Comprehensive Lipidomic Workflow for Multicohort Population Phenotyping Using Stable Isotope Dilution Targeted Liquid Chromatography-Mass Spectrometry

Monique J Ryan; Alanah Grant-St James; Nathan G Lawler; Mark W Fear; Edward Raby; Fiona M Wood; Garth L Maker; Julien Wist; Elaine Holmes; Jeremy K Nicholson; Luke Whiley; Nicola Gray

doi:10.1021/acs.jproteome.2c00682

Comprehensive Lipidomic Workflow for Multicohort Population Phenotyping Using Stable Isotope Dilution Targeted Liquid Chromatography-Mass Spectrometry

J Proteome Res. 2023 May 5;22(5):1419-1433. doi: 10.1021/acs.jproteome.2c00682. Epub 2023 Feb 24.

Authors

Monique J Ryan^{1

2}, Alanah Grant-St James^{1

2}, Nathan G Lawler^{1

2}, Mark W Fear^{3

4}, Edward Raby^{5

6}, Fiona M Wood^{3

7

4}, Garth L Maker¹, Julien Wist^{1

2}, Elaine Holmes^{1

2}, Jeremy K Nicholson^{1

2}, Luke Whiley^{1

2

8}, Nicola Gray^{1

2}

Affiliations

¹ Australian National Phenome Centre, Health Futures Institute, Harry Perkins Institute, Murdoch University, 5 Robin Warren Drive, Perth, Western Australia 6150, Australia.
² Centre for Computational and Systems Medicine, Health Futures Institute, Harry Perkins Institute, Murdoch University, 5 Robin Warren Drive, Perth, Western Australia 6150, Australia.
³ Burn Injury Research Unit, University of Western Australia, Perth, Western Australia 6009, Australia.
⁴ Fiona Wood Foundation, Perth, Western Australia 6150, Australia.
⁵ Department of Microbiology, PathWest Laboratory Medicine, Perth, Western Australia 6009, Australia.
⁶ Department of Infectious Diseases, Fiona Stanley Hospital, Perth, Western Australia 6150, Australia.
⁷ WA Department of Health, Burns Service WA, Perth, Western Australia 6009, Australia.
⁸ Perron Institute for Neurological and Translational Science, Nedlands, Western Australia 6009, Australia.

Abstract

Dysregulated lipid metabolism underpins many chronic diseases including cardiometabolic diseases. Mass spectrometry-based lipidomics is an important tool for understanding mechanisms of lipid dysfunction and is widely applied in epidemiology and clinical studies. With ever-increasing sample numbers, single batch acquisition is often unfeasible, requiring advanced methods that are accurate and robust to batch-to-batch and interday analytical variation. Herein, an optimized comprehensive targeted workflow for plasma and serum lipid quantification is presented, combining stable isotope internal standard dilution, automated sample preparation, and ultrahigh performance liquid chromatography-tandem mass spectrometry with rapid polarity switching to target 1163 lipid species spanning 20 subclasses. The resultant method is robust to common sources of analytical variation including blood collection tubes, hemolysis, freeze-thaw cycles, storage stability, analyte extraction technique, interinstrument variation, and batch-to-batch variation with 820 lipids reporting a relative standard deviation of <30% in 1048 replicate quality control plasma samples acquired across 16 independent batches (total injection count = 6142). However, sample hemolysis of ≥0.4% impacted lipid concentrations, specifically for phosphatidylethanolamines (PEs). Low interinstrument variability across two identical LC-MS systems indicated feasibility for intra/inter-lab parallelization of the assay. In summary, we have optimized a comprehensive lipidomic protocol to support rigorous analysis for large-scale, multibatch applications in precision medicine. The mass spectrometry lipidomics data have been deposited to massIVE: data set identifiers MSV000090952 and 10.25345/C5NP1WQ4S.

Keywords: lipid profiling; lipid quantification; lipidomics; lipids; liquid chromatography-mass spectrometry; metabolic phenotyping; molecular epidemiology.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Chromatography, Liquid / methods
Hemolysis*
Humans
Lipidomics* / methods
Lipids
Mass Spectrometry / methods
Workflow

Substances

Lipids