首页> 外文期刊>Saudi Pharmaceutical Journal >Development and validation of bioanalytical UHPLC-UV method for simultaneous analysis of unchanged fenofibrate and its metabolite fenofibric acid in rat plasma: Application to pharmacokinetics
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Development and validation of bioanalytical UHPLC-UV method for simultaneous analysis of unchanged fenofibrate and its metabolite fenofibric acid in rat plasma: Application to pharmacokinetics

机译:同时分析大鼠血浆中未改变的非诺贝特及其代谢产物非诺贝特酸的生物分析UHPLC-UV方法的开发和验证:在药代动力学中的应用

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A simple, precise, selective and fast ultra-high performance liquid chromatography (UHPLC-UV) method has been developed and validated for the simultaneous determination of a lipid regulating agent fenofibrate and its metabolite fenofibric acid in rat plasma. The chromatographic separation was carried out on a reversed-phase Acquity(R) BEH C"1"8 column using methanol-water (65:35, v/v) as the mobile phase. The isocratic flow was 0.3ml/min with rapid run time of 2.5min and UV detection was at 284nm. The method was validated over a concentration range of 100-10000ng/ml (r^2=0.9993). The selectivity, specificity, recovery, accuracy and precision were validated for determination of fenofibrate/fenofibric acid in rat plasma. The lower limits of detection and quantitation of the method were 30 and 90ng/ml for fenofibrate and 40 and 100ng/ml for fenofibric acid, respectively. The within and between-day coefficients of variation were less than 5%. The validated method has been successfully applied to measure the plasma concentrations in pharmacokinetics study of fenofibrate in an animal model to illustrate the scope and application of the method.
机译:已经开发了一种简单,精确,选择性和快速的超高效液相色谱(UHPLC-UV)方法,并已验证该方法可同时测定大鼠血浆中的脂质调节剂非诺贝特及其代谢产物非诺贝特酸。色谱分离在反相Acquity BEH C“ 1” 8柱上进行,使用甲醇-水(65:35,v / v)作为流动相。等度流速为0.3ml / min,快速运行时间为2.5min,紫外检测波长为284nm。该方法在100-10000ng / ml的浓度范围内得到验证(r ^ 2> = 0.9993)。验证了测定大鼠血浆中非诺贝特/非诺贝特酸的选择性,特异性,回收率,准确性和精密度。该方法的检测和定量的下限分别是非诺贝特为30和90ng / ml,非诺贝特酸为40和100ng / ml。日内和日间变异系数均小于5%。经过验证的方法已成功应用于动物模型中非诺贝特药代动力学研究中的血浆浓度测量,以说明该方法的范围和应用。

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