国产血竭总黄酮成分的纯化及活性成分的含量测定

张明媛; 宓鹤鸣; 范国荣; 陆峰; 亓云鹏

doi:10.3969/j.issn.1006-0111.2014.01.010

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国产血竭总黄酮成分的纯化及活性成分的含量测定

张明媛, 宓鹤鸣, 范国荣, 陆峰, 亓云鹏

文章导航 > 药学实践与服务 > 2014 > 32(1): 42-44

张明媛, 宓鹤鸣, 范国荣, 陆峰, 亓云鹏. 国产血竭总黄酮成分的纯化及活性成分的含量测定[J]. 药学实践与服务, 2014, 32(1): 42-44. doi: 10.3969/j.issn.1006-0111.2014.01.010

引用本文:

ZHANG Mingyuan, MI Heming, FAN Guorong, LU Feng, QI Yunpeng. Purification of total flavones by macroporous resin and its determination of the active components from Resina Draconis[J]. Journal of Pharmaceutical Practice and Service, 2014, 32(1): 42-44. doi: 10.3969/j.issn.1006-0111.2014.01.010

Citation:

ZHANG Mingyuan, MI Heming, FAN Guorong, LU Feng, QI Yunpeng. Purification of total flavones by macroporous resin and its determination of the active components from Resina Draconis[J]. Journal of Pharmaceutical Practice and Service, 2014, 32(1): 42-44. doi: 10.3969/j.issn.1006-0111.2014.01.010

国产血竭总黄酮成分的纯化及活性成分的含量测定

doi: 10.3969/j.issn.1006-0111.2014.01.010

1.
第二军医大学药学院药物分析学教研室, 上海 200433;福建医科大学附属南平第一医院药学部, 福建南平 353000
2.
第二军医大学药学院药物分析学教研室, 上海 200433

基金项目: 国家自然科学基金(30901981);第二军医大学药学院"时珍学者培养计划"资助.

Purification of total flavones by macroporous resin and its determination of the active components from Resina Draconis

1.
Department of Pharmaceutical Analysis, School of Pharmacy, Second Military Medical University, 325 Guohe Road, Shanghai 200433, China;Department of Pharmacy, the First Hospital of Naping, Fujian Medical University, Nanping 353000, China
2.
Department of Pharmaceutical Analysis, School of Pharmacy, Second Military Medical University, 325 Guohe Road, Shanghai 200433, China

摘要: 目的采用大孔树脂对国产血竭总黄酮进行分离纯化,并测定其中活性成分的含量。方法收集大孔树脂70%乙醇和95%乙醇洗脱液,采用高效液相色谱(HPLC)法测定其中活性成分—龙血素A、龙血素B的含量。以ODS柱为分析柱,乙腈:1%冰醋酸(34.5:65.5)为流动相,检测波长为280 nm。结果龙血素A、龙血素B分别在11.00~275.00 g/ml、20.00~500.00 g/ml范围内线性关系良好,线性方程分别为Y=35 844C+44 725(r=0.999 9),Y=28 533C-41 085(r=0.999 9);方法的准确度、精密度、稳定性均符合要求。制得的国产血竭精制总黄酮中龙血素A、龙血素B的含量分别为26.93、25.53 mg/g。结论本法可用于国产血竭中相关活性成分的分析及制备,为进一步研究国产血竭活血化瘀作用提供依据。
- 国产血竭总黄酮 /
- 大孔树脂 /
- 龙血素A /
- 龙血素B /
- HPLC
Abstract: Objective To purify the total flavones from Resina Draconis using D101 resin, and set up a method of simultaneously determining the contents of loureirin A and B in the extract. Methods Fractions in 70% and 95% ethanol were collected. Mixture of acetonitrile and l% acetic acid (34.5:65.5) was used as the mobile phase and ODS column was used as stationary phase to determine loureirin A and B. The detecting wave length was 280 nm. Results In the established HPLC method, the linear range of loureirin A was 11.00-275.00 g/ml, and that of loureirin B was 20.00-500.00 g/ml. Linear equation of loureirin A was Y=35 844C+44 725(r=0.999 9) and that of loureirin B was Y=28 533C-41 085, r=0.999 9.The accuracy, precision and stability of this method were satisfactory. Conclusion The proposed method was suitable for preparation of total flavones and determination of its active components from Resina Draconis.
- total flavones in Resina Draconis /
- macroporous resin /
- loureirin A /
- loureirin B /
- HPLC

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国产血竭总黄酮成分的纯化及活性成分的含量测定

doi: 10.3969/j.issn.1006-0111.2014.01.010

1. 第二军医大学药学院药物分析学教研室, 上海 200433;福建医科大学附属南平第一医院药学部, 福建南平 353000

2. 第二军医大学药学院药物分析学教研室, 上海 200433

基金项目: 国家自然科学基金(30901981);第二军医大学药学院"时珍学者培养计划"资助.

