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Quantification of live and dead probiotic bacteria in lyophilised product by real-time PCR and by flow cytometry

机译:通过实时PCR和流式细胞仪定量分析冻干产品中的活和死益生菌

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The basic requirement for probiotic bacteria to be able to exert expected positive effects is to be alive; therefore, appropriate quantification methods are crucial. Due to disadvantages of conventional microbiological methods, the bacterial quantification based on the nucleic acid detection is increasingly used. The objective of this study was to evaluate the possibility to use propidium monoazide (PMA) in combination with real-time polymerase chain reaction (PCR) method or LIVE/DEAD BacLight viability kit in combination with flow cytometry (FCM) for determination of probiotic bacteria in a lyophilised product containing Lactobacillus acidophilus LA-5 and Bifidobacterium animalis ssp. lactis BB-12. In addition, the viability of probiotic bacteria in lyophilised product during 3 months storage was investigated. In the product, the results of real-time PCR quantification of PMA-treated cells did not differ significantly from those of non-treated cells, which indicate that most of the bacterial cells retained the membrane integrity although they have lost the culturability. The results obtained by FCM analysis were comparable with those by PMA real-time PCR. In conclusion, the PMA real-time PCR and FCM determination of the viability of probiotic bacteria could complement the plate count method which considers only the culturable part of the population.
机译:益生菌能够发挥预期的积极作用的基本要求是活着。因此,适当的量化方法至关重要。由于常规微生物学方法的缺点,越来越多地使用基于核酸检测的细菌定量。这项研究的目的是评估将单叠氮化丙锭(PMA)与实时聚合酶链反应(PCR)方法结合使用或将LIVE / DEAD BacLight生存力试剂盒与流式细胞仪(FCM)结合用于确定益生菌的可能性含有嗜酸乳杆菌LA-5和动物双歧杆菌ssp的冻干产物中的糖。乳酸菌BB-12。另外,研究了冻干产品在3个月的储存过程中益生菌的生存能力。在该产品中,PMA处理的细胞的实时PCR定量结果与未处理的细胞没有显着差异,这表明大多数细菌细胞尽管失去了可培养性,但仍保持了膜的完整性。通过FCM分析获得的结果与通过PMA实时PCR获得的结果相当。总之,通过PMA实时PCR和FCM测定益生菌的活力可以补充仅考虑人群可培养部分的平板计数法。

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