Park Gyungsoon, Colot Hildur V, Collopy Patrick D, Krystofova Svetlana, Crew Christopher, Ringelberg Carol, Litvinkova Liubov, Altamirano Lorena, Li Liande, Curilla Susan, Wang Wei, Gorrochotegui-Escalante Norma, Dunlap Jay C, Borkovich Katherine A
Department of Plant Pathology and Microbiology, University of California, Riverside, CA, USA.
Methods Mol Biol. 2011;722:179-89. doi: 10.1007/978-1-61779-040-9_13.
The model filamentous fungus Neurospora crassa has been the focus of functional genomics studies for the past several years. A high-throughput gene knockout procedure has been developed and used to generate mutants for more than two-thirds of the ∼10,000 annotated N. crassa genes. Yeast recombinational cloning was incorporated as an efficient procedure to produce all knockout cassettes. N. crassa strains with the Δmus-51 or Δmus-52 deletion mutations were used as transformation recipients in order to reduce the incidence of ectopic integration and increase homologous recombination of knockout cassettes into the genome. A 96-well format was used for many steps of the procedure, including fungal transformation, isolation of homokaryons, and verification of mutants. In addition, development of software programs for primer design and restriction enzyme selection facilitated the high-throughput aspects of the overall protocol.
在过去几年中,模式丝状真菌粗糙脉孢菌一直是功能基因组学研究的重点。已经开发出一种高通量基因敲除方法,并用于为约10,000个已注释的粗糙脉孢菌基因中的三分之二以上生成突变体。酵母重组克隆作为一种高效方法被用于产生所有的敲除盒。带有Δmus-51或Δmus-52缺失突变的粗糙脉孢菌菌株被用作转化受体,以降低异位整合的发生率,并增加敲除盒在基因组中的同源重组。该方法的许多步骤都采用了96孔板形式,包括真菌转化、同核体分离和突变体验证。此外,用于引物设计和限制酶选择的软件程序的开发促进了整个方案的高通量操作。