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首页> 外文期刊>Journal of chromatography, A: Including electrophoresis and other separation methods >FULLY AUTOMATED DETERMINATION OF SELECTIVE RETINOIC ACID RECEPTOR LIGANDS IN MOUSE PLASMA AND TISSUE BY REVERSED-PHASE LIQUID CHROMATOGRAPHY COUPLED ON-LINE WITH SOLID-PHASE EXTRACTION
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FULLY AUTOMATED DETERMINATION OF SELECTIVE RETINOIC ACID RECEPTOR LIGANDS IN MOUSE PLASMA AND TISSUE BY REVERSED-PHASE LIQUID CHROMATOGRAPHY COUPLED ON-LINE WITH SOLID-PHASE EXTRACTION

机译:固相萃取-反相液相色谱法全自动测定小鼠血浆和组织中的选择性维甲酸受体配体

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A fully automated reversed-phase HPLC method was developed for the quantitative assay of three retinoids (Am-580, CD-2019 and CD-437) which selectively activate the retinoic acid receptors RAR alpha, RAR beta and RAR gamma, respectively. Mouse plasma, embryo and maternal tissues were prepared for injection by on-line solid-phase extraction (SPE) and valve-switching techniques. Following automatic injection, the sample was loaded on preconditioned disposable cartridges, cleaned-up and then transferred onto the analytical column to be eluted in the backflush mode, separated by gradient elution and detected by UV, while a new cartridge was concomitantly conditioned. The overall recovery was quantitative allowing for external standardization. The calibration curves were linear in all biological samples tested so far, with a correlation coefficient (r) >0.99. The intra-day precision was less than or equal to 7.8% (n=5-6) and the inter-day variability was less than or equal to 9.4% (n=3). The lower limit of detection was 2.5 ng/ml or ng/g for CD-2019 and CD-437, and 5 ng/ml for Am-580 with a SIN ratio of 5 using a sample weight of 25 mu l or mg. The method is now in routine use in our laboratory for the assessment of the pharmacokinetic profiles of these retinoids. The small sample size required, the simple sample prepration and the rapid analysis with high degree of automation make this method convenient for microanalysis of biological samples both in animal and human studies.
机译:开发了一种全自动反相HPLC方法,用于定量检测分别选择性激活视黄酸受体RARα,RARβ和RARγ的三种类维生素A(Am-580,CD-2019和CD-437)。通过在线固相萃取(SPE)和阀切换技术,准备了小鼠血浆,胚胎和母体组织进行注射。自动进样后,将样品上样到预处理的一次性小柱上,进行清洁,然后将其转移到分析柱上,以反吹模式洗脱,通过梯度洗脱分离并通过UV进行检测,同时对新的小柱进行调节。总体回收率是定量的,可以进行外部标准化。到目前为止,所有测试的生物样品中的校准曲线都是线性的,相关系数(r)> 0.99。日内精确度小于或等于7.8%(n = 5-6),日间变异性小于或等于9.4%(n = 3)。对于CD-2019和CD-437,检测下限为2.5 ng / ml或ng / g,对于SIN为5的Am-580,使用25μl或mg的样品重量检测下限为5 ng / ml。该方法现已在我们的实验室中常规用于评估这些类维生素A的药代动力学特征。所需的小样本量,简单的样品前处理以及具有高度自动化的快速分析功能,使该方法便于在动物和人体研究中对生物样品进行微量分析。

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