Development of SSR markers and assessment of genetic diversity in medicinal Chrysanthemum morifolium cultivars

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Abstract

Chrysanthemum morifolium, is a well-known flowering plant worldwide, and has a high commercial, floricultural, and medicinal value. In this study, simple-sequence repeat (SSR) markers were generated from EST datasets and were applied to assess the genetic diversity among 32 cultivars. A total of 218 in silico SSR loci were identified from 7300 C. morifolium ESTs retrieved from GenBank. Of all SSR loci, 61.47% of them (134) were hexa-nucleotide repeats, followed by tri-nucleotide repeats (17.89%), di-nucleotide repeats (12.39%), tetra-nucleotide repeats (4.13%), and penta-nucleotide repeats (4.13%). In this study, 17novel EST-SSR markers were verified. Along with 38 SSR markers reportedpreviously, 55 C. morifolium SSR markers were selected for further genetic diversity analysis. PCR amplification of these EST-SSRs produced 1319 fragments, 1306 of which showed polymorphism. The average polymorphism information content of the SSR primer pairs was 0.972 (0.938-0.993), which showed high genetic diversity among C. morifolium cultivars. Based on SSR markers, 32 C. morifolium cultivars were separated into two main groups by partitioning of the clusters usingthe unweighted pair group method with arithmetic mean dendrogram, whichwas further supported by a principal coordinate analysis plot. Phylogenetic relationship among C. morifolium cultivars as revealed by SSR markers was highly consistent with the classification of medicinal C. morifolium populations according to their origin and ecological distribution. Our results demonstrated that SSR markers were highly reproducible and informative, and could be used to evaluate genetic diversityand relationships among medicinal C. morifolium cultivars.

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Feng, S., He, R., Lu, J., Jiang, M., Shen, X., Jiang, Y., … Wang, H. (2016). Development of SSR markers and assessment of genetic diversity in medicinal Chrysanthemum morifolium cultivars. Frontiers in Genetics, 7(JUN). https://doi.org/10.3389/fgene.2016.00113

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