Distinguishing Isomeric Caffeine Metabolites through Protomers and Tautomers using Cryogenic Gas-Phase Infrared Spectroscopy

31 August 2025, Version 1
This content is an early or alternative research output and has not been peer-reviewed by Cambridge University Press at the time of posting.

Abstract

Caffeine is metabolised through various pathways in the human body, with the primary steps yielding isomeric products. Distinguishing these metabolites is crucial for mass spectrometry-based metabolomics, for example to assess specific drug interactions. Here, we investigate the gas-phase structures of caffeine and its metabolites theophylline, theobromine, paraxanthine, 1-methylxanthine, 3-methylxanthine and 7-methylxanthine in their respective protonated ions using cryogenic gas-phase infrared spectroscopy and supported by density functional theory. The analytes exhibited varying preferences for protonation and tautomerism, particularly N9 protonation and, where applicable, a tendency for N3O2 and N1O2 amide – imidic acid and N7N9 imine – imine tautomerism. We further demonstrate that the two isomeric sets of caffeine metabolites can easily be distinguished with gas-phase IR spectroscopy, paving the route for robust identification of such molecules in metabolomics using hyphenated gas-phase techniques.

Keywords

Gas-Phase Infrared Spectroscopy
Caffeine Metabolism
Metabolomics
Density Functional Theory
Tautomerism
Protomers

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