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鉴定构巢曲霉生物素生物合成基因簇和利用 bioDA 基因作为新的转化标记。

Characterization of the Aspergillus nidulans biotin biosynthetic gene cluster and use of the bioDA gene as a new transformation marker.

机构信息

Department of Plant Molecular Biology, Biophore Building, University of Lausanne, CH-1015 Lausanne, Switzerland.

出版信息

Fungal Genet Biol. 2011 Feb;48(2):208-15. doi: 10.1016/j.fgb.2010.08.004. Epub 2010 Aug 14.

DOI:10.1016/j.fgb.2010.08.004
PMID:20713166
Abstract

The genes involved in the biosynthesis of biotin were identified in the hyphal fungus Aspergillus nidulans through homology searches and complementation of Escherichia coli biotin-auxotrophic mutants. Whereas the 7,8-diaminopelargonic acid synthase and dethiobiotin synthetase are encoded by distinct genes in bacteria and the yeast Saccharomyces cerevisiae, both activities are performed in A. nidulans by a single enzyme, encoded by the bifunctional gene bioDA. Such a bifunctional bioDA gene is a genetic feature common to numerous members of the ascomycete filamentous fungi and basidiomycetes, as well as in plants and oömycota. However, unlike in other eukaryota, the three bio genes contributing to the four enzymatic steps from pimeloyl-CoA to biotin are organized in a gene cluster in pezizomycotina. The A. nidulans auxotrophic mutants biA1, biA2 and biA3 were all found to have mutations in the 7,8-diaminopelargonic acid synthase domain of the bioDA gene. Although biotin auxotrophy is an inconvenient marker in classical genetic manipulations due to cross-feeding of biotin, transformation of the biA1 mutant with the bioDA gene from either A. nidulans or Aspergillus fumigatus led to the recovery of well-defined biotin-prototrophic colonies. The usefulness of bioDA gene as a novel and robust transformation marker was demonstrated in co-transformation experiments with a green fluorescent protein reporter, and in the efficient deletion of the laccase (yA) gene via homologous recombination in a mutant lacking non-homologous end-joining activity.

摘要

参与生物素生物合成的基因在丝状真菌构巢曲霉中通过同源搜索和大肠杆菌生物素营养缺陷型突变体的互补鉴定。虽然 7,8-二氨基庚酸合酶和脱硫生物素合成酶在细菌和酵母酿酒酵母中由不同的基因编码,但这两种活性都由单个酶在构巢曲霉中完成,该酶由双功能基因 bioDA 编码。这种双功能的 bioDA 基因是子囊菌丝状真菌和担子菌以及植物和卵菌中许多成员的遗传特征。然而,与其他真核生物不同的是,对从丙二酰辅酶 A 到生物素的四个酶促步骤做出贡献的三个 bio 基因在 pezizomycotina 中组织在一个基因簇中。发现构巢曲霉营养缺陷型突变体 biA1、biA2 和 biA3 在 bioDA 基因的 7,8-二氨基庚酸合酶结构域中均发生突变。尽管生物素营养缺陷型是由于生物素的交叉喂养而在经典遗传操作中不方便的标记,但将 bioDA 基因从构巢曲霉或烟曲霉转化到 biA1 突变体中,导致了明确的生物素原养型菌落的恢复。在与绿色荧光蛋白报告基因的共转化实验以及在缺乏非同源末端连接活性的突变体中通过同源重组有效删除漆酶 (yA) 基因的实验中,bioDA 基因作为一种新型且强大的转化标记的有用性得到了证明。

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