Tanabe Soichi, Miyauchi Eiji, Muneshige Akemi, Mio Kazuhiro, Sato Chikara, Sato Masahiko
Graduate School of Biosphere Science, Hiroshima University, Higashi-hiroshima, Hiroshima, Japan.
Biosci Biotechnol Biochem. 2007 Jul;71(7):1663-7. doi: 10.1271/bbb.70075. Epub 2007 Jul 7.
A PCR method to detect porcine DNA was developed for verifying the allergen labeling of foods and for identifying hidden pork ingredients in processed foods. The primer pair, F2/R1, was designed to detect the gene encoding porcine cytochrome b for the specific detection of pork with high sensitivity. The amplified DNA fragment (130 bp) was specifically detected from porcine DNA, while no amplification occurred with other species such as cattle, chicken, sheep, and horse. When the developed PCR method was used for investigating commercial food products, porcine DNA was clearly detected in those containing pork in the list of ingredients. In addition, 100 ppb of pork in heated gyoza (pork and vegetable dumpling) could be detected by this method. This method is rapid, specific and sensitive, making it applicable for detecting trace amounts of pork in processed foods.
开发了一种用于检测猪DNA的PCR方法,以验证食品的过敏原标签,并识别加工食品中隐藏的猪肉成分。引物对F2/R1被设计用于检测编码猪细胞色素b的基因,以高灵敏度特异性检测猪肉。从猪DNA中特异性检测到扩增的DNA片段(130 bp),而在牛、鸡、羊和马等其他物种中未发生扩增。当使用开发的PCR方法调查商业食品时,在成分列表中含有猪肉的食品中清晰地检测到了猪DNA。此外,该方法可以检测出加热后的饺子(猪肉蔬菜馅)中100 ppb的猪肉。该方法快速、特异且灵敏,适用于检测加工食品中的微量猪肉。
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