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Combined hydrophilic interaction liquid chromatography-scanning field asymmetric waveform ion mobility spectrometry-time-of-flight mass spectrometry for untargeted metabolomics

机译:结合的亲水相互作用液相色谱-扫描场非对称波形离子迁移谱-飞行时间质谱用于非目标代谢组学

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摘要

Untargeted metabolite profiling of biological samples is a challenge for analytical science due to the high degree of complexity of biofluids. Isobaric species may also not be resolved using mass spectrometry alone. As a result of these factors, many potential biomarkers may not be detected or are masked by co-eluting interferences in conventional LC-MS metabolomic analyses. In this study, a comprehensive liquid chromatography-mass spectrometry workflow incorporating a fast-scanning miniaturised high-field asymmetric waveform ion mobility spectrometry separation (LC-FAIMS-MS) is applied to the untargeted metabolomic analysis of human urine. The time-of-flight mass spectrometer used in the study was scanned at a rate of 20 scans s−1 enabling a FAIMS CF spectrum to be acquired within a 1-s scan time, maintaining an adequate number of data points across each LC peak. The developed method is demonstrated to be able to resolve co-eluting isomeric species and shows good reproducibility (%RSD < 4.9%). The nested datasets obtained for fresh, aged, and QC urine samples were submitted for multivariate statistical analysis. Seventy unique biomarker ions showing a statistically significant difference between fresh and aged urine were identified with optimal transmission CF values obtained across the full CF spectrum. The potential of using FAIMS to select ions for in-source collision-induced dissociation is demonstrated for FAIMS-selected methylxanthine ions yielding characteristic fragment ion species indicative of the precursor. Graphical abstract
机译:由于生物流体的高度复杂性,生物样品的非靶向代谢物谱分析对于分析科学是一个挑战。单独使用质谱也可能无法解决同量异位物种。由于这些因素,在传统的LC-MS代谢组学分析中,许多潜在的生物标记可能无法检测到或被共洗脱干扰所掩盖。在这项研究中,将结合快速扫描的小型化高场非对称波形离子迁移谱分离(LC-FAIMS-MS)的全面液相色谱-质谱联用技术用于人尿的非目标代谢组学分析。该研究中使用的飞行时间质谱仪以20次扫描s -1 的速率进行扫描,从而可以在1 s的扫描时间内获取FAIMS CF光谱,并保持足够的数量每个LC峰的数据点数。经证实,所开发的方法能够分离共洗脱的异构体,并具有良好的重现性(%RSD <4.9%)。将获得的新鲜,陈旧和QC尿液样本的嵌套数据集提交进行多元统计分析。通过在整个CF谱图上获得最佳的透射CF值,鉴定出70个独特的生物标志物离子,这些离子在新鲜尿液和老化尿液之间显示出统计学上的显着差异。通过FAIMS选择的甲基黄嘌呤离子产生了表征前体的特征碎片离子,证明了使用FAIMS选择离子进行源内碰撞诱导的离解的潜力。 <!-fig ft0-> <!-fig @ position =“ position” anchor“ == f4-> <!-fig mode =” anchred“ f5-> <!-fig / graphic | fig / alternatives / graphic mode =“ anchored” m1-> <!-caption a7->图形摘要

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