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通过类异戊二烯途径的代谢工程提高食用酵母产朊假丝酵母的类胡萝卜素产量。

Increased carotenoid production by the food yeast Candida utilis through metabolic engineering of the isoprenoid pathway.

作者信息

Shimada H, Kondo K, Fraser P D, Miura Y, Saito T, Misawa N

机构信息

Central Laboratories for Key Technology, Kirin Brewery Co., Ltd., Kanagawa, Japan.

出版信息

Appl Environ Microbiol. 1998 Jul;64(7):2676-80. doi: 10.1128/AEM.64.7.2676-2680.1998.

Abstract

The yeast Candida utilis does not possess an endogenous biochemical pathway for the synthesis of carotenoids. The central isoprenoid pathway concerned with the synthesis of prenyl lipids is present in C. utilis and active in the biosynthesis of ergosterol. In our previous study, we showed that the introduction of exogenous carotenoid genes, crtE, crtB, and crtI, responsible for the formation of lycopene from the precursor farnesyl pyrophosphate, results in the C. utilis strain that yields lycopene at 1.1 mg per g (dry weight) of cells (Y. Miura, K. Kondo, T. Saito, H. Shimada, P. D. Fraser, and N. Misawa, Appl. Environ. Microbiol. 64:1226-1229, 1998). Through metabolic engineering of the isoprenoid pathway, a sevenfold increase in the yield of lycopene has been achieved. The influential steps in the pathway that were manipulated were 3-hydroxy methylglutaryl coenzyme A (HMG-CoA) reductase, encoded by the HMG gene, and squalene synthase, encoded by the ERG9 gene. Strains overexpressing the C. utilis HMG-CoA reductase yielded lycopene at 2.1 mg/g (dry weight) of cells. Expression of the HMG-CoA catalytic domain alone gave 4.3 mg/g (dry weight) of cells; disruption of the ERG9 gene had no significant effect, but a combination of ERG9 gene disruption and the overexpression of the HMG catalytic domain yielded lycopene at 7.8 mg/g (dry weight) of cells. The findings of this study illustrate how modifications in related biochemical pathways can be utilized to enhance the production of commercially desirable compounds such as carotenoids.

摘要

产朊假丝酵母不具备合成类胡萝卜素的内源性生化途径。与异戊二烯脂质合成相关的中心类异戊二烯途径存在于产朊假丝酵母中,并在麦角固醇的生物合成中发挥作用。在我们之前的研究中,我们表明引入负责从前体法尼基焦磷酸形成番茄红素的外源类胡萝卜素基因crtE、crtB和crtI,可使产朊假丝酵母菌株产生番茄红素,产量为每克(干重)细胞1.1毫克(Y. Miura、K. Kondo、T. Saito、H. Shimada、P. D. Fraser和N. Misawa,《应用与环境微生物学》64:1226 - 1229,1998)。通过对类异戊二烯途径进行代谢工程改造,番茄红素产量提高了七倍。该途径中被操控的有影响力的步骤是由HMG基因编码的3 - 羟基 - 3 - 甲基戊二酰辅酶A(HMG - CoA)还原酶和由ERG9基因编码的角鲨烯合酶。过表达产朊假丝酵母HMG - CoA还原酶的菌株产生番茄红素的量为每克(干重)细胞2.1毫克。仅表达HMG - CoA催化结构域可产生每克(干重)细胞4.3毫克;破坏ERG9基因没有显著影响,但ERG9基因破坏与HMG催化结构域过表达相结合可产生每克(干重)细胞7.8毫克的番茄红素。这项研究的结果说明了如何利用相关生化途径的修饰来提高类胡萝卜素等商业上所需化合物的产量。

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