Scout triggered multiple reaction monitoring mass spectrometry for the rapid transfer of large multiplexed targeted methods in metabolomics

Thomas Alexandre Brunet; Sophie Ayciriex; Delphine Arquier; Jérôme Lemoine; Jérôme Randon; Arnaud Salvador

doi:10.1016/j.jchromb.2023.123849

Scout triggered multiple reaction monitoring mass spectrometry for the rapid transfer of large multiplexed targeted methods in metabolomics

J Chromatogr B Analyt Technol Biomed Life Sci. 2023 Aug 1:1228:123849. doi: 10.1016/j.jchromb.2023.123849. Epub 2023 Aug 12.

Authors

Thomas Alexandre Brunet¹, Sophie Ayciriex¹, Delphine Arquier¹, Jérôme Lemoine¹, Jérôme Randon¹, Arnaud Salvador²

Affiliations

¹ Univ Lyon, CNRS, Université Claude Bernard Lyon 1, Institut des Sciences Analytiques, UMR 5280, 5 rue de la Doua, F-69100 Villeurbanne, France.
² Univ Lyon, CNRS, Université Claude Bernard Lyon 1, Institut des Sciences Analytiques, UMR 5280, 5 rue de la Doua, F-69100 Villeurbanne, France. Electronic address: arnaud.salvador@univ-lyon1.fr.

PMID: 37634392
DOI: 10.1016/j.jchromb.2023.123849

Abstract

The field of metabolomics based on mass spectrometry has grown considerably in recent years due to the need to detect and, above all, quantify a very large number of metabolites, simultaneously. Up to now, targeted multiplexed analysis on complex samples by Liquid Chromatography coupled with tandem Mass Spectrometry (LC-MS/MS) has relied almost exclusively on compound detection based on absolute retention times, as in the Scheduled-MRM (sMRM) approach. Those methods turn out to be poorly transferable from one instrument to another and result in a time-consuming and tedious method development involving a significant number of critical parameters that need specific re-optimisation. To address this challenge, we introduce a novel acquisition mode called scout-triggered MRM (stMRM). In stMRM, a marker transition is used to trigger MS analysis for a group of dependent target analytes. These marker transitions are strategically distributed throughout the chromatographic run, and the dependent analytes are associated based on their retention times. The result is a targeted assay that remains robust even in the presence of retention time shifts. A 3 to 5-fold increase in the number of detected transitions associated to plasma metabolites was obtained when transferring from a direct application of a published sMRM to a stMRM method. This significant improvement highlights the universal applicability of the stMRM method, as it can be implemented on any LC system without the need for extensive method development. We subsequently illustrate the robustness of stMRM in modified chromatographic elution conditions. Despite a large change in metabolite's selectivity, the multiplexed assay successfully recovered 70% of the monitored transitions when consequently modifying the gradient method. These findings demonstrate the versatility and adaptability of stMRM, opening new avenues for the development of highly multiplexed LC-MS/MS methods in metabolomics. These methods are characterized by their analytical transparency and straightforward implementation using existing literature data.

Keywords: LC-MS/MS; Liquid chromatography; Method transfer; Multiple Reaction Monitoring; Targeted metabolomics; scout-triggered MRM.

MeSH terms

Biological Assay
Chromatography, Liquid
Metabolomics*
Plasma
Tandem Mass Spectrometry*