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A structural examination and collision cross section database for over 500 metabolites and xenobiotics using drift tube ion mobility spectrometry

机译:使用漂移管离子迁移光谱法为超过500种代谢物和异卵虫的结构检查和碰撞横截面数据库

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摘要

The confident identification of metabolites and xenobiotics in biological and environmental studies is an analytical challenge due to their immense dynamic range, vast chemical space and structural diversity. Ion mobility spectrometry (IMS) is widely used for small molecule analyses since it can separate isomeric species and be easily coupled with front end separations and mass spectrometry for multidimensional characterizations. However, to date IMS metabolomic and exposomic studies have been limited by an inadequate number of accurate collision cross section (CCS) values for small molecules, causing features to be detected but not confidently identified. In this work, we utilized drift tube IMS (DTIMS) to directly measure CCS values for over 500 small molecules including primary metabolites, secondary metabolites and xenobiotics. Since DTIMS measurements do not need calibrant ions or calibration like some other IMS techniques, they avoid calibration errors which can cause problems in distinguishing structurally similar molecules. All measurements were performed in triplicate in both positive and negative polarities with nitrogen gas and seven different electric fields, so that relative standard deviations (RSD) could be assessed for each molecule and structural differences studied. The primary metabolites analyzed to date have come from key metabolism pathways such as glycolysis, the pentose phosphate pathway and the tricarboxylic acid cycle, while the secondary metabolites consisted of classes such as terpenes and flavonoids, and the xenobiotics represented a range of molecules from antibiotics to polycyclic aromatic hydrocarbons. Different CCS trends were observed for several of the diverse small molecule classes and when urine features were matched to the database, the addition of the IMS dimension greatly reduced the possible number of candidate molecules. This CCS database and structural information are freely available for download at http://panomics.pnnl.gov/metabolites/ with new molecules being added frequently.
机译:生物和环境研究中代谢物和异恶蛋白的自信鉴定是由于它们的巨大动态范围,巨大的化学空间和结构多样性,是一种分析挑战。离子迁移谱分析(IMS)广泛用于小分子分析,因为它可以分离异构物质并容易地与前端分离和质谱进行耦合,以进行多维特征。然而,迄今为止,IMS代谢组和扩张组研究受到小分子的准确碰撞横截面(CCS)值的数量不足,导致要检测的特征但不受信心鉴定。在这项工作中,我们利用漂移管IMS(DTIM)直接测量超过500种小分子的CCS值,包括初级代谢物,次生代谢物和异种菌。由于DTIMS测量不需要校准离子或类似于其他IMS技术的校准,因此它们避免校准误差,这可能导致在结构类似的分子中造成问题。所有测量均在具有氮气和七种不同的电场的正极和负极的两次进行,从而可以对每个分子评估相对标准偏差(RSD)和所研究的结构差异。分析到迄今为止的主要代谢产物来自糖酵解,戊糖磷酸途径和三羧酸循环等关键代谢途径,而次生代谢物由诸如萜烯和黄酮类化合物等类别组成,并且Xenobiotics代表了一系列来自抗生素的分子多环芳烃。对于多个不同的小分子类以及尿液特征与数据库匹配时,观察到不同的CCS趋势,加入IMS维度大大降低了可能数量的候选分子。此CCS数据库和结构信息可免费下载http://panomics.pnnl.gov/metabolites/,频繁添加新分子。

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  • 来源
    《Chemical science》 |2017年第11期|共13页
  • 作者单位

    Pacific Northwest Natl Lab Biol Sci Div 902 Battelle Blvd POB 999 MSIN K8-98 Richland WA 99352 USA;

    Pacific Northwest Natl Lab Biol Sci Div 902 Battelle Blvd POB 999 MSIN K8-98 Richland WA 99352 USA;

    Pacific Northwest Natl Lab Biol Sci Div 902 Battelle Blvd POB 999 MSIN K8-98 Richland WA 99352 USA;

    Pacific Northwest Natl Lab Biol Sci Div 902 Battelle Blvd POB 999 MSIN K8-98 Richland WA 99352 USA;

    Pacific Northwest Natl Lab Biol Sci Div 902 Battelle Blvd POB 999 MSIN K8-98 Richland WA 99352 USA;

    Pacific Northwest Natl Lab Biol Sci Div 902 Battelle Blvd POB 999 MSIN K8-98 Richland WA 99352 USA;

    Pacific Northwest Natl Lab Biol Sci Div 902 Battelle Blvd POB 999 MSIN K8-98 Richland WA 99352 USA;

    Pacific Northwest Natl Lab Biol Sci Div 902 Battelle Blvd POB 999 MSIN K8-98 Richland WA 99352 USA;

    Pacific Northwest Natl Lab Biol Sci Div 902 Battelle Blvd POB 999 MSIN K8-98 Richland WA 99352 USA;

    Pacific Northwest Natl Lab Biol Sci Div 902 Battelle Blvd POB 999 MSIN K8-98 Richland WA 99352 USA;

    Pacific Northwest Natl Lab Biol Sci Div 902 Battelle Blvd POB 999 MSIN K8-98 Richland WA 99352 USA;

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  • 正文语种 eng
  • 中图分类 化学;
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