牛蒡(Arctium lappa Linn)的PCR测序鉴定与鉴定

Hui-Jen Chang , Wan-Ting Huang , Der-An Tsao , Kuo-Ming Huang , Shih-Chiang Lee , Shiu-Ru Lin , Shu-Chun Yang , Ching-Sheng Yeh
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引用次数: 7

摘要

传统的中草药视觉识别方法是不客观的。分子生物学技术可用于准确鉴定每种草药的来源。这可以进一步纯化和控制重要的草药物种。利用聚合酶链反应和测序等分子技术,在物种水平上对牛蒡进行相对简单和客观的鉴定。结果表明,6个牛蒡品种的ITS1-5.8S rRNA-ITS2序列长度为358碱基对(bp),分别为:坪东盖来、总雪、日本、凤山、Wholesaler和台南。自动测序分析发现,屏东鬼来和日本品种ITS DNA序列相同,而一般雪品种与它们在277 bp处存在差异。本研究利用DNA测序技术,分析了原产于台湾不同地区的A. lappa Linn ITS的高特异性区域,发现了277 bp位置的品种鉴定单核苷酸多态性,用于局部分化。
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Identification and Authentication of Burdock (Arctium lappa Linn) Using PCR Sequencing

The traditional visual identification of Chinese herbs is not objective. Molecular biological techniques can be used to accurately identify the origin of each herbal species. This can enable the further purification and control of important herbal species. Molecular techniques involving polymerase chain reaction and sequencing were used to provide a relatively simple and objective means of identifying burdock at the species level. This study proved that the length of the ITS1–5.8S rRNA-ITS2 sequence was 358 base-pairs (bp) for six types of Arctium lappa Linn (the following breeds: Pingtung Gueilai, General Snow, Japanese, Fengshan, Wholesaler, and Tainan). Automatic sequencing analysis found that ITS DNA sequences for Pingtung Gueilai and Japanese breeds were the same, and the General Snow breed differed from them at its 277 bp. This study used DNA sequencing to analyze the high specificity regions of A. lappa Linn ITS, originated in different parts of Taiwan, and discovered the breed identification single-nucleotide polymorphism at the 277 bp position for local differentiation.

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