首页> 美国卫生研究院文献>Evidence-based Complementary and Alternative Medicine : eCAM >DNA Barcode-Based PCR-RFLP and Diagnostic PCR for Authentication of Jinqian Baihua She (Bungarus Parvus)
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DNA Barcode-Based PCR-RFLP and Diagnostic PCR for Authentication of Jinqian Baihua She (Bungarus Parvus)

机译:基于DNA条码的PCR-RFLP和诊断PCR用于金千百花蛇(Bungarus Parvus)的鉴定

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摘要

We established polymerase chain reaction-restriction fragment length polymorphism (PCR-RFLP) and diagnostic PCR based on cytochrome C oxidase subunit I (COI) barcodes of Bungarus multicinctus, genuine Jinqian Baihua She (JBS), and adulterant snake species. The PCR-RFLP system utilizes the specific restriction sites of SpeI and BstEII in the COI sequence of B. multicinctus to allow its cleavage into 3 fragments (120 bp, 230 bp, and 340 bp); the COI sequences of the adulterants do not contain these restriction sites and therefore remained intact after digestion with SpeI and BstEII (except for that of Zaocys dhumnades, which could be cleaved into a 120 bp and a 570 bp fragment). For diagnostic PCR, a pair of species-specific primers (COI37 and COI337) was designed to amplify a specific 300 bp amplicon from the genomic DNA of B. multicinctus; no such amplicons were found in other allied species. We tested the two methods using 11 commercial JBS samples, and the results demonstrated that barcode-based PCR-RFLP and diagnostic PCR both allowed effective and accurate authentication of JBS.
机译:我们建立了聚合酶链反应-限制性片段长度多态性(PCR-RFLP)和诊断PCR基于Bungarus multicinctus,真正的金千百花蛇(JBS)和掺假蛇种的细胞色素C氧化酶亚基I(COI)条码。 PCR-RFLP系统利用多芽孢杆菌COI序列中SpeI和BstEII的特异性限制性酶切位点,将其切割成3个片段(120bp,230bp和340bp)。掺假物的COI序列不包含这些限制性酶切位点,因此在用SpeI和BstEII消化后仍保持完整(Zaocys dhumnades除外,它们可以切割成120bp和570bp的片段)。为了进行诊断PCR,设计了一对物种特异性引物(COI37和COI337),以从多芽孢杆菌的基因组DNA扩增特异性的300 bp扩增子。在其他盟友物种中未发现此类扩增子。我们使用11个商业JBS样品测试了这两种方法,结果表明基于条形码的PCR-RFLP和诊断PCR都可以有效,准确地验证JBS。

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