted mutant produced significantly higher levels of fumarate but did not form malate at all. These results indicate that succinate, fumarate and malate are mainly synthesized through the TCA cycle (oxidative direction) even in the presence of glucose at a concentration as high as 15%. When the growth condition was shifted from aerobic to anaerobic, the increased level of succinate in SDH1 disruptants was no longer observed, whereas the decreased level of succinate in the KGD1 diruptant was still observed. A double mutant of the two fumarate reductase isozyme genes (OSM1 and FRDS) showed a succinate productivity of 50% as compared to the parent when cells were incubated in glucose-buffered solution. These results indicate that succinate could be synthesized through two pathways, namely, alpha-ketoglutarate oxidation via the TCA cycle and fumarate reduction under anaerobic conditions.

摘要

琥珀酸是酵母在清酒(日本米酒)发酵过程中产生的主要风味成分。在有氧和无氧条件下,使用一系列破坏了三羧酸循环(TCA循环)中所需酶表达的酿酒酵母菌株,在含有高浓度(15%)葡萄糖的液体培养中研究了导致琥珀酸积累的途径。当在有氧条件下于含有15%葡萄糖的YPD培养基中培养时,破坏KGD1(α-酮戊二酸脱氢酶)基因的突变体产生的琥珀酸水平低于野生型菌株,而破坏SDH1(琥珀酸脱氢酶)基因的突变体产生的琥珀酸水平升高。另一方面,破坏FUM1(延胡索酸酶)基因的突变体产生的富马酸水平显著更高,但根本不形成苹果酸。这些结果表明,即使在葡萄糖浓度高达15%的情况下,琥珀酸、富马酸和苹果酸也主要通过TCA循环(氧化方向)合成。当生长条件从有氧转变为无氧时,在SDH1破坏菌株中不再观察到琥珀酸水平的升高,而在KGD1破坏菌株中仍观察到琥珀酸水平的降低。当细胞在葡萄糖缓冲溶液中培养时,两个富马酸还原酶同工酶基因(OSM1和FRDS)的双突变体与亲本相比,琥珀酸产量为50%。这些结果表明,琥珀酸可以通过两条途径合成,即通过TCA循环进行α-酮戊二酸氧化和在厌氧条件下进行富马酸还原。

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