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首页> 外文期刊>Biomedical Chromatography: An International Journal Devoted to Research in Chromatographic Methodologies and Their Applications in the Biosciences >Bioanalytical assay development and validation for simultaneous quantification of five schisandra lignans in rat primary hepatocytes based on LC-MS/MS: application to a real-time uptake study for Schisandra Lignan Extract
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Bioanalytical assay development and validation for simultaneous quantification of five schisandra lignans in rat primary hepatocytes based on LC-MS/MS: application to a real-time uptake study for Schisandra Lignan Extract

机译:基于LC-MS / MS的大鼠原发性肝细胞同时定量5种Schisandra Lignans同时定量的生物分析验证:应用于Schisandra lignan提取物的实时摄取研究

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摘要

Schisandra lignans, mainly including schizandrol A, schizandrol B, schisantherin A, schizandrin A, schizandrin B, etc., are the major active ingredients of Schisandra chinensis. In the present study, a robust liquid chromatography-tandem mass spectrometric (LC-MS/MS) method was developed for the simultaneous quantification of schisandra lignans in rat primary hepatocytes. Lovastatin was used as an internal standard, and chromatographic separation was achieved on a Shimadzu C-18 column with a gradient elution at the flow rate of 0.2 mL/min. All of the analytes were detected in multiple reaction monitoring mode with positive electrospray ionization since the sodium adduct ion [M + Na](+) was observed as the most intensive peak in the MS spectrum. For schizandrol A, schisantherin A and schizandrin A, the dynamic range was within 2-1000 ng/mg protein, and the linear range of schizandrol B and schizandrin B was from 5 to 1000 ng/mg protein. The intra-and inter-day precision was < 15% and the accuracy (relative error) ranged from -15 to 15%. No significant variation was observed in the stability tests. The validated method was then successfully applied to the time-dependent uptake study for the Schisandra Lignan Extract in rat primary hepatocytes.
机译:Schisandra Lignans,主要包括Schizandrol A,Schizandrol B,Schisantherin A,Schizandrin A,Schizandrin B等是Schisandra Chinensis的主要活性成分。在本研究中,开发了一种稳健的液相色谱 - 串联质谱(LC-MS / MS)方法,用于同时定量大鼠原发性肝细胞中的Schisandra Lignans。 Lovastatin用作内标,在Shimadzu C-18柱上达到色谱分离,其流速为0.2ml / min的流速。在多反应监测模式中检测到所有分析物,其具有正电喷雾电离,因为钠加合离子[M + Na](+)作为MS光谱中最强烈的峰值。对于Schizandrol A,Schisantherin A和Schizandrin A,动态范围在2-1000ng / mg蛋白内,Schizandrol B和Schizandrinb的线性范围为5至1000ng / mg蛋白。内部和日间精度<15%,精度(相对误差)范围为-15至15%。在稳定性测试中没有观察到显着的变化。然后成功地应用了验证的方法对大鼠原发性肝细胞的Schisandra Lignan提取物的时间依赖性摄取研究。

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