The kidney cytochrome P-450 2C23 arachidonic acid epoxygenase is upregulated during dietary salt loading
Vijaykumar R. Holla, … , Peter G. Zaphiropoulos, Jorge H. Capdevila
Vijaykumar R. Holla, … , Peter G. Zaphiropoulos, Jorge H. Capdevila
Published September 15, 1999
Citation Information: J Clin Invest. 1999;104(6):751-760. https://doi.org/10.1172/JCI7013.
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Article

The kidney cytochrome P-450 2C23 arachidonic acid epoxygenase is upregulated during dietary salt loading

Abstract

Excess dietary salt intake induces the activity of the kidney arachidonate epoxygenase and markedly increases the urinary excretion of its metabolites. The epoxyeicosatrienoic acids, products of the kidney P-450 arachidonate epoxygenase, inhibit distal nephron Na+ reabsorption. Nucleic acid hybridization studies demonstrated the expression of P-450s 2C23, 2C24, and 2C11 as the predominant kidney 2C isoforms and the lack of significant dietary salt-dependent transcriptional regulation of these proteins. Recombinant P-450s 2C11, 2C23, and 2C24 catalyze arachidonate metabolism to mixtures of epoxy- and monohydroxylated acids. Whereas the arachidonate 11,12-olefin was the preferred target for epoxidation by P-450 2C23 (57% of total products), P-450s 2C11 and 2C24 epoxidized the 11,12-olefins and 14,15-olefins with nearly equal efficiency. Stereochemical comparisons demonstrated that the regiochemical and enantiofacial selectivity of P-450 2C23 matched that of the kidney microsomal epoxygenase and that excess dietary salt does not alter the regiochemical or stereochemical selectivity of the kidney arachidonate epoxygenase. Inhibition and immunoelectrophoresis experiments using antibodies raised against recombinant P-450s 2C11 and 2C23 demonstrated that P-450 2C23 is the major 2C arachidonic acid epoxygenase in the rat kidney and the renal P-450 isoform regulated by excess dietary salt intake.

Authors

Vijaykumar R. Holla, Keiko Makita, Peter G. Zaphiropoulos, Jorge H. Capdevila

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Antibody inhibition profiles for the arachidonate monooxygenase activiti...
Antibody inhibition profiles for the arachidonate monooxygenase activities of microsomal fractions isolated from the kidneys of salt-loaded animals. Microsomal fractions were isolated from the kidneys of adult male rats fed a 2% solution of NaCl as drinking water for 10 days; suspended in a buffer system (1 mg/mL of protein) containing an NADPH-regenerating system; and incubated for 15 minutes at room temperature with either nonimmune rabbit IgG or the anti-2C11 or anti-2C23 IgGs (at a ratio of 5 or 10 mg of IgG/nmol of microsomal P-450). The reaction mixtures were then incubated for 15 minutes at 35°C in the presence of [1-14C]AA and NADPH (100 μM and 1 mM final concentrations, respectively). Shown are the radiochromatograms of the organic soluble products derived from reaction mixtures containing a total of 1 mg of microsomal protein. See Methods for further details.