
To provide application and identification basis for Panax notoginseng by constructing the HPLC-FP of Panax Notoginsing.The luna C18(2) column was used with a mobile phase of (A) acetonitrile-(B) 0.05% phosphoric acid gradient elution, 0-8 min (20% A, 80% B), 8-20 min (20% A-40% A, 80% B-60% B), 20-30 min(40% A-20% A, 60% B-80% B), 30-36 min(20% A-100% A, 80% B-0), 36-50 min(100% A), 50-65 min (100% A-20% A, 0-80% B). The flow rate was 1.0 ml.min-1. The wavelength of detecter was set at 203 nm. Caffeine was internal standard.By Cluster Analysis, the twenty-one notoginseng samples were classified as four clusters: the superior in producing area, the ordinary in producing area, the ordinary and the inferior. By Similarty Calculation, the similarity of the twenty-one notoginseng samples were 0.9-1.0, and the similarity of the eight common falses are less than 0.9.The HPLC-FP of notoginseng has been established. The method can be used to identify and evaluate the quality of notoginseng.
Quality Control, Plants, Medicinal, Panax, Drug Contamination, Plant Roots, Chromatography, High Pressure Liquid
Quality Control, Plants, Medicinal, Panax, Drug Contamination, Plant Roots, Chromatography, High Pressure Liquid
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