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利用平行柱分析同时进行反相和亲水相互作用液相色谱分离,并与串联质谱联用进行定量代谢产物分析。

Quantitative metabolite profiling utilizing parallel column analysis for simultaneous reversed-phase and hydrophilic interaction liquid chromatography separations combined with tandem mass spectrometry.

机构信息

Department of Chemistry, Division of Analytical Chemistry, University of Natural Resources and Life Sciences, BOKU-Vienna , Muthgasse 18, 1190 Vienna, Austria.

出版信息

Anal Chem. 2014 May 6;86(9):4145-50. doi: 10.1021/ac5003454. Epub 2014 Apr 8.

DOI:10.1021/ac5003454
PMID:24678888
Abstract

In this work, a fully automated parallel LC column method was established in order to perform orthogonal hydrophilic interaction chromatography (HILIC) and reversed-phase (RPLC) chromatography within one analytical run for targeted quantitative mass spectrometric determination of metabolites from central carbon metabolism. In this way, the analytical throughput could be significantly improved compared to previously established dual separation work flows involving two separate analytical runs. Two sample aliquots were simultaneously injected onto a dual column setup columns using a ten-port valve, and parallel separations were carried out. Sub 2 μm particle size stationary phases were employed for both separation methods. HILIC and RPLC eluents were combined post column followed by ESI-MS/MS detection. The orthogonal separations were optimized, aiming at an overall separation with 2 retention time segments, while reversed-phase separation was accomplished within 5.5 min; metabolites on the HILIC phase were retained for a minimum time of 6 min. The overall run time was 15 min. The setup was applied to the quantification of 30 primary intercellular metabolites, including amino acids, organic acids, and nucleotides employing internal standardization by a fully (13)C-labeled yeast extract. The comparison with HILIC-MS/MS and RPLC-MS/MS in separate analytical runs revealed that an excellent analytical performance was achieved by the parallel LC column method. The experimental repeatability (N = 5) was on average <5% (only for 2 compounds >5%). Moreover, limits of detection for the new approach ranging from 0.002-15 μM were in a good agreement with ones obtained in separate HILIC-MS/MS and RPLC-MS/MS runs (ranging from 0.01-44 μM).

摘要

在这项工作中,建立了一种完全自动化的平行 LC 柱方法,以便在一次分析运行中同时进行正交亲水相互作用色谱(HILIC)和反相(RPLC)色谱,用于靶向定量质谱法测定中心碳代谢中的代谢物。通过这种方式,与涉及两个单独分析运行的先前建立的双分离工作流程相比,可以显著提高分析通量。两个样品等分试样同时通过十通阀注入双柱系统的两个柱上,并进行平行分离。两种分离方法均采用 2μm 以下粒径的固定相。HILIC 和 RPLC 洗脱液在柱后合并,然后进行 ESI-MS/MS 检测。优化了正交分离,旨在实现总体分离保留两个保留时间段,同时反相分离在 5.5 分钟内完成;HILIC 相上的代谢物保留时间最短为 6 分钟。整个运行时间为 15 分钟。该装置用于通过完全(13)C 标记酵母提取物进行内部标准化来定量 30 种主要细胞内代谢物,包括氨基酸、有机酸和核苷酸。与单独的 HILIC-MS/MS 和 RPLC-MS/MS 分析相比,平行 LC 柱方法实现了出色的分析性能。实验重复性(N=5)平均<5%(仅对于 2 种化合物>5%)。此外,新方法的检测限范围为 0.002-15 μM,与单独的 HILIC-MS/MS 和 RPLC-MS/MS 运行获得的检测限(范围为 0.01-44 μM)非常吻合。

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