4.8 Article

Rapid Enumeration of Phage in Monodisperse Emulsions

期刊

ANALYTICAL CHEMISTRY
卷 86, 期 12, 页码 5642-5648

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AMER CHEMICAL SOC
DOI: 10.1021/ac500244g

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  1. SENTINEL Bioactive Paper Network
  2. Alberta Glycomics Centre
  3. Alberta Innovates-Health Solutions (AIHS)
  4. Natural Sciences and Engineering Research Council of Canada (NSERC)

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Phage-based detection assays have been developed for the detection of viable bacteria for applications in clinical diagnosis, monitoring of water quality, and food safety. The majority of these assays deliver a positive readout in the form of newly generated progeny phages by the bacterial host of interest. Progeny phages are often visualized as plaques, or holes, in a lawn of bacteria on an agar-filled Petri dish; however, this rate-limiting step requires up to 12 h of incubation time. We have previously described an amplification of bacteriophages MI3 inside droplets of media suspended in perfluorinated oil; a single phage MI3 in a droplet yields 107 copies in 3-4 h. Here, we describe that encapsulation of reporter phages, both lytic T4-LacZ and nonlytic M13, in monodisperse droplets can also be used for rapid enumeration of phage. Compartmentalization in droplets accelerated the development of the signal from the reporter enzyme; counting of positive droplets yields accurate enumeration of phage particles ranging from 10(2) to 10(6) pfu/mL. For enumeration of T4-LacZ phage, the fluorescent signal appeared in as little as 90 min. Unlike bulk assays, quantification in emulsion is robust and insensitive to fluctuations in environmental conditions (e.g., temperature). Power-free emulsification using gravity-driven flow in the absence of syringe pumps and portable fluorescence imaging solutions makes this technology promising for use at the point of care in low-resource environments. This droplet-based phage enumeration method could accelerate and simplify point-of-care detection of the pathogens for which reporter bacteriophages have been developed.

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