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Development of an integrative DNA transformation system for the yeast Candida tropicalis.

机译:酵母热带假丝酵母的综合DNA转化系统的开发。

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摘要

We developed the alkane and fatty-acid utilizing yeast Candida tropicalis as a host for DNA transformations. The system is based on an auxotrophic mutant host of C. tropicalis which is defective in orotidine monophosphate decarboxylase (ura3). The ura3 host was isolated by mutagenesis and a double-selection procedure that combined nystatin enrichment selection and 5-fluoro-orotic acid resistance selection. As a selectable marker, we isolated and characterized the C. tropicalis URA3 gene. Plasmid vectors that contained the C. tropicalis URA3 gene transformed the C. tropicalis mutant host at a frequency of 10(3) to 10(4) transformants per micrograms of plasmid DNA. Vectors that contained the Saccharomyces cerevisiae URA3 gene could not transform C. tropicalis. DNA transfer was accomplished by modified versions of either spheroplast generation (CaCl2-polyethylene glycol)-fusion or cation (LiCl) procedures developed for S. cerevisiae. Plasmid vectors that had been cut within the C. tropicalis URA3 fragment integrated by homologous recombination at the URA3 locus.
机译:我们利用酵母假丝酵母作为DNA转化的宿主,开发了烷烃和脂肪酸。该系统基于热带梭状芽孢杆菌的营养缺陷型突变宿主,该宿主在奥洛替丁单磷酸脱羧酶(ura3)中存在缺陷。 ura3宿主是通过诱变和双重选择程序分离的,该程序将制霉菌素富集选择和5-氟乳清酸抗性选择结合在一起。作为一种选择标记,我们分离并鉴定了热带假丝酵母URA3基因。包含热带假丝酵母URA3基因的质粒载体以每微克质粒DNA 10(3)至10(4)个转化子的频率转化了热带假丝酵母突变体宿主。包含酿酒酵母URA3基因的载体不能转化热带假丝酵母。通过为酿酒酵母开发的原生质球生成(CaCl2-聚乙二醇)-融合或阳离子(LiCl)程序的修改版本来完成DNA转移。通过在URA3基因座处的同源重组整合的整合在热带假丝酵母URA3片段中的质粒载体。

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