INRA, UR342 Technologie et Analyses Laitières, BP 20089, F-39800 Poligny, France.
Food Microbiol. 2013 Dec;36(2):286-95. doi: 10.1016/j.fm.2013.06.024. Epub 2013 Jul 6.
The first objective of this work was to develop real-time quantitative PCR (qPCR) assays to quantify two species of mesophilic lactic acid bacteria technologically active in food fermentation, including cheese making: Lactococcus lactis and Lactobacillus paracasei. The second objective was to compare qPCR and plate counts of these two species in cheese samples. Newly designed primers efficiently amplified a region of the tuf gene from the target species. Sixty-three DNA samples from twenty different bacterial species, phylogenetically related or commonly found in raw milk and dairy products, were selected as positive and negative controls. Target DNA was successfully amplified showing a single peak on the amplicon melting curve; non-target DNA was not amplified. Quantification was linear over 5 log units (R(2) > 0.990), down to 22 gene copies/μL per well for Lc. lactis and 73 gene copies/μL per well for Lb. paracasei. qPCR efficiency ranged from 82.9% to 93.7% for Lc. lactis and from 81.1% to 99.5% for Lb. paracasei. At two stages of growth, Lc. lactis was quantified in 12 soft cheeses and Lb. paracasei in 24 hard cooked cheeses. qPCR proved to be useful for quantifying Lc. lactis, but not Lb. paracasei.
这项工作的首要目标是开发实时定量 PCR(qPCR)分析方法,以定量两种在食品发酵(包括奶酪制作)中具有技术活性的嗜温性乳酸菌:乳球菌和副干酪乳杆菌。第二个目标是比较奶酪样品中这两种菌的 qPCR 和平板计数。新设计的引物有效地扩增了目标物种 tuf 基因的一个区域。从 20 个不同的细菌物种中选择了 63 个 DNA 样本,这些细菌物种在进化上相关或常见于生乳和乳制品中,作为阳性和阴性对照。目标 DNA 成功扩增,在扩增子熔解曲线中显示出单个峰值;非目标 DNA 未扩增。定量线性范围为 5 个对数单位(R(2)>0.990),对于 Lc. lactis ,每个孔 22 个基因拷贝/μL,对于 Lb. paracasei ,每个孔 73 个基因拷贝/μL。qPCR 效率对于 Lc. lactis 范围为 82.9%至 93.7%,对于 Lb. paracasei 范围为 81.1%至 99.5%。在两个生长阶段,12 种软奶酪中定量了 Lc. lactis,24 种硬熟奶酪中定量了 Lb. paracasei。qPCR 被证明可用于定量 Lc. lactis,但不能定量 Lb. paracasei。
