Vipul K, Nitin M, Gupta R C
Pharmacokinetics and Metabolism Division, Central Drug Research Institute, Post Box 173, Lucknow 226001, India.
J Chromatogr B Analyt Technol Biomed Life Sci. 2005 Jun 25;820(2):221-7. doi: 10.1016/j.jchromb.2005.03.032. Epub 2005 Apr 25.
A rapid, sensitive and selective LC-MS-MS method for the simultaneous quantitation of picroside-I and kutkoside (active constituents of herbal hepatoprotectant picroliv) was developed and validated in rabbit plasma. The analytes and internal standard (Amarogentin) were extracted using Oasis HLB solid phase extraction cartridges. Analysis was performed on Spheri RP-18 column (10 microm, 100 mm x 4.6 mm i.d.) coupled with guard column using acetonitrile:MilliQ water (50:50, %v/v) as mobile phase at a flow rate of 1 ml/min with a retention time of 1.39, 1.33 and 1.42 min for picroside-I, kutkoside and amarogentin, respectively. The quantitation was carried out using an API-4000 LC-MS-MS with negative electro spray ionization in multiple reaction monitoring (MRM) mode. The precursor to product ion transitions for picroside-I, kutkoside and amarogentin were m/z 491 > 147, 199; 511 > 167, 235; 585 > 227, respectively. The method was validated in terms of establishing linearity, specificity, sensitivity, recovery, accuracy and precision (within- and between-assay variation), freeze-thaw (f-t), auto injector and dry residue stability. Linearity in plasma was observed over a concentration range of 1.56-400 ng/ml with a limit of detection (LOD) of 0.5 ng/ml for both analytes. The recoveries from spiked control samples were > 60 and > 70% for picroside-I and kutkoside, respectively. Accuracy and precision of the validated method were within the acceptable limits of < 20% at low and < 15% at other concentrations. The analytes were stable after three freeze-thaw cycles and their dry residues were stable at -60 degrees C for 15 days. The method was successfully applied to determine concentrations of picroside-I and kutkoside post i.v. bolus administration of picroliv in rabbit.
建立了一种快速、灵敏且选择性高的液相色谱-串联质谱法,用于同时定量测定兔血浆中的苦味素-I和胡黄连苷(保肝草药制剂苦味叶下珠素的活性成分),并进行了方法验证。使用Oasis HLB固相萃取柱提取分析物和内标(苦味质)。在Spheri RP-18柱(10μm,100mm×4.6mm内径)上进行分析,并连接保护柱,以乙腈:超纯水(50:50,v/v)作为流动相,流速为1ml/min,苦味素-I、胡黄连苷和苦味质的保留时间分别为1.39、1.33和1.42分钟。采用API-4000液相色谱-串联质谱仪,在多反应监测(MRM)模式下进行负离子电喷雾电离定量分析。苦味素-I、胡黄连苷和苦味质的母离子到子离子的跃迁分别为m/z 491>147、199;511>167、235;585>227。该方法在建立线性、特异性、灵敏度、回收率、准确度和精密度(批内和批间变异)、冻融(f-t)、自动进样器和干残渣稳定性方面进行了验证。血浆中的线性范围为1.56-400ng/ml,两种分析物的检测限(LOD)均为0.5ng/ml。加标对照样品中苦味素-I和胡黄连苷的回收率分别>60%和>70%。验证方法的准确度和精密度在低浓度时<20%,其他浓度时<15%,均在可接受范围内。分析物在三个冻融循环后稳定,其干残渣在-60℃下稳定15天。该方法成功应用于测定兔静脉注射苦味叶下珠素后苦味素-I和胡黄连苷的浓度。
