Genetic Relationships among Rehmannia glutinosa Cultivars and Varieties

 

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Abstract

Many cultivars of Rehmannia glutinosa are grown in China for medicinal uses, but detailed agronomic and morphological descriptions are available for only a few. Knowledge of genetic relationships among most of the cultivars is also scanty and poorly documented. Here, cultivars, varieties and some sexually produced seeds of R. glutinosa were raised in the field and studied for morphological diversity including shape, color, edges of leaves, color of anther, cornal and root, as well as yield of the medicinal part of the roots. Random amplified polymorphism DNA (RAPD) and amplified fragment length polymorphism (AFLP) were used to determine genetic relationships and ribosome DNA internal transcribed spacer (ITS) sequences were used for analyzing sequence variations and phylogenetic history. The 118 and 1019 polymorphic markers produced by 10 RAPD and 8 AFLP primers discriminated cultivars and varieties satisfactorily. Sixty-eight accessions were clustered in three main groups at 0.69 similarity levels by unweighted pair-group method arithmetic average (UPGMA) cluster analysis using RAPD in combination with AFLP markers. The average polymorphism information content (PIC) and Shannon index were 0.438 and 2.19 in RAPD and 0.476 and 26.68 in AFLP primers, respectively. This indicates that AFLP markers would be more efficient than RAPD for screening large numbers of R. glutinosa accessions. The analysis of ITS sequences indicated that ITS1 – 5.8S-ITS2 of R. glutinosa was informative in its 611 – 614-bp-long sequence and had 106 variable sites. Phylogenetic trees generated based on ITS sequences as well as the dendrogram obtained from two molecular markers identified four accessions: BY3, BY5, BY6 and Wildness6, with great genetic divergence.

References

• 1 Yan K, Zhao L, Li Q H. Systematic relationships among Rehmannia species.  Acta Bot Boreali-Occidentalia Sin. 2007;  27 1112-20
  PubMedGoogle Scholar
• 2 Chen J J, Devanand P S, Norman D J, Henny R J, Chao C T. Genetic relationships of Aglaonema species and cultivars inferred from AFLP markers.  Ann Bot. 2004;  93 157-66
  CrossrefPubMedGoogle Scholar
• 3 Karol M, Juidita L, Marian P, Walter B. Comparative ITS and AFLP analysis of diploid Cardamine (Brassicaceae) taxa from closely related polyploidy complexes.  Ann Bot. 2004;  93 507-20
  CrossrefPubMedGoogle Scholar
• 4 Li X, Ding X, Chu B, Zhou Q, Ding G, Gu S. Genetic diversity analysis and conservation of the endangered Chinese endemic herb Dendrobium officinale Kimuraet Migo based on AFLP.  Genetica. 2008;  133 159-66
  CrossrefPubMedGoogle Scholar
• 5 Ni X, Huang Y, Wu L, Zhou R, Deng S, Wu D. et al . Genetic diversity of the endangered Chinese endemic herb Primulina tabacum revealed by AFLP.  Genetica. 2006;  127 177-83
  CrossrefPubMedGoogle Scholar
• 6 Williams J G, Kubelik A R, Livak K J, Rafalski J A, Tingey S V. DNA polymorphism amplified by arbitrary primers are useful as genetic markers.  Nucleic Acids Res. 1991;  18 6531-5
  PubMedGoogle Scholar
• 7 Vos P, Hogers R, Bleeker M, Vande Lee T, Hornes M, Frijters A. et al . AFLP a new technique for DNA fingerprinting.  Nucleic Acids Res. 1995;  23 4407-14
  PubMedGoogle Scholar
• 8 Roy A, Bandyopadhyay A, Mahapatra A K, Ghosh S K, Singh N K, Bansal K C. et al . Evaluation of genetic diversity in jute (Corchorus species ) using STMS, ISSR and RAPD markers.  Plant Breed. 2006;  125 292-7
  CrossrefPubMedGoogle Scholar
• 9 Kumar S, Tamura K, Nei M. MEGA3: intergrated software for molecular evolutionary genetics analysis and sequence alignment.  Brief Bioinform. 2004;  5 150-63
  CrossrefPubMedGoogle Scholar
• 10 Karp A, Seberg O, Buiatti M. Molecular techniques in the assessment of botanical diversity.  Ann Bot. 1996;  78 143-9
  CrossrefPubMedGoogle Scholar
• 11 Hodkinson T R, Chase M W, Renvoize S A. Characterization of a genetic resource collection for Miscanthus using AFLP and ISSR PCR.  Ann Bot. 2002;  89 627-36
  CrossrefPubMedGoogle Scholar
• 12 Scariot V, Keyser D E, Handa T, Riek D e. Comparative study of the discriminating capacity and effectiveness of AFLP, STMS and EST markers in assessing genetic relationship among evergreen azaleas.  Plant Breed. 2007;  126 207-12
  CrossrefPubMedGoogle Scholar
• 13 Carr J, Korban S S. Evaluating genetic relationships in seed impatiens, Impatiens walleriana, using AFLP profiling.  Plant Breed. 2004;  123 577-81
  CrossrefPubMedGoogle Scholar
• 14 Wang C Z, Li P, Ding J Y, Jin G Q, Yuan C S. Identification of Fritillaria pallidiflora using diagnostic PCR and PCR-RFLP based on nuclear ribosomal DNA internal transcribed spacer sequences.  Planta Med. 2005;  71 384-6
  Article in Thieme ConnectPubMedGoogle Scholar
• 15 Xue H G, Zhou S D, He X J, Yu Y. Molecular authentication of the traditional Chinese medicinal plant Euphorbia pekinensis. .  Planta Med. 2007;  73 91-3
  Article in Thieme ConnectPubMedGoogle Scholar
• 16 Xue H G, Zhou S D, He X J, Yu Y. Molecular authentication of the traditional dai medicinal plant Croton caudate. .  . 2007;  73 611-3
  Article in Thieme ConnectPubMedGoogle Scholar
• 17 Chiou S J, Yen J H, Fang C L, Chen H L, Lin T Y. Authentication of medicinal herbs using PCR-amplified ITS2 with specific primers.  Planta Med. 2007;  73 1421-6
  Article in Thieme ConnectPubMedGoogle Scholar
• 18 Baldwin B G. Phylogenetic utility of the internal transcribed spacers of nuclear ribosomal DNA in plants: an example from the Compositae.  Mol Phylogenet Evol. 1992;  1 3-16
  CrossrefPubMedGoogle Scholar
• 19 Sonnante G, Galasso I, Pignone D. ITS sequence analysis and phylogenetic inference in the genus Lens Mill.  Ann Bot. 2003;  91 49-54
  CrossrefPubMedGoogle Scholar

Prof. Dr. Xiaojun Ma

Institute of Medicinal PlantsDevelopment

Peking Union Medical College

Chinese Academy of Medical Sciences

Beijing 100193

People’s Republic of China

Phone: +86-10-6281-0019

Fax: +86-10-6289-6313

Email: xiaojunma001@hotmail.com

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