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作 者:肖远灿[1] 魏立新[1] 杨红霞[1,2] 杜玉枝[1]
机构地区:[1]中国科学院西北高原生物研究所,青海省青藏高原特色生物资源研究重点实验室,西宁810008 [2]中国科学院研究生院,北京100049
出 处:《中国药学杂志》2010年第4期255-258,共4页Chinese Pharmaceutical Journal
基 金:国家药典委员会课题(YS-200)
摘 要:目的建立印度獐牙莱药材的质量标准。方法采用薄层色谱法鉴别印度獐牙菜药材中獐牙莱苦苷、龙胆苦苷和芒果苷成分;以高效液相色谱法测定该3种成分的含量。色谱柱为ZorbaxEclipseXDB—C18(4.6mm×250mm,5μm),流动相为甲醇-水(0.1%冰醋酸)线性梯度洗脱,甲醇体积分数从22%经18min至32%并保持5min,流速为1.0mL·min^-1,柱温为25℃,检测波长为243nm。结果印度獐牙菜药材中獐牙菜苦苷、龙胆苦苷和芒果苷的薄层色谱鉴别特征明显,专属性强;药材中獐牙菜苦苷、龙胆苦苷和芒果苷的含量测定线性范围分别为0.06~2.00μg(r=0.9997),0.09—2.90μg(r=0.9997)和0.05~1.65μg(r=0.9998),平均回收率(n=9)分别为103.76%(RSD=1.34%),99.43%(RSD=1.60%)和96.22%(RSD=1.30%)。结论所建立的印度獐牙菜定性定量测定方法简单准确,能够为印度獐牙菜药材的质量控制提供有效数据.OBJECTIVE To establish a method of quality control of Swertia chirayita ( Roxb. ex Fleming) Karsten. METHODS Swertiamain, gentiopicrin and mangiferin was identified by TLC in Swertia chirayita (Roxb. ex Fleming) Karsten. Its content was determined by HPLC equipped with, Zorbax Eclipse XDB-C18 (4. 6 mm× 250 mm ,5 μm)column. The mobile phase consisted of meth- anol-water( 0. 1% glacial acetic acid), which concentration of methanol from 22% to 32% in 18 rain, then kept for 5 min. The anlysis was done at a flow rate of 1.0 mL · min^-1. The column temperature was 25 ℃ and the detection wavelength was 243 nm. RESULTS The linearities of swertiamain, gentiopicrin and mangi%rin were in the ranges of 0.06 - 2.00 μg ( r = 0. 999 7 ) , 0.09 - 2.90 μg ( r = 0. 999 7) and 0. 05 - 1.65 μg( r = 0. 999 8), respectively. The average recoveries ( n = 9) were 103.76% ( RSD = 1.34% ) for swertiamain,99. 43% ( RSD = 1.60% ) for gentiopicrin and 96.22% ( RSD = 1.30% ) for mangiferin. CONCLUSION This method is simple, accurate with good reproducibility. It is suitable for quality control of Swertia chirayita( Roxb. ex Fleming) Karsten.
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