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Swine-Specific PCR-RFLP Assay Targeting Mitochondrial Cytochrome B Gene for Semiquantitative Detection of Pork in Commercial Meat Products

机译:猪线粒体细胞色素B基因的猪特异性PCR-RFLP检测,用于半定量检测商品肉制品中的猪肉

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Verification of pork adulteration in commercial meat products is increasingly important for the authentication of Halal labels in processed foods. Here, we documented a PCR–restriction fragment length polymorphism (RFLP) assay with high precision and reproducibility for the tracing of porcine DNA in commercial meat products. The assay combined the species-specific primers to selectively amplify a short fragment (109 bp) of porcine cytochrome b gene from a heterogeneous background of genomic DNAs followed by RFLP analysis to authenticate real amplicon. The analysis of PCR products and restriction digests was automated in a chip-based capillary electrophoresis incorporated in Agilent 2100 bioanalyzer. The swine specificity of the assay was checked with 11 different meat-providing animal and fish species. Model experiments, mimicking the processed foods, were performed in binary and ternary mixtures after mechanical grinding and prolonged autoclaving. Finally, four types of the most popular finished meat products (meatball, streaky beacon, frankfurter, and burger) which are prevalent in the Malaysian food market were analyzed in order to verify the assay performance. The assay was sensitive enough to detect 0.0001 ng of swine DNA in pure formats and 0.01% (w/w) spiked pork in extensively processed ternary mixture of pork, beef, and wheat flour.
机译:商用肉制品中猪肉掺假的验证对于认证加工食品中的清真标签越来越重要。在这里,我们记录了PCR限制性片段长度多态性(RFLP)检测方法,该方法具有很高的精确度和可重复性,可用于追踪商品肉产品中的猪DNA。该检测方法结合了物种特异性引物,从基因组DNA的异质背景中选择性扩增了猪细胞色素b基因的短片段(109 bp),然后进行RFLP分析以鉴定真实的扩增子。 PCR产物和限制性酶切产物的分析是在Agilent 2100生物分析仪中基于芯片的毛细管电泳中自动进行的。用11种不同的肉类动物和鱼类检查了猪的特异性。机械研磨和长时间高压灭菌后,以二元和三元混合物的形式进行模拟加工食品的模型实验。最后,分析了马来西亚食品市场上流行的四种最流行的成品肉产品(肉丸,五谷信标,法兰克福啤酒和汉堡),以验证分析性能。该检测方法足够灵敏,可以检测到0.0001 ng纯格式的猪DNA和0.01%(w / w)加标猪肉中的猪肉,牛肉和面粉的三元混合物。

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