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Molecular identification of pufferfish species using PCR amplification and restriction analysis of a segment of the 16S rRNA gene

机译:河豚的分子识别的物种限制使用PCR扩增和分析一段16 s rRNA的基因

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This study amplified the mitochondrial 16S rRNA gene using polymerase chain reaction (PCR) with a template of total DNA from muscle tissues of nine pufferfish species collected from the coastal area of Okinawa Islands in Japan: Pleuranacanthus sceleratus, Triodon macropterus, Chelonodon patoca, Sphoeroides pachygaster, Arothron hispidus, A. stellatus, A. manilensis, A. mappa, and A. nigropunctatus. Then nucleotide sequence encoding a partial region of the 16S rRNA gene was compared among species. The sequenced fragment was also used to select restriction enzymes, yielding species-specific restriction fragment length polymorphisms (RFLP). The sequence of the segment of the 16S rRNA gene consisted of about 615 nucleotides and showed interspecies variations in the targeted region. After calculation of corresponding RFLP-patterns of nine species investigated with suitable restriction enzymes, three restriction enzymes BanII, DdeI, and NlaIII - were found to be sufficient for identification of all nine species. Successful testing of this methodology in frozen and heated food samples suggests its utility for pufferfish species authentication in food products. (c) 2005 Elsevier Inc. All rights reserved.
机译:本研究放大线粒体16 s rRNA基因用聚合酶链反应(PCR)模板总DNA的肌肉组织的9河豚从沿海收集的物种在日本冲绳群岛面积:Pleuranacanthussceleratus, Triodon macropterus ChelonodonA . stellatus, hispidus manilensis, A .地图,和a . nigropunctatus。编码的部分地区16 s rRNA基因物种之间的比较。碎片也被用于选择限制酶,产生特有的限制片段长度多态性(RFLP)。16 s rRNA基因的部分序列由大约615个核苷酸和显示目标地区的种间差异。计算相应的RFLP-patterns之后九种与合适的调查限制性内切酶,三个限制性内切酶BanII、DdeI NlaIII——被发现满足所有9的识别物种。在冷冻和加热食物样本显示它效用河豚物种认证食品产品。保留。

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