4.4 Article

Multiple reaction monitoring profiling as an analytical strategy to investigate lipids in extracellular vesicles

Journal

JOURNAL OF MASS SPECTROMETRY
Volume 56, Issue 1, Pages -

Publisher

WILEY
DOI: 10.1002/jms.4681

Keywords

direct injection; exploratory lipidomics; extracellular vesicles; lipid profiling; MRM profiling

Funding

  1. National Institutes of Health [K08-DK107864, K08GM119006, P30 CA023168]

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A simple workflow for lipid profiling of EVs using microgram amounts of sample was reported. Human lymphocyte EVs and rat cell line EVs showed distinguishable lipid profiles in terms of protein and drug exposure as well as tissue origin.
Extracellular vesicles (EVs) convey information used in cell-to-cell interactions. Lipid analysis of EVs remains challenging because of small sample amounts available. Lipid discovery using traditional mass spectrometry platforms based on liquid chromatography and high mass resolution typically employs milligram sample amounts. We report a simple workflow for lipid profiling of EVs based on multiple reaction monitoring (MRM) profiling that uses microgram amounts of sample. After liquid-liquid extraction, individual EV samples were injected directly into the electrospray ionization (ESI) ion source at low flow rates (10 mu l/min) and screened for 197 MRM transitions chosen to be a characteristic of several classes of lipids. This choice was based on a discovery experiment, which applied 1,419 MRMs associated with multiple lipid classes to a representative pooled sample. EVs isolated from 12 samples of human lymphocytes and 16 replicates from six different rat cells lines contained an estimated amount of total lipids of 326 to 805 mu g. Samples showed profiles that included phosphatidylcholine (PC), sphingomyelin (SM), cholesteryl ester (CE), and ceramide (Cer) lipids, as well as acylcarnitines. The lipid profiles of human lymphocyte EVs were distinguishable using principal component and cluster analysis in terms of prior antibody and drug exposure. Lipid profiles of rat cell lines EV's were distinguishable by their tissue of origin.

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