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首页> 外文期刊>Applied and Environmental Microbiology >A PCR-based assay for the detection of Escherichia coli Shiga-like toxin genes in ground beef.
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A PCR-based assay for the detection of Escherichia coli Shiga-like toxin genes in ground beef.

机译:基于PCR的检测牛肉中大肠杆菌志贺样毒素基因的检测方法。

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摘要

A detection system based on the PCR has been developed for Escherichia coli strains which harbor the Shiga-like toxin genes. This quantitative detection system involves the 5'-->3' nuclease activity of Thermus aquaticus DNA polymerase, which cleaves an internal oligonucleotide probe that has been labeled with both a fluorescent reporter dye (6-carboxy-fluorescein [FAM]) and a quencher dye (6-carboxytetramethyl-rhodamine [TAMRA]). Parameters which affected the performance of the assay included primer probe distance, probe concentration, and probe target sequence homology. The optimized assay format includes two PCR primers that generate a 497-bp amplicon specific for the sltI gene with the fluorogenic probe located 19 bp from the upstream PCR primer. When the distance between the upstream PCR primer and the probe was reduced from 190 to 19 bp, delta RQ values increased from approximately 1.5 to 3.0. The delta RQ for Shiga-like toxin I probe 102 reached a maximum of 4.15 at concentrations between 25 and 50 nM. The assay is sensitive and can detect approximately 10 +/- 5 CFU per PCR. As few as 0.5 CFU of Shiga-like toxin I-producing E. coli per g could be detected in ground beef with only 12 h of enrichment in modified E. coli broth.
机译:已开发出基于PCR的检测系统,用于带有志贺样毒素基因的大肠杆菌菌株。此定量检测系统涉及水生栖热菌DNA聚合酶的5'-> 3'核酸酶活性,该酶裂解内部的寡核苷酸探针,该探针已被荧光报告染料(6-羧基荧光素[FAM])和淬灭剂标记染料(6-羧基四甲基罗丹明[TAMRA])。影响测定性能的参数包括引物探针距离,探针浓度和探针靶序列同源性。优化的分析形式包括两个PCR引物,它们产生一个sltI基因特异的497 bp扩增子,其中荧光探针位于上游PCR引物19 bp处。当上游PCR引物和探针之间的距离从190 bp减少到19 bp时,ΔRQ值从大约1.5增加到3.0。志贺样毒素I探针102的增量RQ在25至50 nM之间的浓度达到最大值4.15。该测定法灵敏,每个PCR可以检测到大约10 +/- 5 CFU。在绞碎的牛肉中检测到每克只有0.5 CFU的产生志贺样毒素I的大肠杆菌,而在修饰的大肠杆菌肉汤中仅富集了12 h。

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