Effects of sphingosine and sphingosine analogues on the free radical production by stimulated neutrophils: ESR and chemiluminescence studies

Author:

Mouithys-Mickalad A.1,Deby-Dupont G.12,Hoebeke M.3,Mathy-Hartert M.1,Lamy M.12,Deby C.1

Affiliation:

1. Centre for the Biochemistry of Oxygen, University of Liège, Domaine Universitaire du Sart Tilman, Liège 4000, Belgium

2. Department of Anesthesia and Intensive Care Medicine, University Hospital of Liège, Domaine Universitaire du Sart Tilman, Liège 4000, Belgium

3. Laboratory of Experimental Physics, University of Liège, Domaine Universitaire du Sart Tilman, Liège 4000, Belgium

Abstract

Sphingolipids inhibit the activation of the neutrophil (PMN) NADPH oxidase by protein kinase C pathway. By electron spin resonance spectroscopy (ESR) and chemiluminescence (CL), we studied the effects of sphingosine (SPN) and ceramide analogues on phorbol 12-myristate 13-acetate (PMA, 5 × 10-7M) stimulated PMN (6 × 106cells). By ESR with spin trapping (100 mM DMPO: 5,5-dimethyl-1-pyrroline-Noxide), we showed that SPN (5 to 8 × 10-6M), C2-ceramide (N-acetyl SPN) and C6-ceramide (N-hexanoyl SPN) at the final concentration of 2 × 10-5and 2 × 10-4M inhibit the production of free radicals by stimulated PMN. The ESR spectrum of stimulated PMN was that of DMPO-superoxide anion spin adduct. Inhibition by 5 × 10-6M SPN was equivalent to that of 30 U/ml SOD. SPN (5 to 8 × 10-6M) has no effect onin vitrosystems generating superoxide anion (xanthine 50 mM/xanthine oxidase 110 mU/ml) or hydroxyl radical (Fenton reaction: 88 mM H2O2, 0.01 mM Fe2+and 0.01 mM EDTA). SPN and N-acetyl SPN also inhibited the CL of PMA stimulated PMN in a dose dependent manner (from 2 × 10-6to 10-5M), but N-hexanoyl SPN was less active (from 2 × 10-5to 2 × 10-4M). These effects were compared with those of known PMN inhibitors, superoxide dismutase, catalase and azide. SPN was a better inhibitor compared with these agents. The complete inhibition by SPN of ESR signal and CL of stimulated PMN confirms that this compound or one of its metabolites act at the level of NADPH-oxidase, the key enzyme responsible for production of oxygen-derived free radicals.

Funder

FRSM, Belgium

Publisher

Hindawi Limited

Subject

Cell Biology,Immunology

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