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白毛茛根粉中生物碱含量测定的方法验证

Method validation for determination of alkaloid content in goldenseal root powder.

作者信息

Weber Holly A, Zart Matthew K, Hodges Andrew E, White Kellie D, Barnes Sarah M, Moody Leslie A, Clark Alice P, Harris Roger K, Overstreet J Diane, Smith Cynthia S

机构信息

Midwest Research Institute, 425 Volker Blvd, Kansas City, MO 64110, USA.

出版信息

J AOAC Int. 2003 May-Jun;86(3):476-83.

Abstract

A fast, practical ambient extraction methodology followed by isocratic liquid chromatography (LC) analysis with UV detection was validated for the determination of berberine, hydrastine, and canadine in goldenseal (Hydrastis canadensis L.) root powder. The method was also validated for palmatine, a major alkaloid present in the possible bioadulterants Coptis, Oregon grape root, and barberry bark. Alkaloid standard solutions were linear over the evaluated concentration ranges. The analytical method was linear for alkaloid extraction using 0.3-2 g goldenseal root powder/100 mL extraction solvent. Precision of the method was demonstrated using 10 replicate extractions of 0.5 g goldenseal root powder, with percent relative standard deviation for all 4 alkaloids < or = 1.6. Alkaloid recovery was determined by spiking each alkaloid into triplicate aliquots of neat goldenseal root powder. Recoveries ranged from 92.3% for palmatine to 101.9% for hydrastine. Ruggedness of the method was evaluated by performing multiple analyses of goldenseal root powder from 3 suppliers over a 2-year period. The method was also used to analyze Coptis root, Oregon grape root, barberry bark, and celandine herb, which are possible goldenseal bioadulterants. The resulting chromatographic profiles of the bioadulterants were significantly different from that of goldenseal. The method was directly transferred to LC with mass spectrometry, which was used to confirm the presence of goldenseal alkaloids tetrahydroberberastine, berberastine, canadaline, berberine, hydrastine, and canadine, as well as alkaloids from the bioadulterants, including palmatine, jatrorrhizine, and coptisine.

摘要

一种快速、实用的环境萃取方法,随后采用等度液相色谱(LC)分析并结合紫外检测,已被验证可用于测定白毛茛(Hydrastis canadensis L.)根粉中的小檗碱、北美黄连碱和加拿大黄连碱。该方法也被验证可用于巴马汀的测定,巴马汀是可能的掺假品黄连、俄勒冈葡萄根和伏牛花树皮中的主要生物碱。生物碱标准溶液在评估的浓度范围内呈线性。使用0.3 - 2 g白毛茛根粉/100 mL萃取溶剂进行生物碱萃取时,该分析方法呈线性。通过对0.5 g白毛茛根粉进行10次重复萃取来证明该方法的精密度,所有4种生物碱的相对标准偏差百分比≤1.6。通过将每种生物碱加入到纯净的白毛茛根粉的三份等分试样中来测定生物碱回收率。回收率范围从巴马汀的92.3%到北美黄连碱的101.9%。通过在两年时间内对来自3个供应商的白毛茛根粉进行多次分析来评估该方法的耐用性。该方法还用于分析黄连根、俄勒冈葡萄根、伏牛花树皮和白屈菜,它们是可能的白毛茛掺假品。所得掺假品的色谱图与白毛茛的色谱图有显著差异。该方法直接转移至液相色谱 - 质谱联用仪,用于确认白毛茛生物碱四氢小檗胺、小檗胺、加拿大黄连次碱、小檗碱、北美黄连碱和加拿大黄连碱的存在,以及掺假品中的生物碱,包括巴马汀、药根碱和黄连碱。

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