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Comparison of blood sirolimus, tacrolimus and everolimus concentrations measured by LC-MS/MS, HPLC-UV and immunoassay methods

机译:通过LC-ms / ms,HpLC-UV和免疫测定方法测量血液西罗莫司,他克莫司和依维莫司浓度的比较

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摘要

An LC-MS/MS method was developed for simultaneous quantitation of tacrolimus, sirolimus and everolimus in whole blood, and compared to HPLC-UV and immunoassay methods.Blood (0.1mL) was analysed following solid-phase extraction and chromatographic resolution using a C18 column (45°C) and mobile phase of methanol/40mM ammonium acetate/glacial acetic acid (83/17/0.1) at 200μL/min, with positive electrospray ionisation and multiple reaction monitoring.Intra- and inter-day imprecision and inaccuracy were ≤12.2% over a 1.5-40μg/L calibration range. An external quality assurance programme confirmed acceptable inaccuracy and imprecision of the LC-MS/MS method, but highlighted problems with immunoassay quantitation, particularly for everolimus, showing a >30% bias in FPIA everolimus concentrations measured in pooled patient samples versus spiked drug-free whole blood.LC-MS/MS provides significant accuracy and precision advantages compared to HPLC and immunoassays. Discrepancies in everolimus concentrations measured by the Seradyn FPIA immunoassay require further investigation.
机译:建立了LC-MS / MS方法同时定量全血中他克莫司,西罗莫司和依维莫司的方法,并与HPLC-UV和免疫测定方法进行了比较。固相萃取和色谱分离后使用C18分析血液(0.1mL)色谱柱(45°C)和甲醇/ 40mM醋酸铵/冰醋酸(83/17 / 0.1)的流动相以200μL/ min的流速进行正电喷雾电离和多反应监测,日内和日间不精确度和不准确性在1.5-40μg/ L的校准范围内≤12.2%。外部质量保证程序确认了LC-MS / MS方法可接受的不准确性和不精确性,但突出了免疫测定定量的问题,尤其是依维莫司的定量分析,显示在合并患者样品中测量的FPIA依维莫司浓度偏差大于30%,而无加标药物与HPLC和免疫分析相比,LC-MS / MS具有显着的准确性和精密度优势。 Seradyn FPIA免疫测定法测量的依维莫司浓度差异需要进一步研究。

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