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DOI: 10.1055/s-0043-121470
What Else Is in Salviae officinalis folium? Comprehensive Species Identification of Plant Raw Material by DNA Metabarcoding
Publikationsverlauf
received 09. Mai 2017
revised 28. August 2017
accepted 10. Oktober 2017
Publikationsdatum:
17. November 2017 (online)
Abstract
Quality control of drugs consists of identifying the raw material to avoid unwanted admixtures or exchange of material as well as looking for abiotic and biotic contaminations. So far, identity and microbial contamination are analyzed by separate processes and separate methods. Species identification by their DNA (“DNA barcoding”) has the potential to supplement existing methods of identification. The introduction of next-generation sequencing methods offers completely new approaches like the identification of whole communities in one analysis, termed “DNA metabarcoding”. Here we present a next-generation sequencing assessment to identify plants and fungi of two commercial sage samples (Salvia officinalis) using the standard DNA barcoding region “internal transcribed spacer” consisting of internal transcribed spacer 1 and internal transcribed spacer 2, respectively. The main species in both samples was identified as S. officinalis. The spectrum of accompanying plant and fungal species, however, was completely different between the samples. Additionally, the composition between internal transcribed spacer 1 and internal transcribed spacer 2 within the samples was different and demonstrated the influence of primer selection and therefore the need for harmonization. This next-generation sequencing approach does not result in quantitative species composition but gives deeper insight into the composition of additional species. Therefore, it would allow for a better knowledge-based risk assessment than any other method available. However, the method is only economically feasible in routine analysis if a high sample throughput can be guaranteed.
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References
- 1 Sanzini E, Badea M, Santos AD, Restani P, Sievers H. Quality control of plant food supplements. Food Funct 2011; 2: 740-746
- 2 Ouarghidi A, Powell B, Martin GJ, De Boer H, Abbad A. Species substitution in medicinal roots and possible implications for toxicity of herbal remedies in Morocco. Econ Bot 2012; 66: 370-382
- 3 Palhares RM, Goncalves Drummond M, Dos Santos Alves Figueiredo Brasil B. Pereira Cosenza G, das Gracas Lins Brandao M, Oliveira G. Medicinal plants recommended by the world health organization: DNA barcode identification associated with chemical analyses guarantees their quality. PLoS One 2015; 10: e0127866
- 4 Mader E, Ruzicka J, Schmiderer C, Novak J. Quantitative high-resolution melting analysis for detecting adulterations. Anal Biochem 2011; 409: 153-155
- 5 Techen N, Parveen I, Pan Z, Khan IA. DNA barcoding of medicinal plant material for identification. Curr Opin Biotechnol 2014; 25: 103-110
- 6 Schoch CL, Seifert KA, Huhndorf S, Robert V, Spouge JL, Levesque CA, Chen W. Nuclear ribosomal internal transcribed spacer (ITS) region as a universal DNA barcode marker for Fungi. Proc Natl Acad Sci U S A 2012; 109: 6241-6246
- 7 Seifert KA. Progress towards DNA barcoding of fungi. Mol Ecol Resour 2009; 9 (Suppl. 01) 83-89
- 8 Schmidt PA, Bálint M, Greshake B, Bandow C, Römbke J, Schmitt I. Illumina metabarcoding of a soil fungal community. Soil Biol Biochem 2013; 65: 128-132
- 9 Taberlet P, Coissac E, Pompanon F, Brochmann C, Willerslev E. Towards next-generation biodiversity assessment using DNA metabarcoding. Mol Ecol 2012; 21: 2045-2050
- 10 Ivanova NV, Kuzmina ML, Braukmann TWA, Borisenko AV, Zakharov EV. Authentication of herbal supplements using next-generation sequencing. PLoS One 2016; 11: e0156426
- 11 Cheng X, Su X, Chen X, Zhao H, Bo C, Xu J, Bai H, Ning K. Biological ingredient analysis of traditional Chinese medicine preparation based on high-throughput sequencing: the story for Liuwei Dihuang Wan. Sci Rep 2014; 4: 5147
