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1.中国中医科学院 中药研究所,北京 100700
2.北京中医药大学 东直门医院,北京 100700
3.葵花药业集团(襄阳)隆中有限公司,湖北 襄阳 441003
郝雨,在读硕士,从事临床药学研究,E-mail:1240334783@qq.com
代云桃,博士,研究员,硕士生导师,从事中药药效物质基础和质量标准研究,E-mail:ytdai@icmm.ac.cn
修回日期:2019-11-19,
网络出版日期:2020-02-06,
纸质出版日期:2020-08-05
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郝雨,焦其树,周严严等.麦冬与山麦冬饮片及标准汤剂的薄层色谱鉴别[J].中国实验方剂学杂志,2020,26(15):124-129.
HAO Yu,JIAO Qi-shu,ZHOU Yan-yan,et al.Identification of Decoction Pieces and Standard Decoction of Ophiopogonis Radix and Liriopes Radix by TLC[J].Chinese Journal of Experimental Traditional Medical Formulae,2020,26(15):124-129.
郝雨,焦其树,周严严等.麦冬与山麦冬饮片及标准汤剂的薄层色谱鉴别[J].中国实验方剂学杂志,2020,26(15):124-129. DOI: 10.13422/j.cnki.syfjx.20201048.
HAO Yu,JIAO Qi-shu,ZHOU Yan-yan,et al.Identification of Decoction Pieces and Standard Decoction of Ophiopogonis Radix and Liriopes Radix by TLC[J].Chinese Journal of Experimental Traditional Medical Formulae,2020,26(15):124-129. DOI: 10.13422/j.cnki.syfjx.20201048.
目的
2
2015年版《中国药典》收录含麦冬的成方制剂92种,但缺乏有效鉴别麦冬复方制剂的方法,且麦冬与山麦冬外形相似,应用中易混淆。笔者拟建立鉴别麦冬制剂、区分麦冬与山麦冬饮片和标准汤剂的薄层色谱法(TLC)。
方法
2
收集麦冬和山麦冬饮片,制备二者的标准汤剂。采用TLC对麦冬与山麦冬饮片、标准汤剂以及含麦冬复方汤剂进行定性鉴别,选择三氯甲烷-甲醇-水(65∶35∶10)的下层溶液为展开剂,10%硫酸乙醇溶液为显色剂。
结果
2
所得薄层色谱分离度良好,麦冬饮片、标准汤剂和复方汤剂有相同的特征条带,即紫外光灯(365 nm)下的2条亮白色荧光条带,而山麦冬饮片及其标准汤剂并未显示该条带;经高分辨质谱鉴定,上述2条特征条带对应的成分均为含皂苷的混合物(包含麦冬皂苷Ra,Tb,麦冬皂苷D',麦冬皂苷C,短葶山麦冬皂苷C和龙脑苷)。
结论
2
该方法特征性强、灵敏度高,能用于麦冬饮片和标准汤剂的特征鉴别、复方汤剂中麦冬药味的鉴别,并能区分麦冬与山麦冬,为麦冬及含麦冬复方制剂的定性鉴别提供了可靠的检测方法。
Objective
2
There were 92 kinds of compound preparations containing Ophiopogonis Radix in the 2015 edition of
Chinese Pharmacopoeia
, but there was no effective method to identify these compound preparations. Because Ophiopogonis Radix and Liriopes Radix are similar in appearance, it is easy to be confused in application. The aim of this study was to set up a thin layer chromatography (TLC) to identify compound preparations containing Ophiopogonis Radix and distinguish Ophiopogonis Radix and Liriopes Radix in the forms of decoction pieces and standard decoction.
Method
2
In this study, decoction pieces of Ophiopogonis Radix and Liriopes Radix were collected and separately prepared as standard decoction. TLC was used to qualitatively identify decoction pieces and standard decoction of Ophiopogonis Radix and Liriopes Radix, and compound preparations containing Ophiopogonis Radix. In the TLC, the lower solution of chloroform-methanol-water (65∶35∶10) was selected as the developing agent and 10% sulfuric acid ethanol solution as the chromogenic agent.
Result
2
The resolution of this TLC was good. Decoction pieces, standard decoction and preparations of Ophiopogonis Radix had the same characteristic strips, which were two bright white fluorescent strips under ultraviolet lamp (365 nm). But these two characteristic strips were not existed in the TLC of decoction pieces and standard decoction of Liriopes Radix. The corresponding components of both of these two strips were identified as mixture containing saponins by LC-MS
n
, including ophiopogonin Ra, Tb, ophiopogonin D', borneol glycoside, ophiopogonin C and
Liriope muscari
baily saponins C.
Conclusion
2
The established TLC method, which has significant advantages such as high specificity and sensitivity, can be applied to the characteristic identification of decoction pieces and standard decoction of Ophiopogonis Radix, the identification of compound preparations containing Ophiopogonis Radix, and the distinction of Ophiopogonis Radix and Liriopes Radix, thus serving as an effective method to qualitatively identify Ophiopogonis Radix and its compound preparations.
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