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首页> 外文期刊>Current Genetics: Eukaryotes with Emphasis on Yeasts, Fungi, Mitochondria, Plastids >Insertion mutagenesis of the yeast Candida famata (Debaryomyces hansenii) by random integration of linear DNA fragments.
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Insertion mutagenesis of the yeast Candida famata (Debaryomyces hansenii) by random integration of linear DNA fragments.

机译:酵母假丝酵母(假丝酵母)的插入诱变通过线性DNA片段的随机整合。

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摘要

The feasibility of using random insertional mutagenesis to isolate mutants of the flavinogenic yeast Candida famata was explored. Mutagenesis was performed by transformation of the yeast with an integrative plasmid containing the Saccharomyces cerevisiae LEU2 gene as a selective marker. The addition of restriction enzyme together with the plasmid (restriction enzyme-mediated integration, REMI) increased the transformation frequency only slightly. Integration of the linearized plasmid occurred randomly in the C. famata genome. To investigate the potential of insertional mutagenesis, it was used for tagging genes involved in positive regulation of riboflavin synthesis in C. famata. Partial DNA sequencing of tagged genes showed that they were homologous to the S. cerevisiae genes RIB1, MET2, and SEF1. Intact orthologs of these genes isolated from Debaryomyces hansenii restored the wild phenotype of the corresponding mutants, i.e., the ability to overproduce riboflavin under iron limitation. The Staphylococcus aureus ble gene conferring resistance to phleomycin was used successfully in the study as a dominant selection marker for C. famata. The results obtained indicate that insertional mutagenesis is a powerful tool for tagging genes in C. famata.
机译:探索了使用随机插入诱变分离黄素生成酵母假丝酵母念珠菌的突变体的可行性。通过用包含酿酒酵母LEU2基因作为选择标记的整合质粒转化酵母来进行诱变。与质粒一起添加限制酶(限制酶介导的整合,REMI)仅稍微增加了转化频率。线性化质粒的整合随机发生在C. famata基因组中。为了研究插入诱变的潜力,将其用于标记参与正念珠菌核黄素合成正调控的基因。标记基因的部分DNA测序表明它们与酿酒酵母基因RIB1,MET2和SEF1同源。从汉逊德巴利酵母分离的这些基因的完整直系同源物恢复了相应突变体的野生表型,即在铁限制下过量生产核黄素的能力。赋予对毛霉素抗性的金黄色葡萄球菌ble基因已成功用于该研究中,作为C. famata的主要选择标记。获得的结果表明,插入诱变是标记C. famata中基因的强大工具。

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