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WdURA5基因的克隆及其作为hisG盒选择标记在皮炎外瓶霉中潜在破坏多个基因的应用

Cloning and use of the WdURA5 gene as a hisG cassette selection marker for potentially disrupting multiple genes in Wangiella dermatitidis.

作者信息

Zheng L, Szaniszlo P J

机构信息

Department of Microbiology, University of Texas at Austin, Austin, TX 78712, USA.

出版信息

Med Mycol. 1999 Apr;37(2):85-96.

Abstract

A genomic clone encoding the Wangiella dermatitidis orotidine monophosphate pyrophosphorylase gene (WdURA5) was isolated by screening a subgenomic plasmid DNA library of this phaeohyphomycotic agent using a PCR amplification product of the gene as a probe. When plasmid DNA containing the cloned WdURA5 gene was introduced by electroporation into a wdura5 auxotrophic recipient strain derived previously by selection with 5-fluoroorotic acid (5-FOA), an apparent gene repair event occurred at high frequency without any evidence of integration of the plasmid DNA. Therefore, the hygromycin B resistance gene (the hph gene) was used as a dominant selective marker for the disruption of WdURA5 to generate a new, more stable, wdura5 auxotrophic strain. Transformation of this strain was then achieved with high efficiency and high frequency by site-specific integration using WdURA5 as a selective marker. To initiate attempts to use this marker repeatedly for multiple chitin synthase (WdCHS) gene disruptions in single strains of W. dermatitidis, a hisG_WdURA5_hisG cassette was constructed and used to disrupt WdCHS2. The WdURA5 gene in the disruptant was then successfully recycled under selection for resistance to 5-FOA.

摘要

通过使用该基因的PCR扩增产物作为探针,筛选该暗色丝孢霉病原体的亚基因组质粒DNA文库,分离出编码皮炎万吉拉霉乳清苷单磷酸焦磷酸化酶基因(WdURA5)的基因组克隆。当通过电穿孔将含有克隆的WdURA5基因的质粒DNA导入先前通过用5-氟乳清酸(5-FOA)选择获得的wdura5营养缺陷型受体菌株时,高频发生了明显的基因修复事件,且没有质粒DNA整合的任何证据。因此,潮霉素B抗性基因(hph基因)被用作破坏WdURA5的显性选择标记,以产生新的、更稳定的wdura5营养缺陷型菌株。然后,以WdURA5作为选择标记,通过位点特异性整合,高效且高频地实现了该菌株的转化。为了开始尝试在皮炎万吉拉霉的单个菌株中反复使用该标记进行多个几丁质合酶(WdCHS)基因的破坏,构建了hisG_WdURA5_hisG盒并用于破坏WdCHS2。然后,在对5-FOA抗性的选择下,成功回收了破坏株中的WdURA5基因。

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