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Real-time quantitative PCR with gene probe, fluorochrome and flow cytometry for microorganism analysis

机译:使用基因探针,荧光染料和流式细胞仪进行实时定量PCR进行微生物分析

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摘要

Microorganism concentrations and viability can be better understood and clarified by using both culture and non-culture methods. Here, using pure suspensions of E. coli, three non-culture methods, namely, flow cytometry (FCM), epifluorescence microscopy (EFM), and real-time quantitative polymerase chain reaction (real-time qPCR), were compared with a traditional culture-based method. Using. uorocome-labeling methods with FCM and EFM applications, acridine orange (AO) and propidium iodide ( PI) dyes were used to determine the total cell concentration and microorganism viability, respectively. The results indicated that total cell concentrations determined using FCM were statistically higher (2.62 - 4.94 times) than those determined using EFM. The difference might be due to cell losses induced by extensive preparations needed for EFM. In addition, EFM and FCM were highly associated for both the total cell concentration and viability. FCM-measured viability was the highest, whereas the culture-measured viability was the lowest. Furthermore, DNA concentrations measured by real-time qPCR with gene probe were highly associated with the total number concentrations measured by either the EFM or FCM. In summary, the three non-culture methods compared here could provide rapid and accurate information about microorganism concentrations and viabilities.
机译:通过使用培养和非培养方法,可以更好地理解和阐明微生物的浓度和生存力。在这里,使用大肠杆菌的纯悬液,将三种非培养方法,即流式细胞术(FCM),落射荧光显微镜(EFM)和实时定量聚合酶链反应(实时qPCR)与传统方法进行了比较。基于文化的方法。使用。使用FCM和EFM的荧光标记法,a啶橙(AO)和碘化丙啶(PI)染料分别测定总细胞浓度和微生物活力。结果表明,使用FCM确定的总细胞浓度在统计学上高于使用EFM确定的总细胞浓度(2.62-4.94倍)。差异可能是由于EFM所需的大量准备工作引起的细胞损失。此外,EFM和FCM在总细胞浓度和生存力上都高度相关。 FCM测量的生存力最高,而培养物测量的生存力最低。此外,使用基因探针通过实时qPCR测量的DNA浓度与通过EFM或FCM测量的总浓度高度相关。总之,此处比较的三种非培养方法可提供有关微生物浓度和生存力的快速准确信息。

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