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作 者:刘明周[1] 陈平[1] 汤进[1] 张芳[1] 马方[1] 于晓丹[1]
机构地区:[1]武汉工业学院生物与制药工程学院,武汉430023
出 处:《中国临床药理学杂志》2013年第5期378-380,共3页The Chinese Journal of Clinical Pharmacology
摘 要:目的建立高效液相串联质谱法测定人血浆中普拉克索浓度的方法。方法在碱性条件下,用乙酸乙酯提取浓缩后,进样用LC-MS/MS,固定相为AQ-C18柱(4.6 mm×150 mm,10μm),流动相为乙腈-20 mmol.L-1醋酸铵水溶液=60∶40,质谱条件为电喷雾离子源、正离子方式、多级离子反应监测,离子反应分别为m/z:212.2→152.9(普拉克索)和m/z 273.2→109.6(吡西卡尼)。结果普拉克索的血浆浓度在5~1000 pg.mL-1内线性关系良好,Y=1.33×103X+0.05(r=0.9979),定量下限可达5 pg.mL-1。结论建立的检测方法准确、稳定,可满足血浆中普拉克索含量测定。Objective To establish an HPLC -MS/MS method for the determination of pramipexole in healthy human plasma. Methods The plasma sample was extracted with acetic ether after evaporation of the organic layer and separated on a AQ - C18 column(4. 6 mm × 150 mm, 10 μm). The mobile phase consisted of acetonitrile and 20 mmol · L^-1 ammonium acetate (60: 40). A mass spectrometer equipped with electrosprayionization source was used as detector operate in the positive ion mode . Multiple reaction monitoring mode using the transition of m/z: 212.2- 152.9 and m/z: 273.2 -109.6 were used to quantify pramipexole and internal standard (IS), respectively. Results In human plasma, the standard curve was linear from 5 - 1000 pg · mL^-1 , Y = 1.33×10^-3X +0. 05 (r =0. 9979). The lower limit of quantification of faropenem was 5 pg·mL^-1. Conclusion The method had a good selectivity and reproducibility and can be used for the investigation of pramipexole in human plasma.
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