Optimal LC-MS metabolomic profiling reveals emergent changes to monocyte metabolism in response to lipopolysaccharide

Emma Leacy; Isabella Batten; Laetitia Sanelli; Matthew McElheron; Gareth Brady; Mark A Little; Hania Khouri

doi:10.3389/fimmu.2023.1116760

Optimal LC-MS metabolomic profiling reveals emergent changes to monocyte metabolism in response to lipopolysaccharide

Front Immunol. 2023 Mar 23:14:1116760. doi: 10.3389/fimmu.2023.1116760. eCollection 2023.

Authors

Emma Leacy¹, Isabella Batten¹, Laetitia Sanelli², Matthew McElheron¹, Gareth Brady¹, Mark A Little^{1

3}, Hania Khouri⁴

Affiliations

¹ Trinity Translational Medicine Institute, Faculty of Health Sciences, Trinity College Dublin, Dublin, Ireland.
² Faculty of Health Medicine and Life Sciences, Maastricht University, Maastricht, Netherlands.
³ Trinity Health Kidney Centre, Tallaght University Hospital, Dublin, Ireland.
⁴ Agilent Technologies, Stockpoty, England, United Kingdom.

Abstract

Introduction: Immunometabolism examines the links between immune cell function and metabolism. Dysregulation of immune cell metabolism is now an established feature of innate immune cell activation. Advances in liquid chromatography mass spectrometry (LC-MS) technologies have allowed discovery of unique insights into cellular metabolomics. Here we have studied and compared different sample preparation techniques and data normalisation methods described in the literature when applied to metabolomic profiling of human monocytes.

Methods: Primary monocytes stimulated with lipopolysaccharide (LPS) for four hours was used as a study model. Monocytes (n=24) were freshly isolated from whole blood and stimulated for four hours with lipopolysaccharide (LPS). A methanol-based extraction protocol was developed and metabolomic profiling carried out using a Hydrophilic Interaction Liquid Chromatography (HILIC) LC-MS method. Data analysis pipelines used both targeted and untargeted approaches, and over 40 different data normalisation techniques to account for technical and biological variation were examined. Cytokine levels in supernatants were measured by ELISA.

Results: This method provided broad coverage of the monocyte metabolome. The most efficient and consistent normalisation method was measurement of residual protein in the metabolite fraction, which was further validated and optimised using a commercial kit. Alterations to the monocyte metabolome in response to LPS can be detected as early as four hours post stimulation. Broad and profound changes in monocyte metabolism were seen, in line with increased cytokine production. Elevated levels of amino acids and Krebs cycle metabolites were noted and decreases in aspartate and β-alanine are also reported for the first time. In the untargeted analysis, 154 metabolite entities were significantly altered compared to unstimulated cells. Pathway analysis revealed the most prominent changes occurred to (phospho-) inositol metabolism, glycolysis, and the pentose phosphate pathway.

Discussion: These data report the emergent changes to monocyte metabolism in response to LPS, in line with reports from later time points. A number of these metabolites are reported to alter inflammatory gene expression, which may facilitate the increases in cytokine production. Further validation is needed to confirm the link between metabolic activation and upregulation of inflammatory responses.

Keywords: LC-MS; LPS; data normalization; metabolomics; monocyte.

Publication types

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

MeSH terms

Chromatography, Liquid / methods
Humans
Lipopolysaccharides*
Metabolomics / methods
Monocytes*
Tandem Mass Spectrometry / methods

Substances

Lipopolysaccharides

Grants and funding

This work was funded by Irish Research Council Enterprise Partnership Scheme (Postgraduate) Award EPSPG/2017/321 in collaboration with Agilent Technologies. Agilent Technologies was not involved in the study design, collection, analysis, interpretation of data, the writing of this article, nor the decision to submit it for publication.