
doi: 10.1021/jf103311k
pmid: 21319852
To develop cleaved amplified polymorphic sequence (CAPS) markers for cultivar identification of the tea leaf, 5 primer pairs designed on the basis of genes that encode proteins related to nitrogen assimilation and 26 primer pairs based on expressed sequence tag (EST) sequences of the root of tea plant were screened. From combinations of primer pair and restriction enzyme that showed polymorphism among tea plants, 16 markers were selected and applied to DNA fingerprinting of Japanese tea cultivars. Sixty-three cultivars, except for a bud sport (Kiraka) and its original cultivar (Yabukita) and a pair that was the progeny of the same crossing parent (Harumoegi and Sakimidori), were distinguished from one another. By combining the 16 markers with previously developed CAPS markers and observing the physical appearance, 67 cultivars were distinguishable. The cultivars involve approximately 95% of total tea cultivating area in Japan; therefore, about 95% of tea leaves produced in Japan can be authenticated by labeling their cultivars.
Expressed Sequence Tags, Genetic Markers, Plant Leaves, Polymorphism, Genetic, DNA, Plant, Japan, Nitrogen, DNA Fingerprinting, Plant Roots, Camellia sinensis
Expressed Sequence Tags, Genetic Markers, Plant Leaves, Polymorphism, Genetic, DNA, Plant, Japan, Nitrogen, DNA Fingerprinting, Plant Roots, Camellia sinensis
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