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Development of the CRISPR/Cas9 System for Targeted Gene Disruption in Aspergillus fumigatus

机译:用于烟曲霉中靶向基因破坏的CRISPR / Cas9系统的开发

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摘要

Low rates of homologous recombination have broadly encumbered genetic studies in the fungal pathogen Aspergillus fumigatus. The CRISPR/Cas9 system of bacteria has recently been developed for targeted mutagenesis of eukaryotic genomes with high efficiency and, importantly, through a mechanism independent of homologous repair machinery. As this new technology has not been developed for use in A. fumigatus, we sought to test its feasibility for targeted gene disruption in this organism. As a proof of principle, we first demonstrated that CRISPR/Cas9 can indeed be used for high-efficiency (25 to 53%) targeting of the A. fumigatus polyketide synthase gene (pksP), as evidenced by the generation of colorless (albino) mutants harboring the expected genomic alteration. We further demonstrated that the constitutive expression of the Cas9 nuclease by itself is not deleterious to A. fumigatus growth or virulence, thus making the CRISPR system compatible with studies involved in pathogenesis. Taken together, these data demonstrate that CRISPR can be utilized for loss-of-function studies in A. fumigatus and has the potential to bolster the genetic toolbox for this important pathogen.
机译:真菌病原体烟曲霉的低同源重组率已广泛地进行了遗传学研究。细菌的CRISPR / Cas9系统最近已经开发出来,可以高效,重要的是通过独立于同源修复机制的机制进行真核基因组的定向诱变。由于尚未开发出可用于烟曲霉的新技术,我们寻求测试其在该生物中靶向基因破坏的可行性。作为原理的证明,我们首先证明了CRISPR / Cas9确实可以用于烟曲霉聚酮化合物合酶基因(pksP)的高效靶向(25%至53%),这一点已通过无色(白蛋白)的产生得以证明。具有预期的基因组改变的突变体。我们进一步证明,Cas9核酸酶本身的组成型表达对烟曲霉的生长或毒力无害,因此使CRISPR系统与发病机理相关的研究兼容。综上所述,这些数据表明CRISPR可以用于烟曲霉的功能丧失研究,并有可能增强这一重要病原体的遗传工具箱。

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