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Protective action of CLA against oxidative inactivation of paraoxonase 1, an antioxidant enzyme
Authors:Nguyen-Duy?Su  Xi-Wen?Liu  Mee?Ree?Kim  Tae-Sook?Jeong  Email author" target="_blank">Dai-Eun?SokEmail author
Affiliation:(1) College of Pharmacy, Chungnam National University, 305-764 Taejon, Korea;(2) Department of Food and Nutrition, Chungnam National University, 305-764 Taejon, Korea;(3) Lipid Metabolism Laboratory, Korea Research Institute of Bioscience and Biotechnology, 305-333 Taejon, Korea
Abstract:The effect of CLA on paraoxonase 1 (PON1), one of the antioxidant proteins associated with HDL, was investigated for its protective action against oxidative inactivation as well as its stabilization activity. When cis-9 (c9),trans-11 (t11)-CLA and t10,c12-CLA were examined for their protective activity against ascorbate/Cu2−-induced inactivation of PON1 in the presence of Ca2+, two CLA isomers exhibited a remarkable protection (E max, 71–74%) in a concentration-dependent manner (50% effective concentration, 3–4 μM), characterized by a saturation pattern. Such a protective action was also reproduced with oleic acid, but not linoleic acid. Rather, linoleic acid antagonized the protective action of CLA isomers in a noncompetitive fashion. Additionally, the two CLA isomers also protected PON1 from oxidative inactivation by H2O2 or cumene hydroperoxide. The concentration-dependent protective action of CLA against various oxidative inactivation systems suggests that the protective action of CLA isomers may be mediated through their selective binding to a specific binding site in a PON1 molecule. Separately, the inactivation of PON1 by p-hydroxymercuribenzoate (PHMB), a modifier of the cysteine residue, was also prevented by CLA isomers, suggesting the possible existence of the cysteine residue in the binding site of CLA. The c9,t11-CLA isomer seems to be somewhat more effective than t10,c12-CLA in protecting against the inactivation of PON1 by either peroxides or PHMB, in contrast to the similar efficacy of these two CLA isomers in preventing ascorbate/Cu2+-induced inactivation of PON1. Separately, CLA isomers successfully stabilized PON1, but not linoleic acid. These data suggest that the two CLA isomers may play a beneficial role in protecting PON1 from oxidative inactivation as well as in its stabilization.
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