Profiling of Oxylipins as Markers of Oxidative Stress in Biological Samples

Author:

Yang Liping1,Choi Jaewoo1,Maier Claudia S.12,Stevens Jan F.23ORCID

Affiliation:

1. Department of Chemistry Oregon State University Corvallis Oregon

2. Linus Pauling Institute Oregon State University Corvallis Oregon

3. Department of Pharmaceutical Sciences Oregon State University Corvallis Oregon

Abstract

AbstractOxylipins are oxidized metabolites of polyunsaturated fatty acids (PUFAs). They represent a class of risk markers and/or therapeutic targets for diseases associated with inflammation, including cardiovascular disease and brain disorders. Because the biological activities of free PUFAs and oxylipins depend on their chemical structures and concentrations, monitoring PUFAs and oxylipin levels in biological systems is critical for understanding their roles in health and disease. Traditionally, accurate quantification of free PUFAs and oxylipins in biological samples was performed separately, as PUFAs are often 1000‐fold more abundant than the derived oxidized fatty acids (oxylipins). This article describes a liquid chromatography multiple reaction monitoring tandem mass spectrometry method for the quantitative analysis of five free PUFAs and 88 oxylipins in various biological fluids, including plasma, platelet supernatants, and tissues. The same approach can also be used in conjunction with an alkaline hydrolysis step to quantify total oxylipins in fish oils. We observed that in some samples, linoleic acid levels in plasma and eicosapentaenoic acid and arachidonic acid levels in brain tissue were above the upper limit of quantification. To address this issue, we developed a data analysis method to obtain PUFA and oxylipin concentrations in these samples without additional sample preparation, thus significantly saving time and labor. © 2024 Wiley Periodicals LLC.Basic Protocol: Quantification of polyunsaturated fatty acids (PUFAs) and oxylipins using liquid chromatography multiple reaction monitoring tandem mass spectrometrySupport Protocol 1: Preparation of internal standard mixed working solutionSupport Protocol 2: Preparation of standard mixed stock solutionSupport Protocol 3: Preparation of standard mixed working solutionAlternate Protocol 1: Extraction and quantitation of free PUFAs and oxylipins from mouse brain tissueAlternate Protocol 2: Extraction and quantitation of total PUFAs and oxylipins from fish oil

Publisher

Wiley

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