Abstract
Oxidatively damaged lipids play critical roles in numerous human pathologies, yet methods to directly identify these species within living cells remain limited due to their transient and low-abundance nature. Existing probes for imaging lipid oxidation often rely on indirect strategies, such as monitoring changes in the fluorescence intensity or color of oxidizable probes, which detect the presence of lipid peroxidation but not its direct chemical products. Among lipid oxidation products, aldehyde-containing lipids are particularly significant due to their heightened reactivity and strong links to disease pathology. Here, we introduce OxiLox, a method that leverages fluorescent hydroxylamine-based probes to enable direct, chemoselective tagging of aldehyde-containing lipids in situ within living cells via rapid oxime ligation. Using confocal microscopy, we map the subcellular localization of these oxidized lipids, highlighting prominent accumulation within perinuclear membranes, particularly under oxidative stress conditions induced by the ferroptosis activator RSL3. Coupled with high-resolution mass spectrometry, our method precisely identifies aldehyde lipid species, notably revealing the abundance of oxidized plasmenyl phosphatidylethanolamines in ferroptotic cells. We demonstrate that cellular labeling by hydroxylamine probes can be modulated by altering the expression of antioxidant enzymes such as aldose reductase (AKR1B1), underscoring the relationship between enzymatic antioxidant defenses and lipid aldehyde metabolism. Our work establishes OxiLox as a robust approach for direct, sensitive, and chemically precise detection of lipid aldehydes in live cells, offering critical new insights into the role of lipid oxidation in health and disease.
Supplementary materials
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Supplementary Information
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Supplementary data, tables, and spectra
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Table S1
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Polyunsaturated lipids included in LPPTiger2 analysis
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Table S2
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LPPTiger 2 raw output
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MS2
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MS2 spectra for all 20 TAMRA oxime adducts of phospholipids
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