收稿日期: 2012-12-14
修回日期: 2013-09-24

关键词:

国产血竭总黄酮 /

大孔树脂 /

龙血素A /

龙血素B /

HPLC

摘要: 目的采用大孔树脂对国产血竭总黄酮进行分离纯化,并测定其中活性成分的含量。方法收集大孔树脂70%乙醇和95%乙醇洗脱液,采用高效液相色谱(HPLC)法测定其中活性成分—龙血素A、龙血素B的含量。以ODS柱为分析柱,乙腈:1%冰醋酸(34.5:65.5)为流动相,检测波长为280 nm。结果龙血素A、龙血素B分别在11.00~275.00 g/ml、20.00~500.00 g/ml范围内线性关系良好,线性方程分别为Y=35 844C+44 725(r=0.999 9),Y=28 533C-41 085(r=0.999 9);方法的准确度、精密度、稳定性均符合要求。制得的国产血竭精制总黄酮中龙血素A、龙血素B的含量分别为26.93、25.53 mg/g。结论本法可用于国产血竭中相关活性成分的分析及制备,为进一步研究国产血竭活血化瘀作用提供依据。

English Abstract

Purification of total flavones by macroporous resin and its determination of the active components from Resina Draconis

1. Department of Pharmaceutical Analysis, School of Pharmacy, Second Military Medical University, 325 Guohe Road, Shanghai 200433, China;Department of Pharmacy, the First Hospital of Naping, Fujian Medical University, Nanping 353000, China

2. Department of Pharmaceutical Analysis, School of Pharmacy, Second Military Medical University, 325 Guohe Road, Shanghai 200433, China

Received Date: 2012-12-14
Rev Recd Date: 2013-09-24

Keywords:

Abstract: Objective To purify the total flavones from Resina Draconis using D101 resin, and set up a method of simultaneously determining the contents of loureirin A and B in the extract. Methods Fractions in 70% and 95% ethanol were collected. Mixture of acetonitrile and l% acetic acid (34.5:65.5) was used as the mobile phase and ODS column was used as stationary phase to determine loureirin A and B. The detecting wave length was 280 nm. Results In the established HPLC method, the linear range of loureirin A was 11.00-275.00 g/ml, and that of loureirin B was 20.00-500.00 g/ml. Linear equation of loureirin A was Y=35 844C+44 725(r=0.999 9) and that of loureirin B was Y=28 533C-41 085, r=0.999 9.The accuracy, precision and stability of this method were satisfactory. Conclusion The proposed method was suitable for preparation of total flavones and determination of its active components from Resina Draconis.

引用本文:

Citation:

ZHANG Mingyuan, MI Heming, FAN Guorong, LU Feng, QI Yunpeng. Purification of total flavones by macroporous resin and its determination of the active components from Resina Draconis[J]. Journal of Pharmaceutical Practice and Service, 2014, 32(1): 42-44. doi: 10.3969/j.issn.1006-0111.2014.01.010

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国产血竭总黄酮成分的纯化及活性成分的含量测定

doi: 10.3969/j.issn.1006-0111.2014.01.010

Purification of total flavones by macroporous resin and its determination of the active components from Resina Draconis

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国产血竭总黄酮成分的纯化及活性成分的含量测定

doi: 10.3969/j.issn.1006-0111.2014.01.010

1. 第二军医大学药学院药物分析学教研室, 上海 200433;福建医科大学附属南平第一医院药学部, 福建 南平 353000 2. 第二军医大学药学院药物分析学教研室, 上海 200433

English Abstract

Purification of total flavones by macroporous resin and its determination of the active components from Resina Draconis

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1. 第二军医大学药学院药物分析学教研室, 上海 200433;福建医科大学附属南平第一医院药学部, 福建南平 353000

2. 第二军医大学药学院药物分析学教研室, 上海 200433