1. Posttranslational modification by an isolevuglandin diminishes activity of the mitochondrial cytochrome P450 27A1[S]
- Author
-
Casey D. Charvet, Irina A. Pikuleva, James Laird, Robert G. Salomon, and Yunfeng Xu
- Subjects
multiple reaction monitoring ,Mutant ,Lysine ,QD415-436 ,Mitochondrion ,Biochemistry ,Retina ,Macular Degeneration ,Endocrinology ,CYP27A1 ,oxidative stress ,Animals ,Humans ,age-related macular degeneration ,Research Articles ,chemistry.chemical_classification ,biology ,Prostaglandins E ,Wild type ,Cytochrome P450 ,lipid peroxidation ,Cell Biology ,γ-ketoaldehydes ,Enzyme assay ,Mitochondria ,Protein Structure, Tertiary ,Enzyme ,Cholesterol ,chemistry ,Mutation ,biology.protein ,cholesterol metabolism ,Cholestanetriol 26-Monooxygenase ,Cattle ,Protein Processing, Post-Translational - Abstract
Posttranslational modification by isolevuglandins (isoLGs), arachidonate oxidation products, is an important yet understudied process associated with altered protein properties. This type of modification is detected in cytochrome P450 27A1 (CYP27A1), a multifunction enzyme expressed in almost every cell and involved in the metabolism of cholesterol and other sterols. Previously, the CYP27A1 Lys(358)-isoLG adduct was found in human retina afflicted with age-related macular degeneration. Yet, the effect of Lys(358) modification on enzyme activity was not investigated. Herein, we characterized catalytic properties of Lys(358) as well as Lys(476) CYP27A1 mutants before and after isoLG treatment and quantified the extent of modification by multiple reaction monitoring. The K358R mutant was less susceptible to isoLG-induced loss of catalytic activity than the wild type (WT), whereas the K476R mutant was nearly as vulnerable as the WT. Both mutants showed less isoLG modification than WT. Thus, modification of Lys(358), a residue involved in redox partner interactions, is the major contributor to isoLG-associated loss of CYP27A1 activity. Our data show the specificity of isoLG modification, provide direct evidence that isoLG adduction impairs enzyme activity, and support our hypothesis that isoLG modification in the retina is detrimental to CYP27A1 enzyme activity, potentially disrupting cholesterol homeostasis.
- Published
- 2013