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实时 PCR 检测和定量检测蜡样芽胞杆菌组物种的方法的建立:从牛奶中区分魏氏芽孢杆菌和根状芽孢杆菌的分离株。

Development of real-time PCR assays for detection and quantification of Bacillus cereus group species: differentiation of B. weihenstephanensis and rhizoid B. pseudomycoides isolates from milk.

机构信息

Department of Chemical and Environmental Sciences, University of Limerick, Limerick, Ireland.

出版信息

Appl Environ Microbiol. 2011 Jan;77(1):80-8. doi: 10.1128/AEM.01581-10. Epub 2010 Nov 5.

Abstract

Quantitative real-time PCR (qRT-PCR) offers an alternative method for the detection of bacterial contamination in food. This method provides the quantitation and determination of the number of gene copies. In our study, we established an RT-PCR assay using the LightCycler system to detect and quantify the Bacillus cereus group species, which includes B. cereus, B. anthracis, B. thuringiensis, B. weihenstephanensis, B. mycoides, and B. pseudomycoides. A TaqMan assay was designed to detect a 285-bp fragment of the motB gene encoding the flagellar motor protein, which was specific for the detection of the B. cereus group species, excluding B. pseudomycoides, and the detection of a 217-bp gene fragment of a hypothetical protein specific only for B. pseudomycoides strains. Based on three hydrolysis probes (MotB-FAM-1, MotB-FAM-2, and Bpm-FAM-1), it was possible to differentiate B. weihenstephanensis from the B. cereus group species with nonrhizoid growth and B. pseudomycoides from the whole B. cereus group. The specificity of the assay was confirmed with 119 strains belonging to the Bacillus cereus group species and was performed against 27 other Bacillus and non-Bacillus bacteria. A detection limit was determined for each assay. The assays performed well not only with purified DNA but also with DNA extracted from milk samples artificially contaminated with bacteria that belong to the B. cereus group species. This technique represents an alternative approach to traditional culture methods for the differentiation of B. cereus group species and differentiates B. weihenstephanensis and B. pseudomycoides in one reaction.

摘要

实时荧光定量 PCR(qRT-PCR)为检测食品中的细菌污染提供了一种替代方法。该方法提供了定量和基因拷贝数的测定。在我们的研究中,我们使用 LightCycler 系统建立了 RT-PCR 检测方法,以检测和定量包括芽孢杆菌、炭疽芽孢杆菌、苏云金芽孢杆菌、魏氏芽孢杆菌、蕈状芽孢杆菌和假蕈状芽孢杆菌在内的芽孢杆菌群物种。设计了 TaqMan 检测法来检测编码鞭毛运动蛋白的 motB 基因的 285-bp 片段,该检测法特异性地检测芽孢杆菌群物种,不包括假蕈状芽孢杆菌,并且只检测假蕈状芽孢杆菌菌株特有的 217-bp 基因片段。基于三个水解探针(MotB-FAM-1、MotB-FAM-2 和 Bpm-FAM-1),可以将非根状生长的魏氏芽孢杆菌与芽孢杆菌群物种区分开来,将假蕈状芽孢杆菌与整个芽孢杆菌群区分开来。该检测法的特异性通过 119 株属于芽孢杆菌群物种的菌株得到了确认,并与 27 株其他芽孢杆菌和非芽孢杆菌进行了比较。确定了每个检测法的检测限。该检测法不仅可以很好地用于纯化 DNA,也可以用于从人工污染细菌的牛奶样本中提取的 DNA。该技术代表了传统培养方法的替代方法,用于区分芽孢杆菌群物种,并在一个反应中区分魏氏芽孢杆菌和假蕈状芽孢杆菌。

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