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通过代谢工程和经典选育,对产朊假丝酵母(弗氏毕赤酵母)进行改造,构建提高核黄素产量的工程菌。

Metabolic engineering and classic selection of the yeast Candida famata (Candida flareri) for construction of strains with enhanced riboflavin production.

机构信息

Department of Molecular Genetics and Biotechnology, Institute of Cell Biology, NAS of Ukraine, Drahomanov Street 14/16, Lviv 79005, Ukraine.

出版信息

Metab Eng. 2011 Jan;13(1):82-8. doi: 10.1016/j.ymben.2010.10.005. Epub 2010 Oct 30.

DOI:10.1016/j.ymben.2010.10.005
PMID:21040798
Abstract

Currently, the mutant of the flavinogenic yeast Candida famata dep8 isolated by classic mutagenesis and selection is used for industrial riboflavin production. Here we report on construction of a riboflavin overproducing strain of C. famata using a combination of random mutagenesis based on the selection of mutants resistant to different antimetabolites as well as rational approaches of metabolic engineering. The conventional mutagenesis involved consecutive selection for resistance to riboflavin structural analog 7-methyl-8-trifluoromethyl-10-(1'-d-ribityl)isoalloxazine), 8-azaguanine, 6-azauracil, 2-diazo-5-oxo-L-norleucine and guanosine as well as screening for yellow colonies at high pH. The metabolic engineering approaches involved introduction of additional copies of transcription factor SEF1 and IMH3 (coding for IMP dehydrogenase) orthologs from Debaryomyces hansenii, and the homologous genes RIB1 and RIB7, encoding GTP cyclohydrolase II and riboflavin synthetase, the first and the last enzymes of riboflavin biosynthesis pathway, respectively. Overexpression of the aforementioned genes in riboflavin overproducer AF-4 obtained by classical selection resulted in a 4.1-fold increase in riboflavin production in shake-flask experiments. D. hansenii IMH3 and modified ARO4 genes conferring resistance to mycophenolic acid and fluorophenylalanine, respectively, were successfully used as new dominant selection markers for C. famata.

摘要

目前,通过经典诱变和筛选分离出的黄素产生酵母 Candida famata dep8 的突变体被用于工业核黄素生产。在这里,我们报告了使用基于对不同抗代谢物抗性突变体选择的随机诱变与代谢工程的合理方法相结合,构建了产核黄素高产菌株 C. famata。常规诱变涉及连续选择对核黄素结构类似物 7-甲基-8-三氟甲基-10-(1'-d-核酮糖基)异咯嗪、8-氮杂鸟嘌呤、6-氮尿嘧啶、2-重氮-5-氧代-L-正亮氨酸和鸟嘌呤的抗性,以及在高 pH 值下筛选黄色菌落。代谢工程方法涉及引入 Debaryomyces hansenii 的转录因子 SEF1 和 IMH3(编码 IMP 脱氢酶)同源物以及编码 GTP 环化水解酶 II 和核黄素合成酶的同源基因 RIB1 和 RIB7,它们分别是核黄素生物合成途径的第一个和最后一个酶。在通过经典选择获得的核黄素高产菌 AF-4 中过表达上述基因,在摇瓶实验中核黄素产量增加了 4.1 倍。D. hansenii IMH3 和修饰的 ARO4 基因分别赋予对吗啉代丙氨酸和氟苯丙氨酸的抗性,成功地用作 Candida famata 的新显性选择标记。

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