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使用液滴数字 PCR 技术在体外和体内快速定量噬菌体及其细菌宿主。

Rapid quantification of bacteriophages and their bacterial hosts in vitro and in vivo using droplet digital PCR.

机构信息

Department of Plant and Microbial Biology, University of California, Berkeley, Berkeley, CA, 94720, USA.

Department of Integrative Biology, University of California, Berkeley, Berkeley, CA, 94720, USA.

出版信息

J Virol Methods. 2018 Sep;259:18-24. doi: 10.1016/j.jviromet.2018.05.007. Epub 2018 May 30.

Abstract

Viruses that infect bacteria, bacteriophages (phages), are well-studied across a wide range of environments and among diverse scientific fields. Nevertheless, current methods in phage research are lacking, in part due to limitations in culturability and the lack of a universal gene marker. Here, we demonstrate that droplet digital PCR (ddPCR) can be used as a repeatable and sensitive method to study bacteria-phage dynamics both in vitro and in vivo. Using fluorescent probes designed for the bacterial plant pathogen, Pseudomonas syringae, and two phages that prey upon it, we illustrate the use of ddPCR to enumerate phages, track bacteria and phage densities over time both in media co-culture and during infection of a tomato plant, compare phage time-to-lysis, and explore phage-phage competition. Overall, the ddPCR approach closley mirrors results from more traditional counts of plaque forming units (PFUs) but offers a much faster, lower waste, and more high-throughput way of studying these interactions. As such, we suggest that ddPCR will be a valuable new tool in bacteriophage research.

摘要

感染细菌的病毒,噬菌体(phages),在广泛的环境和不同的科学领域中都得到了很好的研究。然而,目前的噬菌体研究方法还存在不足,部分原因是可培养性的限制以及缺乏通用的基因标记。在这里,我们证明了液滴数字 PCR(ddPCR)可以作为一种可重复且敏感的方法,用于研究体外和体内的细菌-噬菌体动态。我们使用针对细菌植物病原体丁香假单胞菌和两种捕食它的噬菌体设计的荧光探针,说明了 ddPCR 用于计数噬菌体、随时间追踪细菌和噬菌体密度的方法,包括在共培养物中的介质和感染番茄植物的过程中,比较噬菌体的裂解时间,并探索噬菌体之间的竞争。总的来说,ddPCR 方法与传统的噬菌斑形成单位(PFU)计数结果非常吻合,但提供了一种更快、浪费更少、高通量的研究这些相互作用的方法。因此,我们认为 ddPCR 将成为噬菌体研究的一个有价值的新工具。

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