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胶束液相色谱法测定血浆和尿液中的利伐沙班。验证和理论方面。

Micellar liquid chromatography determination of rivaroxaban in plasma and urine. Validation and theoretical aspects.

机构信息

Departament de Química Física i Analítica, Universitat Jaume I, Castelló, Spain.

Departament de Química Analítica, Universitat de València, Burjassot, Spain.

出版信息

J Chromatogr B Analyt Technol Biomed Life Sci. 2019 Jul 1;1120:8-15. doi: 10.1016/j.jchromb.2019.04.040. Epub 2019 Apr 22.

DOI:10.1016/j.jchromb.2019.04.040
PMID:31055191
Abstract

A Micellar Chromatographic method to determine rivaroxaban in plasma and urine has been developed. The samples were dissolved in the mobile phase (SDS 0.05 M - 1-propanol 12.5%, phosphate buffered at pH 7) and 20 μL directly injected, avoiding the extraction and purification steps. Using a C18 column and running under isocratic mode at 1 mL/min, analyte was eluted without interference from the matrix in <6.0 min. The detection absorbance wavelength was set to 250 nm. The procedure was validated by Food and Drug Administration guidelines in terms of: system suitability, calibration range (0.05-5 mg/L), linearity, sensitivity, robustness, carry-over effect, specificity, accuracy (-11.1 to 4.2%), precision (<19.9%), stability and analysis of incurred samples. The method was found reliable, practical, easy-to-conduct, rapid, relatively eco-friendly, safe, inexpensive, widely available and with a high sample throughput. The method was applied to the analysis of incurred samples, including incurred sample reanalysis, to verify that the instrumentation works correctly. In addition, the constants of the different partition equilibria occurring in the column were elucidated in order to have a better comprehension of the theoretical aspects of the retention mechanism. A moderately strong association between rivaroxaban and the stationary phase and the micelles was found, weakened by short chain alcohol.

摘要

已经开发出一种胶束色谱法来测定血浆和尿液中的利伐沙班。样品在流动相(SDS 0.05 M-1-丙醇 12.5%,磷酸盐缓冲,pH 7)中溶解,并直接注入 20 μL,避免了提取和净化步骤。使用 C18 柱,在 1 mL/min 的等度模式下运行,分析物在<6.0 min 内洗脱,没有基质干扰。检测吸光度波长设置为 250 nm。该程序根据食品和药物管理局的指南进行了验证:系统适用性、校准范围(0.05-5 mg/L)、线性、灵敏度、稳健性、拖尾效应、特异性、准确度(-11.1 至 4.2%)、精密度(<19.9%)、稳定性和处理后样品的分析。该方法被发现可靠、实用、易于操作、快速、相对环保、安全、廉价、广泛可用且具有高样品通量。该方法已应用于处理后样品的分析,包括处理后样品的重新分析,以验证仪器是否正常工作。此外,还阐明了在柱中发生的不同分配平衡常数,以便更好地理解保留机制的理论方面。发现利伐沙班与固定相和胶束之间存在中等强度的相互作用,而短链醇会削弱这种相互作用。

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