Li Wenkui, Rettig Joan, Jiang Xiangyu, Francisco Diane T, Naidong Weng
Department of Bioanalytical Chemistry, Covance Laboratories Inc., 3301 Kinsman Blvd, Madison, WI 53704, USA.
Biomed Chromatogr. 2006 Nov;20(11):1242-51. doi: 10.1002/bmc.691.
A rapid, sensitive and specific LC-MS-MS method has been developed for the determination of clarithromycin (CLA) in human plasma using roxithromycin (ROX) as the internal standard. Samples were prepared via liquid-liquid extraction with methyl tert-butyl ether (MTBE) and chromatographed on a Supelco RP(18) (4.6 x 50 mm, 3 microm particle size) column with a mobile phase consisting of acetonitrile:methanol:60 mM (pH 3.5) ammonium acetate buffer (32.5:32.5:35) at a constant flow rate of 0.8 mL/min. The run time was 3 min with retention times of approximately 1.65 and 1.70 min for CLA and ROX, respectively. Detection was performed on a PE Sciex API 365 mass spectrometer equipped with a turboionspray ionization source in multiple reaction monitoring (MRM) mode. The MRM pairs were m/z 748.5 --> m/z 158.2 for CLA and m/z 837.7 --> m/z 679.3 for ROX, respectively, with dwell times of 200 ms for each transition. The validated calibration curve range was 5.00-5000 ng/mL, based on 0.100 mL plasma sample volume with signal-to-noise ratio (S/N) greater than 60 for CLA at the lower limit of quantification level (5.00 ng/mL). The correlation coefficients (r(2)) of the calibration curves were better than or equal to 0.996. The inter-day (n = 18) precision and accuracy of the quality control (QC) samples were less than 3.58% RSD (relative standard deviation) and -10.8% bias, respectively. The intra-day (n = 6) precision and accuracy of the quality control samples were less than 5.0 and 12.6%, respectively. There was no significant deviation from the nominal values after a 10-fold dilution of high concentration QC samples using blank matrix. The QC samples were stable when left on the bench for 24 h or after three freeze-thaw cycles. The processed samples were also stable in HPLC autosampler at 10C for over 72 h. No matrix ionization suppression was observed when extracted blank matrix or reconstitution solvent was injected onto the system with post-column infusion of clarithromycin and roxithromycin. No carryover was observed when an extracted blank plasma sample was injected immediately after a 5000 ng/mL ULOQ (the upper limit of quantification) standard. The mean recovery was 81.5 and 78.3%, respectively, for clarithromycin and internal standard.
已开发出一种快速、灵敏且特异的液相色谱-串联质谱法,以罗红霉素(ROX)为内标物测定人血浆中的克拉霉素(CLA)。样品通过用甲基叔丁基醚(MTBE)进行液-液萃取制备,并在Supelco RP(18)(4.6×50 mm,3微米粒径)柱上进行色谱分离,流动相由乙腈:甲醇:60 mM(pH 3.5)醋酸铵缓冲液(32.5:32.5:35)组成,流速恒定为0.8 mL/min。运行时间为3分钟,CLA和ROX的保留时间分别约为1.65分钟和1.70分钟。检测在配备涡轮离子喷雾电离源的PE Sciex API 365质谱仪上以多反应监测(MRM)模式进行。CLA的MRM对分别为m/z 748.5 --> m/z 158.2,ROX的MRM对为m/z 837.7 --> m/z 679.3,每个跃迁的驻留时间为200毫秒。基于0.100 mL血浆样品体积,验证后的校准曲线范围为5.00 - 5000 ng/mL,在定量下限水平(5.00 ng/mL)时CLA的信噪比(S/N)大于60。校准曲线的相关系数(r(2))优于或等于0.996。质量控制(QC)样品的日间(n = 18)精密度和准确度分别小于3.58%相对标准偏差(RSD)和 - 10.8%偏差。质量控制样品的日内(n = 6)精密度和准确度分别小于5.0%和12.6%。使用空白基质对高浓度QC样品进行10倍稀释后,与标称值无显著偏差。QC样品在室温下放置24小时或经过三个冻融循环后稳定。处理后的样品在10℃的HPLC自动进样器中也稳定超过72小时。当将萃取的空白基质或复溶溶剂与克拉霉素和罗红霉素的柱后输注一起注入系统时,未观察到基质电离抑制。当在5000 ng/mL定量上限(ULOQ)标准后立即注入萃取的空白血浆样品时,未观察到残留。克拉霉素和内标的平均回收率分别为81.5%和78.3%。
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