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Selection of Fluorescent Probes for Flow Cytometric Viability Assessment of Listeria monocytogenes Exposed to Membrane-Active and Oxidizing Disinfectants

机译:用于暴露于膜活性和氧化性消毒剂的单核细胞增生性李斯特菌流式细胞术可行性评估的荧光探针的选择

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The aim of this study was to select fluorescence methods for use as alternatives to plate counting to assess the viability of Listeria monocytogenes cells exposed to benzalkonium chloride (BAC) and hydrogen peroxide, two disinfectants with different mechanisms of action. A further aim of this study was to determine whether growth phase influences fluorescence labeling and whether it is possible to predict whether a probe will be a good viability indicator for cells exposed to a certain disinfectant on the basis of the mechanism of action of the disinfectant and the target of the fluorescent probe. The fluorescence methods used were labeling with 5-cyano-2,3-ditolyl tetrazolium chloride (CTC; dehydrogenase activity), labeling with TOTO-1 iodide (TOTO; membrane-impermeant probe), and assessment of pH gradient maintenance in a low-pH buffer after labeling with the pH-sensitive probe 5-(and 6)-carboxyfluorescein succinimidyl ester (CFSE) (the pH_(in) method). Growth phase influenced fluorescent labeling. However, the cutoff value for distinction between viable and nonviable cells was the same for both growth phases. The viability (determined by plate counts) of BAC-exposed cells correlated well with CTC labeling and TOTO exclusion. For both BAC-exposed and hydrogen peroxide-exposed cells, the pH_(in) method gave a good qualitative indication of viability, sublethal damage, and cell death. CTC labeling and TOTO exclusion did not correlate with the viability of hydrogen peroxide-exposed cells. Our results demonstrate that even if the mechanism of action of a disinfectant is known, in some cases it is still difficult to predict whether a certain fluorescent probe is suitable for viability assessment. Thus, the proper selection of fluorescent probes for the assessment of the efficacy of antimicrobial agents is essential.
机译:这项研究的目的是选择荧光方法作为板计数的替代方法,以评估暴露于两种作用机理不同的苯扎氯铵(BAC)和过氧化氢的单核细胞增生李斯特菌细胞的活力。这项研究的另一个目的是根据消毒剂的作用机理和作用机理,确定生长阶段是否会影响荧光标记,以及是否有可能预测探针对于暴露于某种消毒剂的细胞是否是良好的生存力指标。荧光探针的目标。所使用的荧光方法是用5-氰基2,3-二甲苯基氯化四唑(CTC;脱氢酶活性)标记,用TOTO-1碘化物(TOTO;膜不渗透探针)标记以及在低浓度条件下评估pH梯度维持用pH敏感探针5-(和6)-羧基荧光素琥珀酰亚胺酯(CFSE)标记后的pH缓冲液(pH_(in)方法)。生长期影响荧光标记。但是,在两个生长期,区分活细胞和非活细胞的临界值是相同的。 BAC暴露的细胞的生存能力(由板数确定)与CTC标记和TOTO排除密切相关。对于暴露于BAC的细胞和暴露于过氧化氢的细胞,pH_(in)方法都可以很好地定性显示存活力,亚致死性损伤和细胞死亡。 CTC标记和TOTO排除与暴露于过氧化氢的细胞的活力无关。我们的结果表明,即使已知消毒剂的作用机理,在某些情况下仍然很难预测某种荧光探针是否适合进行生存力评估。因此,正确选择荧光探针以评估抗微生物剂的功效至关重要。

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