Deep Characterisation of the sn‐Isomer Lipidome Using High‐Throughput Data‐Independent Acquisition and Ozone‐Induced Dissociation**

Author:

Michael Jesse A.1ORCID,Young Reuben S. E.1ORCID,Balez Rachelle1ORCID,Jekimovs Lachlan J.2,Marshall David L.2ORCID,Poad Berwyck L. J.2ORCID,Mitchell Todd W.3ORCID,Blanksby Stephen J.2ORCID,Ejsing Christer S.45ORCID,Ellis Shane R.1ORCID

Affiliation:

1. Molecular Horizons and School of Chemistry and Molecular Bioscience University of Wollongong Wollongong, NSW Australia

2. School of Chemistry and Physics and the Central Analytical Research Facility Queensland University of Technology Brisbane, QLD, 4000 Australia

3. Molecular Horizons and School of Medical Indigenous and Health Sciences University of Wollongong Wollongong, NSW Australia

4. Department of Biochemistry and Molecular Biology VILLUM Center for Bioanalytical Sciences University of Southern Denmark Odense Denmark

5. Cell Biology and Biophysics Unit, European Molecular Biology Laboratory Heidelberg Germany

Abstract

AbstractIn recent years there has been a significant interest in the development of innovative lipidomics techniques capable of resolving lipid isomers. To date, methods applied to resolving sn‐isomers have resolved only a limited number of species. We report a workflow based on ozone‐induced dissociation for untargeted characterisation of hundreds of sn‐resolved glycerophospholipid isomers from biological extracts in under 20 min, coupled with an automated data analysis pipeline. It provides an order of magnitude increase in the number of sn‐isomer pairs identified as compared to previous reports and reveals that sn‐isomer populations are tightly regulated and significantly different between cell lines. The sensitivity of this method and potential for de novo molecular discovery is further demonstrated by the identification of unexpected lipids containing ultra‐long monounsaturated acyl chains at the sn‐1 position.

Funder

Australian Research Council

Villum Fonden

Publisher

Wiley

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