Fingerprint construction of Panax notoginseng.

Author: Yan WANG ¹ ; Kai-shun BI
Author Information

1. Panjin Institute of Drug Control, Panjin 124010, Liaoning, China.
Publication Type:Journal Article
MeSH: Chromatography, High Pressure Liquid; methods; Drug Contamination; Panax; chemistry; Plant Roots; chemistry; Plants, Medicinal; chemistry; Quality Control
From: China Journal of Chinese Materia Medica 2003;28(4):316-320
CountryChina
Language:Chinese
Abstract:
OBJECTIVETo provide application and identification basis for Panax notoginseng by constructing the HPLC-FP of Panax Notoginsing.
METHODThe 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.
RESULTBy 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.
CONCLUSIONThe HPLC-FP of notoginseng has been established. The method can be used to identify and evaluate the quality of notoginseng.