4.6 Article

Characterization of acyl chain position in unsaturated phosphatidylcholines using differential mobility-mass spectrometry

Journal

JOURNAL OF LIPID RESEARCH
Volume 55, Issue 8, Pages 1668-1677

Publisher

ELSEVIER
DOI: 10.1194/jlr.M046995

Keywords

lipid isomers; sn-positional isomers; mass spectrometry; differential mobility spectrometry

Funding

  1. Australian Research Council (ARC)
  2. AB SCIEX through the Linkage Scheme [LP110200648]
  3. ARC Centre of Excellence for Free Radical Chemistry and Biotechnology [CE0561607]
  4. Australian Research Council [LP110200648] Funding Source: Australian Research Council

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Glycerophospholipids (GPs) that differ in the relative position of the two fatty acyl chains on the glycerol backbone (i.e., sn-positional isomers) can have distinct physicochemical properties. The unambiguous assignment of acyl chain position to an individual GP represents a significant analytical challenge. Here we describe a workflow where phosphatidylcholines (PCs) are subjected to ESI for characterization by a combination of differential mobility spectrometry and MS (DMS-MS). When infused as a mixture, ions formed from silver adduction of each phospholipid isomer {e. g., [PC (16:0/18:1) + Ag](+) and [PC (18:1/16:0) + Ag](+)} are transmitted through the DMS device at discrete compensation voltages. Varying their relative amounts allows facile and unambiguous assignment of the sn-positions of the fatty acyl chains for each isomer. Integration of the well-resolved ion populations provides a rapid method (< 3 min) for relative quantification of these lipid isomers. The DMS-MS results show excellent agreement with established, but time-consuming, enzymatic approaches and also provide superior accuracy to methods that rely on MS alone. The advantages of this DMS-MS method in identification and quantification of GP isomer populations is demonstrated by direct analysis of complex biological extracts without any prior fractionation.

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