- 12 Coghlan ML, Maker G, Crighton E, Haile J, Murray DC, White NE, Byard RW, Bellgard MI, Mullaney I, Trengove R, Allcock RJN, Nash C, Hoban C, Jarrett K, Edwards R, Musgrave IF, Bunce M. Combined DNA, toxicological and heavy metal analyses provides an auditing toolkit to improve pharmacovigilance of traditional Chinese medicine (TCM). Sci Rep 2015; 5: 17475
- 13 Coghlan ML, Haile J, Houston J, Murray DC, White NE, Moolhuijzen P, Bellgard MI, Bunce M. Deep sequencing of plant and animal DNA contained within traditional Chinese medicines reveals legality issues and health safety concerns. PLoS Genet 2012; 8: e1002657
- 14 Blaalid R, Kumar S, Nilsson RH, Abarenkov K, Kirk PM, Kauserud H. ITS1 versus ITS2 as DNA metabarcodes for fungi. Mol Ecol Resour 2013; 13: 218-224
- 15 China Plant BOL Group. Li DZ, Gao LM, Li HT, Wang H, Ge XJ, Liu JQ, Chen ZD, Zhou SL, Chen SL, Yang JB, Fu CX, Zeng CX, Yan HF, Zhu YJ, Sun YS, Chen SY, Zhao L, Wang K, Yang T, Duan GW. Comparative analysis of a large dataset indicates that internal transcribed spacer (ITS) should be incorporated into the core barcode for seed plants. Proc Natl Acad Sci U S A 2011; 108: 19641-19646
- 16 Wang XC, Liu C, Huang L, Bengtsson-Palme J, Chen H, Zhang JH, Cai D, Li JQ. ITS1: a DNA barcode better than ITS2 in eukaryotes?. Mol Ecol Resour 2015; 15: 573-586
- 17 White TJ, Bruns T, Lee S, Taylor J. Amplification and direct Sequencing of fungal ribosomal RNA Genes for Phylogenetics. In: Innis DH, Gelfand DH, Sninsky JJ, White TJ. eds. PCR Protocols: a Guide to Methods and Applications. New York: Academic Press; 1990: 315-322
- 18 Downie SR, Katz-Downie DS. A molecular phylogeny of Apiaceae subfamily Apioideae: evidence from nuclear ribosomal DNA internal transcribed spacer sequences. Am J Bot 1996; 83: 234-251
- 19 Gobbers E, Fransen K, Oosterlaken T, Janssens W, Heyndrickx L, Ivens T, Vereecken K, Schoones R, van de Wiel P, van der Groen G. Reactivity and amplification efficiency of the NASBA HIV-1 RNA amplification system with regard to different HIV-1 subtypes. J Virol Methods 1997; 66: 293-301
- 20 Pinol J, San Andres V, Clare EL, Mir G, Symondson WOC. A pragmatic approach to the analysis of diets of generalist predators: the use of next-generation sequencing with no blocking probes. Mol Ecol Resour 2014; 14: 18-26
- 21 Lindahl BD, Nilsson RH, Tedersoo L, Abarenkov K, Carlsen T, Kjoller R, Koljalg U, Pennanen T, Rosendahl S, Stenlid J, Kauserud H. Fungal community analysis by high-throughput sequencing of amplified markers – a userʼs guide. New Phytol 2013; 199: 288-299
- 22 Ripp F, Krombholz CF, Liu Y, Weber M, Schafer A, Schmidt B, Koppel R, Hankeln T. All-Food-Seq (AFS): a quantifiable screen for species in biological samples by deep DNA sequencing. BMC Genomics 2014; 15: 639
- 23 Janda JM, Abbott SL. 16S rRNA gene sequencing for bacterial identification in the diagnostic laboratory: pluses, perils, and pitfalls. J Clin Microbiol 2007; 45: 2761-2764
- 24 Jinbo U, Kato T, Ito M. Current progress in DNA barcoding and future implications for entomology. Entomol Sci 2011; 14: 107-124
- 25 Doyle J. DNA Protocols for Plants. In: Hewitt G, Johnston A, Young J. eds. Molecular Techniques in Taxonomy. Berlin: Springer; 1991: 283-285
- 26 Schmiderer C, Lukas B, Novak J. Effect of different DNA extraction methods and DNA dilutions on the amplification success in the PCR of different medicinal and aromatic plants. Z Arznei-Gewurzpfla 2013; 18: 65-72
- 27 Magoc T, Salzberg SL. FLASH: fast length adjustment of short reads to improve genome assemblies. Bioinformatics 2011; 27: 2957-2963
- 28 Goecks J, Eberhard C, Too T, Nekrutenko A, Taylor J. Web-based visual analysis for high-throughput genomics. BMC Genomics 2013; 14: 397
- 29 Huson DH, Mitra S, Ruscheweyh HJ, Weber N, Schuster SC. Integrative analysis of environmental sequences using MEGAN4. Genome Res 2011; 21: 1552-1560
- 30 Ye J, Coulouris G, Zaretskaya I, Cutcutache I, Rozen S, Madden TL. Primer-BLAST: a tool to design target-specific primers for polymerase chain reaction. BMC Bioinformatics 2012; 13: 134