Subscribe to RSS
Download PDF
DOI: 10.1055/s-2003-40632
Authentication of Panax notoginseng by 5S-rRNA Spacer Domain and Random Amplified Polymorphic DNA (RAPD) Analysis
Publication History
Received: October 7, 2002
Accepted: January 25, 2003
Publication Date:
16 July 2003 (online)
Abstract
The great majority of Panax species are well-known herbal medicines in the Orient, and many of them share a close resemblance in appearance and chemical composition. Among these Panax species, the root of P. notoginseng (Sanqi) is a unique herb that has distinct clinical usage. Here, the 5S-rRNA spacer domains were isolated from P. notoginseng, P. japonicus var. major, P. stipuleanatus, P. quinquefolius, P. ginseng, P. zingiberensis, and P. wangianus, and four common adulterants of P. notoginseng including Curcuma wenyujin, Curcuma longa, Bletilla striata and Gynura segetum. The spacer domains were sequenced and compared, which showed over 75 % DNA identity among all Panax species, but not for the adulterants. In addition, random amplification of polymorphic DNA (RAPD) analysis was used to distinguish different members of Panax genus as well as the morphological variants of P. notoginseng. These molecular methods could be used in the authentic identification of P. notoginseng from other Panax species.
References
- 1 Zheng G Z, Yang C R. Biology of Panax notogingseng and its application. Science Press. Beijing, China; 1994: p. 9
MissingFormLabel
- 2 Zheng X Y. Pharmacopoeia of the People's Republic of China. Chemical Industry Press Beijing, China; 2000: p. 180
MissingFormLabel
- 3 Mihalov J J, Mardersian A D, Pierce J C. DNA identification of commercial ginseng samples. J Agric Food Chem. 2000; 48 3744-52
- 4 Cheung K S, Kwan H S, But P P, Shaw P C. Pharmacognostical identification of American and Oriental ginseng roots by genomic fingerprinting using arbitrarily primed polymerase chain reaction (AP-PCR). J Ethnopharmacol. 1994; 42 67-9
- 5 Wen J, Zimmer E A. Phylogeny and biogeography of Panax L. (the ginseng genus, Araliaceae): Inferences from ITS sequences of nuclear ribosomal DNA. Mol Phylogen Evol. 1996; 6 166-77
- 6 Fushimi H, Komatstu K, Isobe M, Namba T. Application of PCR-RFLP and MASA analyses on 18S ribosomal RNA gene sequence for identification of three ginseng drugs. Biol Pharm Bull. 1997; 20 765-9
- 7 Komatsu K, Zhu S, Fushimi H, Qui T K, Cai S, Kadota S. Phylogenetic analysis based on 18S rRNA gene and matK gene sequences of Panax vietnamensis and five related species. Planta Med. 2001; 67 461-5
- 8 Cai Z H, Li P, Dong T TX, Tsim K WK. Molecular diversity of 5S-rRNA spacer domain in Fritillaria species revealed by PCR analysis. Planta Med. 1999; 65 360-4
- 9 Ma X Q, Duan J A, Zhu D Y, Dong T TX, Tsim K WK. Species identification of Huangqi (Radix Astragali) by DNA sequence of its 5S-rRNA spacer domain. Phytochemistry. 2000; 54 363-8
- 10 Ngan F, Shaw P, But P, Wang J. Molecular identification of Panax species. Phytochemistry. 1999; 50 787-91
- 11 Ha W Y, Shaw P C, Liu J, Yau F CF, Wang J. Authenication of Panax ginseng and Panax quinquefolius using amplified fragment length polymorphism (AFLP) and directed amplification of minisatellite region DNA (DAMD). J Agric Food Chem. 2002; 50 1871-5
- 12 Gerlach W L, Dyer T A. Sequence organization of the repeating units in the nucleus of wheat which contain 5S-rRNA genes. Nuclear Acids Res. 1980; 8 4851-65
Dr. Karl W. K. Tsim
Department of Biology
Hong Kong University of Science and Technology
Clear Water Bay Road
Hong Kong SAR
P. R. China
Fax: +(852) 2358-1559
Email: BOTSIM@UST.HK