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利用农杆菌介导的转化在稻瘟病菌中创建插入文库。

Agrobacterium-mediated transformation to create an insertion library in Magnaporthe grisea.

作者信息

Tucker Sara L, Orbach Marc J

机构信息

Division of Plant Pathology and Microbiology, Department of Plant Sciences, University of Arizona, Tucson, USA.

出版信息

Methods Mol Biol. 2007;354:57-68. doi: 10.1385/1-59259-966-4:57.

Abstract

Magnaporthe grisea is the causal agent of rice blast disease and represents a model organism for the study of fungal plant-pathogen interactions. Pathogenicity is a complex phenotype, which is carefully orchestrated by the fungus and begins with recognition and infection of the host plant, followed by growth within the plant cells, and finally dissemination to the next host and continuation of the fungal life cycle. Certain genes must condition the ability of a pathogenic fungus to infect and cause disease symptoms. To learn more about the infection process and the genes that are involved in the complex interplay between M. grisea and rice, we used an insertional mutagenesis approach to attempt to randomly disrupt all genes in the fungal genome. Two transformation approaches were used to build a library of insertion strains in M. grisea. Polyethylene glycol/CaCl2-mediated protoplast transformation was the initial method we used and resulted in the generation of just more than 17,000 insertion strain lines. Later Agrobacterium tumefaciens-mediated transformation was adopted and the final number of insertional mutant strains of M. grisea strain 70-15 generated was more than 57,000. Here, we describe the methods used for A. tumefaciens-mediated transformation of M. grisea and the optimized protocols we have developed to enable high-throughput fungal transformation.

摘要

稻瘟病菌是水稻稻瘟病的致病因子,也是研究真菌与植物病原体相互作用的模式生物。致病性是一种复杂的表型,由真菌精心调控,始于对宿主植物的识别和感染,接着在植物细胞内生长,最后传播到下一个宿主并延续真菌的生命周期。某些基因必须决定致病真菌感染并引发疾病症状的能力。为了更深入了解感染过程以及参与稻瘟病菌与水稻之间复杂相互作用的基因,我们采用插入诱变方法试图随机破坏真菌基因组中的所有基因。我们使用两种转化方法构建了稻瘟病菌插入菌株文库。聚乙二醇/氯化钙介导的原生质体转化是我们最初使用的方法,产生了17000多个插入菌株系。后来采用了根癌农杆菌介导的转化,最终产生的稻瘟病菌70-15插入突变菌株数量超过57000个。在此,我们描述了用于根癌农杆菌介导的稻瘟病菌转化的方法以及我们开发的优化方案,以实现高通量真菌转化。

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