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Development of a Flow Cytometric Method To Analyze Subpopulations of Bacteria in Probiotic Products and Dairy Starters

机译:流式细胞术方法的发展以分析益生菌产品和乳制品发酵剂中细菌的亚群

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摘要

Flow cytometry (FCM) is a rapid and sensitive technique that can determine cell numbers and measure various physiological characteristics of individual cells by using appropriate fluorescent probes. Previously, we developed an FCM assay with the viability probes carboxyfluorescein diacetate (cFDA) and TOTO-1 {1′-(4,4,7,7-tetramethyl-4,7-diazaundecamethylene)-bis-4-[3-methyl-2,3dihydro(benzo-1,3-oxazole)-2-methylidene]-1-(3′-trimethylammoniumpropyl)-pyridinium tetraiodide} for (stressed) lactic acid bacteria (C. J. Bunthof, K. Bloemen, P. Breeuwer, F. M. Rombouts, and T. Abee, Appl. Environ. Microbiol. >67:2326-2335, 2001). cFDA stains intact cells with enzymatic activity, and TOTO-1 stains membrane-permeabilized cells. Here we used this assay to study the viability of bacterial suspensions in milk, dairy fermentation starters, and probiotic products. To facilitate FCM analysis of bacteria in milk, a commercially available milk-clearing solution was used. The procedure was optimized to increase the signal-to-noise ratio. FCM enumerations were accurate down to a concentration of 105 cells ml−1. The level of retrieval of Lactobacillus plantarum WCFS 1 suspended in milk was high, and viability was not affected by the procedure. The plate counts for cleared samples of untreated cell suspensions were nearly as high as the total FCM counts, and the correlation was strong (r > 0.99). In dairy fermentation starters and in probiotic products the FCM total cell counts were substantially higher than the numbers of CFU. Three functional populations could be distinguished: culturable cells, cells that are intact and metabolically active but not culturable, and permeabilized cells. The proportions of the populations differed in the products tested. This FCM method provides tools to assess the functionality of different populations in fermentation starters and probiotic products.
机译:流式细胞术(FCM)是一种快速而灵敏的技术,可以通过使用适当的荧光探针确定细胞数并测量单个细胞的各种生理特征。以前,我们开发了具有活力的双乙酸羧荧光素(cFDA)和TOTO-1 {1'-(4,4,7,7-四甲基-4,7-二氮杂双亚甲基)-bis-4- [3-甲基-2,3二氢(苯并-1,3-恶唑)-2-亚甲基] -1-(3'-三甲基铵丙基)-四碘化吡啶(用于应力乳酸菌)(CJ Bunthof,K.Bloemen,P.Breeuwer, FM Rombouts和T. Abee,应用环境微生物学,> 67: 2326-2335,2001)。 cFDA染色具有酶促活性的完整细胞,TOTO-1染色膜通透性细胞。在这里,我们使用这种分析方法来研究牛奶,乳制品发酵起始剂和益生菌产品中细菌悬浮液的生存能力。为了促进牛奶中细菌的FCM分析,使用了市售的牛奶清除溶液。优化程序以增加信噪比。 FCM枚举精确到10 5 个细胞ml -1 。悬浮在牛奶中的植物乳杆菌WCFS 1的回收水平很高,并且存活率不受该程序的影响。未经处理的细胞悬液的清除样品的平板计数几乎与总FCM计数一样高,并且相关性很强(r> 0.99)。在乳制品发酵发酵剂和益生菌产品中,FCM总细胞数大大高于CFU数。可以区分三个功能群体:可培养细胞,完整且具有代谢活性但不可培养的细胞和通透性细胞。所测试产品中人口的比例有所不同。这种FCM方法提供了评估发酵剂和益生菌产品中不同人群功能的工具。

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