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通过连续培养优化热带假丝酵母细胞色素P450alk基因在酿酒酵母中的表达。

Optimization of Candida tropicalis cytochrome P450alk gene expression in Saccharomyces cerevisiae with continuous cultures.

作者信息

Beretta I, Sanglard D, Käppeli O, Fiechter A

机构信息

Institute of Biotechnology, ETH-Hönggerberg, Zürich, Switzerland.

出版信息

Appl Microbiol Biotechnol. 1991 Oct;36(1):48-60. doi: 10.1007/BF00164698.

Abstract

The cytochrome P450alk gene (P45alk) from Candida tropicalis ATCC 750 was expressed in Saccharomyces cerevisiae GRF18 under control of the alcohol dehydrogenase I (ADHI) promoter. To achieve stable expression over long time periods, a 2-microns derived replicative and an integrative expression system were tested in continuous culture. The 2-microns derived replicative system could not be maintained in cells over high generation numbers. In continuous culture, the instability was more pronounced at high dilution rates (D) and high histidine concentration, for which the yeast is auxotrophic. The nature of the instability was probably due to a gene conversion event between the plasmid and the yeast chromosome. In contrast, the integrative expression system was stably maintained in cells over prolonged cultivation times. Since this work focused on the production of large quantities of P450 by heterologous expression in yeast over prolonged time periods, the integrant was used to optimize P450alk expression by varying continuous culture parameters. The P450alk expression was shown to be dependent on the D applied to the culture. The highest P450alk expression levels were obtained at high D, when cell metabolism was shifted to partial glucose oxidation, yielding ethanol as a major metabolite in the culture supernatant. In contrast, when glucose was completely oxidized at low D, the ADHI-dependent P450alk expression was reduced and followed by a corresponding decrease in heterologous protein.

摘要

热带假丝酵母ATCC 750的细胞色素P450alk基因(P45alk)在乙醇脱氢酶I(ADHI)启动子的控制下,在酿酒酵母GRF18中表达。为了实现长时间的稳定表达,在连续培养中测试了一种源自2-μm的复制型表达系统和整合型表达系统。源自2-μm的复制型系统在高代数细胞中无法维持。在连续培养中,不稳定性在高稀释率(D)和高组氨酸浓度下更为明显,而酵母对组氨酸是营养缺陷型。这种不稳定性的本质可能是由于质粒与酵母染色体之间的基因转换事件。相比之下,整合型表达系统在长时间培养过程中能在细胞中稳定维持。由于这项工作的重点是通过在酵母中长时间异源表达来大量生产P450,因此通过改变连续培养参数,利用整合体来优化P450alk的表达。结果表明,P450alk的表达取决于应用于培养物的D。当细胞代谢转向部分葡萄糖氧化,在培养上清液中产生乙醇作为主要代谢产物时,在高D条件下可获得最高的P450alk表达水平。相反,当在低D条件下葡萄糖完全氧化时,依赖ADHI的P450alk表达降低,随后异源蛋白相应减少。

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