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High performance liquid chromatographyg-mass spectrometry assay for polymyxin B1 and B2 in human plasma

机译:高效液相色谱-质谱法测定人血浆中的多粘菌素B1和B2

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BACKGROUND: Polymyxin B is an old antibiotic with increasing clinical relevance in the treatment of multidrug-resistant Gram-negative bacterial infections. However, current dosing regimens are largely empiric as clinical pharmacological characterization of the drug has been hindered by the lack of assays to measure polymyxin B in human plasma. METHODS: A high-performance liquid chromatography-mass spectrometry assay was developed to quantify polymyxin B1 and B2 in human plasma using pure calibrators. After purification with a solid-phase extraction column, polymyxin B1 and B2 were separated on a C18 column by gradient chromatography with an overall runtime of 12 minutes. Polymyxin B1 and B2 were ionized by positive electrospray ionization, and the resulting ions specific to polymyxin B1 and B2 were monitored (selected ion recording). RESULTS: The dominant ions produced were (M + 2H) at m/z 602.6 and 595.5 for polymyxin B1 and polymyxin B2, respectively. The assay was linear between concentrations of 100 and 2500 ng/mL, with interday precision of 5.9% and 3.4% at 100 ng/mL and 5.3% and 4.0% at 2000 ng/mL for polymyxin B1 and polymyxin B2, respectively. Accuracy was 80.2% and 82.2% at 100 ng/mL and 99.9% and 109.6% at 2000 ng/mL for polymyxin B1 and polymyxin B2, respectively. No interference from other drugs commonly administered with polymyxin B was detected. The performance of the assay is affected by gross hemolysis and hyperlipemia. The method was successfully applied to patient samples. Interestingly, in a single patient the ratio of B1 and B2 did not change over a period of 12 hours after administration of the drug. CONCLUSIONS: A simple method for the simultaneous measurement of polymyxin B1 and polymyxin B2 in human plasma is described, which has the potential to optimize clinical use of this valuable antibiotic by permitting pharmacokinetic studies and therapeutic drug monitoring.
机译:背景:多粘菌素B是一种古老的抗生素,在治疗多药耐药的革兰氏阴性细菌感染中具有越来越高的临床意义。然而,当前的给药方案在很大程度上是经验性的,因为缺乏用于测定人血浆中多粘菌素B的测定法阻碍了该药物的临床药理学表征。方法:开发了一种高效液相色谱-质谱分析法,使用纯净校准品对人血浆中的多粘菌素B1和B2进行定量。用固相萃取柱纯化后,将多粘菌素B1和B2在C18柱上通过梯度色谱分离,总运行时间为12分钟。通过正电喷雾电离使多粘菌素B1和B2离子化,并监测所产生的多粘菌素B1和B2特有的离子(选择离子记录)。结果:多粘菌素B1和多粘菌素B2的主要离子分别为(M + 2H),m / z 602.6和595.5。该测定在100和2500 ng / mL的浓度之间呈线性关系,多粘菌素B1和多粘菌素B2的日间精密度分别为100 ng / mL时的5.9%和3.4%和2000 ng / mL时的5.3%和4.0%。多粘菌素B1和多粘菌素B2的准确度分别为100 ng / mL时的80.2%和82.2%,以及2000 ng / mL时的99.9%和109.6%。没有检测到通常与多粘菌素B一起使用的其他药物的干扰。测定的性能受总溶血和高脂血症的影响。该方法已成功应用于患者样品。有趣的是,在单个患者中,药物给药后12小时内B1和B2的比例没有变化。结论:描述了一种同时测定人血浆中多粘菌素B1和多粘菌素B2的简单方法,通过允许进行药代动力学研究和治疗药物监测,有可能优化这种有价值的抗生素的临床使用。

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