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Targeting double genes in multiplex PCR for discriminating bovine, buffalo and porcine materials in food chain

机译:用于鉴别牛,水牛和猪材的多重PCR中的双基因靶向食物链中的多重PCR

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Beef, buffalo and pork are the major meat of economic, religious and health concern. Current methods to authenticate these materials in food chain are based on mainly single gene targets which are susceptible to break down by food processing treatments. We, for the first time, described here a double gene targeting short-amplicon length multiplex polymerase chain reaction assay for discriminating bovine, buffalo and porcine materials in a single assay platform. The advantage of the assay is evidenced in terms of fidelity, cost and time since it is highly unlikely that two different targets would be missing even in a decomposed specimen. Detection of multiple targets in a single assay definitely saves analytical cost and time. Mitochondrial cytochrome b (cytb) and ND5 genes were targeted and six different targets (length: 90-146 bp), two for each of cow (120 and 106bp), buffalo (90 and 138bp) and pig (73 and 146bp), were amplified from raw, boiled, autoclaved and microwaved cooked meat under pure and mixed matrices. The detection limit was 0.02 ng DNA under pure states and 0.1% meat in binary mixtures and meatball products. Screening of Malaysian meatball products revealed all beef products were buffalo positive in which 35% were totally replaced. In contrast, all pork products were found uncontaminated from beef and buffalo. (C) 2016 Elsevier Ltd. All rights reserved.
机译:牛肉,水牛和猪肉是经济,宗教和健康问题的主要肉类。验证食物链中这些材料的目前的方法主要是主要的单一基因靶标,易于通过食品加工治疗分解。我们首次描述了靶向短扩增常数多重聚合酶链反应测定的双基因,用于在单一测定平台中鉴别牛,水牛和猪材料。在保真度,成本和时间方面证明了测定的优点,因为即使在分解的标本中也可能缺少两种不同的目标。在单个测定中检测多个目标肯定节省了分析成本和时间。针对线粒体细胞色素B(CytB)和ND5基因靶向,六种不同的靶(长度:90-146bp),每种牛(120和106bp),水牛(90和138bp)和猪(73和146bp)在纯和混合基质下从原料,煮沸,高压灭菌和微波煮熟的肉中放大。检测限为0.02ng DNA在纯态下,二元混合物和肉丸产品中的0.1%肉。马来西亚肉丸产品的筛选揭示了所有牛肉产品是水牛阳性,其中35%完全被替换。相比之下,发现所有猪肉产品都被发现从牛肉和水牛污染。 (c)2016 Elsevier Ltd.保留所有权利。

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