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Resolving the Complexity of Spatial Lipidomics Using MALDI TIMS Imaging Mass Spectrometry

2020; American Chemical Society; Volume: 92; Issue: 19 Linguagem: Inglês

10.1021/acs.analchem.0c02520

1520-6882

Katerina Djambazova, Dustin R. Klein, Lukasz G. Migas, Elizabeth K. Neumann, Emilio Rivera, Raf Van de Plas, Richard M. Caprioli, Jeffrey M. Spraggins,

Advanced Proteomics Techniques and Applications

Lipids are a structurally diverse class of molecules with important biological functions including cellular signaling and energy storage. Matrix-assisted laser desorption/ionization (MALDI) imaging mass spectrometry (IMS) allows for direct mapping of biomolecules in tissues. Fully characterizing the structural diversity of lipids remains a challenge due to the presence of isobaric and isomeric species, which greatly complicates data interpretation when only m/z information is available. Integrating ion mobility separations aids in deconvoluting these complex mixtures and addressing the challenges of lipid IMS. Here, we demonstrate that a MALDI quadrupole time-of-flight (Q-TOF) mass spectrometer with trapped ion mobility spectrometry (TIMS) enables a >250% increase in the peak capacity during IMS experiments. MALDI TIMS-MS separation of lipid isomer standards, including sn backbone isomers, acyl chain isomers, and double-bond position and stereoisomers, is demonstrated. As a proof of concept, in situ separation and imaging of lipid isomers with distinct spatial distributions were performed using tissue sections from a whole-body mouse pup.