Off-target effects of the lysosomal acid lipase inhibitors Lalistat-1 and Lalistat-2 on neutral lipid hydrolases
Carbamates/pharmacology
Hydrolases/metabolism
0301 basic medicine
Hydrolases
Sterol Esterase/metabolism
Lipolysis
Lipid hydrolase activity
ATGL
Mice
03 medical and health sciences
Thiadiazoles
Animals
HSL
Internal medicine
Triglycerides
Wolman Disease
LAL
Wolman Disease/genetics
Sterol Esterase
Lipid Metabolism
MGL
RC31-1245
3. Good health
Original Article
Carbamates
Thiadiazoles/pharmacology
DOI:
10.1016/j.molmet.2022.101510
Publication Date:
2022-04-30T06:05:17Z
AUTHORS (8)
ABSTRACT
Lysosomal acid lipase (LAL) is the key enzyme, which degrades neutral lipids at an acidic pH in lysosomes. The role of LAL in various cellular processes has mostly been studied in LAL-knockout mice, which share phenotypical characteristics with humans suffering from LAL deficiency. In vitro, the cell-specific functions of LAL have been commonly investigated by using the LAL inhibitors Lalistat-1 and Lalistat-2.We performed lipid hydrolase activity assays and serine hydrolase-specific activity-based labeling combined with quantitative proteomics to investigate potential off-target effects of Lalistat-1 and -2.Pharmacological LAL inhibition but not genetic loss of LAL impairs isoproterenol-stimulated lipolysis as well as neutral triglyceride and cholesteryl ester hydrolase activities. Apart from LAL, Lalistat-1 and -2 also inhibit major cytosolic lipid hydrolases responsible for lipid degradation in primary cells at neutral pH through off-target effects. Their binding to the active center of the enzymes leads to a decrease in neutral lipid hydrolase activities in cells overexpressing the respective enzymes.Our findings are critically important since they demonstrate that commonly used concentrations of these inhibitors are not suitable to investigate the role of LAL-specific lipolysis in lysosomal function, signaling pathways, and autophagy. The interpretation of their effects on lipid metabolism should be taken with caution and the applied inhibitor concentrations in cell culture studies should not exceed 1 μM.
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