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Deletion and Allelic Exchange of the Aspergillus fumigatus veA Locus via a Novel Recyclable Marker Module

机译:通过新型可回收标记模块删除烟曲霉veA基因座和等位基因交换

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摘要

Detailed evaluation of gene functions in an asexual fungus requires advanced methods of molecular biology. For the generation of targeted gene deletions in the opportunistic pathogen Aspergillus fumigatus we designed a novel blaster module allowing dominant selection of transformants due to resistance to phleomycin as well as dominant (counter)selection of a Cre recombinase-mediated marker excision event. For validation purposes we have deleted the A. fumigatus pabaA gene in a wild-type isolate by making use of this cassette. The resulting pabaA::loxP strain served as the recipient for subsequent targeting of the velvet locus. Homologous reconstitution of the deleted gene was performed by an allele whose expression is driven in a nitrogen source-dependent manner, as validated by Northern analyses. Overexpression of the veA locus in A. fumigatus does not result in any obvious phenotype, whereas the sporulation capacities of the veA null mutant are reduced on nitrate-containing medium, a phenotype that is completely restored in the reconstituted strain.
机译:无性真菌中基因功能的详细评估需要先进的分子生物学方法。为了在机会性病原体烟曲霉中生​​成靶向基因的缺失,我们设计了一种新型的blaster模块,该模块可基于对毛霉素的抗性以及对Cre重组酶介导的标记切除事件的显性(反选择)选择转化子。为了验证目的,我们通过使用该盒删除了野生型分离物中的烟曲霉pabaA基因。所得的pabaA :: loxP菌株用作随后靶向天鹅绒基因座的受体。缺失基因的同源重组是通过等位基因进行的,其表达以依赖氮源的方式驱动,这已被Northern分析证实。烟曲霉中veA基因座的过表达不会导致任何明显的表型,而在含硝酸盐的培养基上veA null突变体的孢子形成能力却降低了,该表型在重组菌株中已完全恢复。

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