Development and validation of a chromatographic method for determining Clematichinenoside AR and related impurities

Development and validation of a chromatographic method for determining Clematichinenoside AR and related impurities

<p>Abstract</p> <p>Background</p> <p>Clematichinenoside AR is a promising lead compound for the treatment of rheumatoid arthritis. A systematic research for the related impurities in AR bulk samples is still lacking. For the safe use of this natural product in future cl...

Full description

Bibliographic Details
Main Authors: Zhou Yang, Guan Yue, Shi Ji, Zhang Xiaolin, Yao Lan, Liu Lifang
Format: Article
Language:English
Published: BMC 2012-12-01
Series:Chemistry Central Journal
Subjects:
Clematichinenoside AR
Related impurities
HPLC-UV
Correction factors
Online Access:http://journal.chemistrycentral.com/content/6/1/150
id doaj-ce20d2177a3a4b948e4df06151215118
record_format Article
spelling doaj-ce20d2177a3a4b948e4df061512151182021-08-02T10:27:28ZengBMCChemistry Central Journal1752-153X2012-12-016115010.1186/1752-153X-6-150Development and validation of a chromatographic method for determining Clematichinenoside AR and related impuritiesZhou YangGuan YueShi JiZhang XiaolinYao LanLiu Lifang<p>Abstract</p> <p>Background</p> <p>Clematichinenoside AR is a promising lead compound for the treatment of rheumatoid arthritis. A systematic research for the related impurities in AR bulk samples is still lacking. For the safe use of this natural product in future clinical practice, the structure and content of each constituent, including the main ingredient as well as the impurities in AR bulk sample must be characterized in detail.</p> <p>Results</p> <p>A simple and stability indicating RP-HPLC method was developed and validated for determining the purity of clematichinenoside AR (AR), a natural product from the roots of <it>Clematis manshurica</it> Rupr. (Ranunculaceae) with the potential of treating rheumatoid arthritis. Five impurities were characterized, and impurity 2 (Clematomandshurica saponin F) is a new triterpenoid saponin isolated from this product. Optimum separation for clematichinenoside AR and five related impurities was carried out on an Agilent octadecylsilane bonded silica gel column (TC-C18, 4.6 mm ×150 mm, 5 μm) using a gradient HPLC method. The validation results showed good sensitivity, specificity, linearity(r<sup>2</sup>>0.9992) precision(RSD<1.63%), accuracy(recoveries in the range of 95.60%-104.76%) and robustness. Three AR bulk samples containing all the impurities were examined by two methods, and the stability of correction factors for the determination of related impurities was discussed. The proposed stability-indicating method was suitable for the quality control of this natural product.</p> <p>Conclusion</p> <p>Five related impurities of clematichinenoside AR were characterized, including a new triterpenoid saponins firstly found in clematichinenoside AR bulk samples. In the simple chromatographic method for determining clematichinenoside AR and its related impurities in bulk samples, the correction factor was better for the quality control in the relative stable concentrations.</p> http://journal.chemistrycentral.com/content/6/1/150Clematichinenoside ARRelated impuritiesHPLC-UVCorrection factors
collection DOAJ
language English
format Article
sources DOAJ
author Zhou Yang
Guan Yue
Shi Ji
Zhang Xiaolin
Yao Lan
Liu Lifang
spellingShingle Zhou Yang
Guan Yue
Shi Ji
Zhang Xiaolin
Yao Lan
Liu Lifang
Development and validation of a chromatographic method for determining Clematichinenoside AR and related impurities
Chemistry Central Journal
Clematichinenoside AR
Related impurities
HPLC-UV
Correction factors
author_facet Zhou Yang
Guan Yue
Shi Ji
Zhang Xiaolin
Yao Lan
Liu Lifang
author_sort Zhou Yang
title Development and validation of a chromatographic method for determining Clematichinenoside AR and related impurities
title_short Development and validation of a chromatographic method for determining Clematichinenoside AR and related impurities
title_full Development and validation of a chromatographic method for determining Clematichinenoside AR and related impurities
title_fullStr Development and validation of a chromatographic method for determining Clematichinenoside AR and related impurities
title_full_unstemmed Development and validation of a chromatographic method for determining Clematichinenoside AR and related impurities
title_sort development and validation of a chromatographic method for determining clematichinenoside ar and related impurities
publisher BMC
series Chemistry Central Journal
issn 1752-153X
publishDate 2012-12-01
description <p>Abstract</p> <p>Background</p> <p>Clematichinenoside AR is a promising lead compound for the treatment of rheumatoid arthritis. A systematic research for the related impurities in AR bulk samples is still lacking. For the safe use of this natural product in future clinical practice, the structure and content of each constituent, including the main ingredient as well as the impurities in AR bulk sample must be characterized in detail.</p> <p>Results</p> <p>A simple and stability indicating RP-HPLC method was developed and validated for determining the purity of clematichinenoside AR (AR), a natural product from the roots of <it>Clematis manshurica</it> Rupr. (Ranunculaceae) with the potential of treating rheumatoid arthritis. Five impurities were characterized, and impurity 2 (Clematomandshurica saponin F) is a new triterpenoid saponin isolated from this product. Optimum separation for clematichinenoside AR and five related impurities was carried out on an Agilent octadecylsilane bonded silica gel column (TC-C18, 4.6 mm ×150 mm, 5 μm) using a gradient HPLC method. The validation results showed good sensitivity, specificity, linearity(r<sup>2</sup>>0.9992) precision(RSD<1.63%), accuracy(recoveries in the range of 95.60%-104.76%) and robustness. Three AR bulk samples containing all the impurities were examined by two methods, and the stability of correction factors for the determination of related impurities was discussed. The proposed stability-indicating method was suitable for the quality control of this natural product.</p> <p>Conclusion</p> <p>Five related impurities of clematichinenoside AR were characterized, including a new triterpenoid saponins firstly found in clematichinenoside AR bulk samples. In the simple chromatographic method for determining clematichinenoside AR and its related impurities in bulk samples, the correction factor was better for the quality control in the relative stable concentrations.</p>
topic Clematichinenoside AR
Related impurities
HPLC-UV
Correction factors
url http://journal.chemistrycentral.com/content/6/1/150
work_keys_str_mv AT zhouyang developmentandvalidationofachromatographicmethodfordeterminingclematichinenosidearandrelatedimpurities
AT guanyue developmentandvalidationofachromatographicmethodfordeterminingclematichinenosidearandrelatedimpurities
AT shiji developmentandvalidationofachromatographicmethodfordeterminingclematichinenosidearandrelatedimpurities
AT zhangxiaolin developmentandvalidationofachromatographicmethodfordeterminingclematichinenosidearandrelatedimpurities
AT yaolan developmentandvalidationofachromatographicmethodfordeterminingclematichinenosidearandrelatedimpurities
AT liulifang developmentandvalidationofachromatographicmethodfordeterminingclematichinenosidearandrelatedimpurities
_version_ 1721233948591259648

Similar Items