Fajardo Violeta, González Isabel, Martín Irene, Rojas María, Hernández Pablo E, García Teresa, Martín Rosario
Universidad Complutense, Facultad de Veterinaria, Departamento de Nutrición, Bromatología y Tecnología de los Alimentos, 28040 Madrid, Spain.
J AOAC Int. 2008 Jan-Feb;91(1):103-11.
A real-time quantitative polymerase chain reaction (PCR) technique was developed for the quantification of chamois and pyrenean ibex DNAs in meat mixtures by using a SYBR green detection platform. Two species-specific systems and a eukaryotic endogenous system were combined in the real-time PCR approach to quantify the target species. In the specific systems, a 133 base pair (bp) fragment of the 12S rRNA gene was amplified from chamois DNA, and an 88 bp fragment from the D-loop region was amplified from pyrenean ibex DNA. In the endogenous system, universal primers amplified a 141 bp fragment on the nuclear 18S rRNA gene from eukaryotic DNA. The threshold cycle values obtained with the 18S rRNA primers were used to normalize those obtained from chamois- or pyrenean ibex-specific systems, serving as endogenous control for the total content of PCR-amplifiable DNA in the sample. Analysis of experimental raw and heat-treated binary mixtures of chamois and pyrenean ibex meat in a swine meat matrix demonstrated the suitability of the assay for the detection and quantification of the target DNAs in the range of 0.1-0.8%, depending on the species and treatment of the meat samples.
开发了一种实时定量聚合酶链反应(PCR)技术,通过使用SYBR Green检测平台来定量肉混合物中的羚羊和比利牛斯山羊DNA。在实时PCR方法中,将两个物种特异性系统和一个真核生物内源性系统结合起来,以定量目标物种。在特异性系统中,从羚羊DNA中扩增出12S rRNA基因的133个碱基对(bp)片段,从比利牛斯山羊DNA中扩增出D-loop区域的88 bp片段。在内源性系统中,通用引物从真核生物DNA的核18S rRNA基因上扩增出141 bp片段。用18S rRNA引物获得的阈值循环值用于对从羚羊或比利牛斯山羊特异性系统获得的值进行标准化,作为样品中可PCR扩增DNA总含量的内源性对照。对猪肉馅中羚羊和比利牛斯山羊肉的实验生肉和热处理二元混合物的分析表明,该检测方法适用于检测和定量0.1%-0.8%范围内的目标DNA,具体取决于肉样品的物种和处理方式。