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Detection of Salmonella Typhimurium and Listeria monocytogenes biofilm cells exposed to different drying and pre-enrichment times using conventional and rapid methods

机译:使用常规和快速方法检测沙门氏菌毒蕈氏菌和李斯特里亚单核细胞增生生物膜细胞的不同干燥和预富集时间

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摘要

The capacity of real-time PCR (RT-PCR), the VIDAS immunoassay system, and the conventional count method for detecting Salmonella enterica serovar Typhimurium and Listeria monocytogenes biofilm cells was evaluated in this study. After biofilm formation, tests were performed under different drying times (0, 6, 12, 24, and 72 h) and pre-enrichment times (0, 6, 18, and 25 h). The direct epifluorescence microscopic results demonstrated that Salmonella Typhimurium and L. monocytogenes biofilm cells can remain viable for 72 h under drying conditions. Pre-enrichment time and type of medium played an essential role in the detection of both microorganisms after drying. Furthermore, RT-PCR was more sensitive than VIDAS and the conventional method for detecting Salmonella Typhimurium and L. monocytogenes cells at different drying times and without pre-enrichment (0 h), with a detection range between 102 and 107 CFU/mL. TSBYE-T80 used as a pre-enrichment medium was effective for detecting both bacteria and was more effective than Demi Fraser-T80 medium for detecting L. monocytogenes. Therefore, pre-enrichment is recommended to avoid false positives and false negatives due to the presence of dead cells or a very low initial concentration of cells after drying.
机译:在本研究中评估了该研究的实时PCR(RT-PCR),VIDA免疫测定系统和常规计数方法,用于检测沙门氏菌肠道血硫伞和李斯特菌单核细胞瘤李斯特菌的李斯特菌菌细胞瘤细胞。在生物膜形成后,在不同的干燥时间(0,6,12,24和72小时)和预富集时间(0,6,18和25小时)进行试验。直接渗流性微观结果证明,在干燥条件下,沙门氏菌毒蕈氏菌和L.单核细胞质生物膜细胞可以保持72小时可行。富集时间和培养基类型在干燥后检测到两种微生物中起重要作用。此外,RT-PCR比Vidas更敏感,并且在不同干燥时间和无预富集(0h)的情况下检测沙门氏菌毛刺和L.单核细胞增生细胞的常规方法,其中检测范围在102和107cfu / ml之间。用作预富集培养基的TSBye-T80对于检测两种细菌有效,并且比Demi Fraser-T80培养基更有效,用于检测L.单核细胞增生。因此,建议预富集以避免由于死细胞存在或干燥后细胞的非常低的初始浓度导致的假阳性和假阴性。

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