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首页> 外文期刊>Cell Reports >Tracing Conidial Fate and Measuring Host Cell Antifungal Activity Using a Reporter of Microbial Viability in the Lung
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Tracing Conidial Fate and Measuring Host Cell Antifungal Activity Using a Reporter of Microbial Viability in the Lung

机译:追踪分生孢子的命运并使用肺部微生物生存力的报告者来测量宿主细胞的抗真菌活性

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Fluorescence can be harnessed to monitor microbial fate and to investigate functional outcomes of individual microbial cell-host cell encounters at portals of entry in native tissue environments. We illustrate this concept by introducing fluorescent Aspergillus reporter (FLARE) conidia that simultaneously report phagocytic uptake and fungal viability during cellular interactions with the murine respiratory innate immune system. Our studies using FLARE conidia reveal stepwise and cell-type-specific requirements for CARD9 and Syk, transducers of C-type lectin receptor and integrin signals, in neutrophil recruitment, conidial uptake, and conidial killing in the lung. By achieving single-event resolution in defined leukocyte populations, the FLARE method enables host cell profiling on the basis of pathogen uptake and killing and may be extended to other pathogens in diverse model host organisms to query molecular, cellular, and pharmacologic mechanisms that shape host-microbe interactions.
机译:可以利用荧光来监测微生物的命运,并研究在天然组织环境中入口处各个微生物细胞-宿主细胞相遇的功能结果。我们通过引入荧光曲霉记者(FLARE)分生孢子来说明这个概念,该孢子同时报告吞噬细胞摄取和真菌活力与小鼠呼吸系统先天免疫系统的细胞相互作用期间。我们使用FLARE分生孢子进行的研究揭示了中性粒细胞募集,分生孢子摄取和分生孢子杀伤中CARD9和Syk(C型凝集素受体和整联蛋白信号的转化子)的逐步和细胞类型特异性要求。通过在限定的白细胞群体中实现单事件解析,FLARE方法可根据病原体摄取和杀死情况对宿主细胞进行分析,并可扩展到多种模型宿主生物中的其他病原体,以查询形成宿主的分子,细胞和药理机制-微生物相互作用。

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