薄层色谱密度法测定中药中木犀草素、槲皮素、芹菜素和西番莲素含量的优化方法及稳定性试验

M. Hidayatullah, M. Yuwono, R. Primaharinastiti
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引用次数: 0

摘要

背景:肾结石是一种在骨盆或肾盏中有一个或多个肾结石的情况。木犀草素、槲皮素、芹菜素、水仙素是车前草、蛇耳草、鹤耳草等植物提取物中具有肾结石作用的标志化合物。为了控制中药材的质量,建立了以木犀草素、槲皮素、芹菜素、五味子素为植物化学标记物的薄层色谱密度测定法。目的:建立木犀草素、槲皮素、芹菜素、五倍子素的最佳分析条件。方法:通过测定流动相组成、腔室饱和时间、分析波长确定最佳分析条件。以硅胶60f254为固定相。稳定性试验通过在0、4、8和24小时分析标准品和样品进行。结果:采用流动相为氯仿:丙酮:二氯甲烷:乙腈:甲酸(6:2:2:0,05:0.05 v/v/v/v/ v/v/v),波长为335 nm,饱和时间为30 min,在等密度条件下可获得最佳的分离峰。结论:本研究确定了测定木犀草素、槲皮素、芹菜素、五倍子素的最佳工艺条件。木犀草素、槲皮素、芹菜素和枳实素在8小时内不稳定。因此,标准溶液和样品必须新鲜,以保持稳定性。
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Optimization Method and Stability Test to Determinate Luteolin, Quercetin, Apigenin, and Sinensetin Levels in Herbal Medicines Using TLC-Densitometry
Background: Nephrolithiasis is a condition in which there are one or more kidney stones in the pelvis or calyces. Luteolin, quercetin, apigenin, and sinensetin are marker compounds in the extracts of Plantago major, Sonchus arvensis, Strobilanthes crispus and Orthosiphon stamineus which have nephrolithiasis activity. To control the quality of herbal medicines, a TLC-Densitometry method was developed in this study using luteolin, quercetin, apigenin, and sinensetin as phytochemical markers. Objective: The present work aimed to develop optimal conditions for analyzing luteolin, quercetin, apigenin, and sinensetin. Methods: Determination of optimal conditions for analysis is carried out by determining the composition of the mobile phase, chamber saturation time, and analysis wavelength. Silica gel 60 F254 was used as the stationary phase. Stability tests were carried out by analyzing standards and samples at 0, 4, 8, and 24 hours. Results: The best separation that produces symmetrical peaks of herbal medicine was achieved under isocratic conditions using the composition of the mobile phase chloroform : acetone: dichloromethane : acetonitrile : formic acid (6 : 2: 2 : 0,05 : 0.05 v/v/v/v/ v) with a wavelength of 335 nm with a saturation time of 30 minutes. Conclusion: In this study, the optimal conditions for the analysis of luteolin, quercetin, apigenin, and sinensetin. Luteolin, quercetin, apigenin, and sinensetin are unstable during 8 hours of storage. Therefore, standard solutions and samples must be made fresh to maintain stability.
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