Authentication of Medicinal Herbs using PCR-Amplified ITS2 with Specific Primers

Abstract Different parts of medicinal herbs have long been used as traditional Chinese drugs for treating many diseases, whereas materials of similar morphology and chemical fingerprints are often misidentified. Analyses of sequence variations in the nuclear ribosomal DNA (rDNA) internal transcribed...

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Veröffentlicht in:Planta medica 2007-10, Vol.73 (13), p.1421-1426
Hauptverfasser: Chiou, S.J, Yen, J.H, Fang, C.L, Chen, H.L, Lin, T.Y
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container_end_page 1426
container_issue 13
container_start_page 1421
container_title Planta medica
container_volume 73
creator Chiou, S.J
Yen, J.H
Fang, C.L
Chen, H.L
Lin, T.Y
description Abstract Different parts of medicinal herbs have long been used as traditional Chinese drugs for treating many diseases, whereas materials of similar morphology and chemical fingerprints are often misidentified. Analyses of sequence variations in the nuclear ribosomal DNA (rDNA) internal transcribed spacer (ITS) have become a valid method for authentication of medicinal herbs at the intergenic and interspecific levels. DNA extracted from processed materials is usually severely degraded or contaminated by microorganisms, thus generates no or unexpected PCR products. The goal of this study is to apply the ITS fragments selectively amplified with two designed primer sets for efficient and precise authentication of medicinal herbs. The designed primers led to an accurate PCR product of the specific region in ITS2, which was confirmed with DNA extracted from 55 processed medicinal herbs belonging to 48 families. Moreover, the selectively amplified ITS2 authenticated five sets of easily confusable Chinese herbal materials. The designed primers were proven to be suitable for a broad application in the authentication of herbal materials.
doi_str_mv 10.1055/s-2007-990227
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Analyses of sequence variations in the nuclear ribosomal DNA (rDNA) internal transcribed spacer (ITS) have become a valid method for authentication of medicinal herbs at the intergenic and interspecific levels. DNA extracted from processed materials is usually severely degraded or contaminated by microorganisms, thus generates no or unexpected PCR products. The goal of this study is to apply the ITS fragments selectively amplified with two designed primer sets for efficient and precise authentication of medicinal herbs. The designed primers led to an accurate PCR product of the specific region in ITS2, which was confirmed with DNA extracted from 55 processed medicinal herbs belonging to 48 families. Moreover, the selectively amplified ITS2 authenticated five sets of easily confusable Chinese herbal materials. 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subjects Biochemistry and Molecular Biology
Biological and medical sciences
DNA Primers
DNA, Plant - analysis
DNA, Ribosomal Spacer - analysis
Drugs, Chinese Herbal - analysis
General pharmacology
Humans
internal transcribed spacers
Medical sciences
medicinal plants
Pharmacognosy. Homeopathy. Health food
Pharmacology. Drug treatments
Phytotherapy - standards
plant taxonomy
Plants, Medicinal - genetics
Polymerase Chain Reaction
product authenticity
title Authentication of Medicinal Herbs using PCR-Amplified ITS2 with Specific Primers
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