4.3 Article

Metabolic profiling of human blood by high-resolution ion mobility mass spectrometry (IM-MS)

Journal

INTERNATIONAL JOURNAL OF MASS SPECTROMETRY
Volume 298, Issue 1-3, Pages 78-90

Publisher

ELSEVIER
DOI: 10.1016/j.ijms.2010.02.007

Keywords

Mobility-mass correlation curve (MMCC); IMS; Isomer separation; Metabolomics; Blood metabolite; IM-MS

Funding

  1. National Institute of Health [R21-DK070274]

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A high-resolution ion mobility time-of-flight mass spectrometer with electrospray ionization source (ESI-IM-MS) was evaluated as an analytical method for rapid analysis of complex biological samples such as human blood metabolome. The hybrid instrument (IM-MS) provided an average ion mobility resolving power of similar to 90 and a mass resolution of similar to 1500 (at m/z 100). A few mu L of whole blood was extracted with methanol, centrifuged and infused into the IM-MS via an electrospray ionization source. Upon IM-MS profiling of the human blood metabolome approximately 1100 metabolite ions were detected and 300 isomeric metabolites separated in short analyses time (30 min). Estimated concentration of the metabolites ranged from the low micromolar to the low nanomolar level. Various classes of metabolites (amino acids, organic acids, fatty acids, carbohydrates. purines and pyrimidines. etc.) were found to form characteristic mobility-mass correlation curves (MMCCs) that aided in metabolite identification. Peaks corresponding to various sterol derivatives, estrogen derivatives, phosphocholines, prostaglandins, and cholesterol derivatives detected in the blood extract were found to occupy characteristic two-dimensional IM-MS space. Low abundance metabolite peaks that can be lost in MS random noise were resolved from noise peaks by differentiation in mobility space. In addition, the peak capacity of MS increased sixfold by coupling IMS prior to MS analysis. (C) 2010 Elsevier B.V. All rights reserved.

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