Changes in antioxidant defense status in hypercholesterolemic rats treated with Ajuga iva

The aim of the study was to investigate the effect of aqueous extract of Ajuga iva ( Ai) on serum and tissues lipid peroxidation as well as antioxidant enzymes activities in red blood cells (RBC) and tissues, in high hypercholesterolemic rats (HC). Male Wistar rats ( n=12) were fed on 1% cholesterol...

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Published in:Phytomedicine (Stuttgart) 2008-06, Vol.15 (6), p.453-461
Main Authors: Bouderbala, S., Lamri-Senhadji, M., Prost, J., Lacaille-Dubois, M.A., Bouchenak, M.
Format: Article
Language:English
Subjects:
Ajuga
Ajuga iva
Animals
Antioxidant enzyme
Antioxidants - metabolism
Body Weight - drug effects
Bugleweed
Care and treatment
Chemical properties
Cholesterol - blood
Cholesterol, Dietary
Eating - drug effects
Erythrocytes - enzymology
Glutathione - metabolism
Health aspects
Hypercholesterolemia
Hypercholesterolemia - drug therapy
Hypercholesterolemic rat
Lipid peroxidation
Lipid Peroxidation - drug effects
Male
Nitric Oxide - metabolism
Physiological aspects
Phytotherapy
Plant Extracts - pharmacology
Plant Extracts - therapeutic use
Rats
Rats, Wistar
TBARS
Vitamins - blood
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Summary:The aim of the study was to investigate the effect of aqueous extract of Ajuga iva ( Ai) on serum and tissues lipid peroxidation as well as antioxidant enzymes activities in red blood cells (RBC) and tissues, in high hypercholesterolemic rats (HC). Male Wistar rats ( n=12) were fed on 1% cholesterol-enriched diet for 15 d. After this adaptation phase, hypercholesterolemic rats (total cholesterol=6.5±0.6 mol/l) were divided into two groups fed the same diet and treated or not with Ai for 15 d. Thiobarbituric acid reactive substances (TBARS) concentrations in serum, LDL-HDL 1, HDL 2 and HDL 3 were respectively, 5-, 7.8-, 2.3- and 5-fold lower in Ai treated than untreated hypercholesterolemic groups. TBARS concentrations were 1.4-fold lower in heart and 2.8-fold higher in kidney in Ai-HC treated than untreated HC group. Superoxide dismutase activity was respectively, 1.2- and 1.4-fold higher in RBC and muscle in Ai treated than untreated group. In RBC, Ajuga iva treatment enhanced glutathione peroxidase (GSH-Px) (+9%) and glutathione reductase (GSSH-Red) (+12%) in Ai-HC treated than untreated HC group. GSSH-Red activity was 1.4- and 1.5-fold higher in adipose tissue and heart, respectively and 3.7-fold lower in kidney in Ai treated than untreated group. Liver catalase activity was 1.6-fold higher in Ai treated than untreated group. Adipose tissue and muscle total glutathione content represented in Ai treated group 35% and 36% of the value noted in untreated group. Nitric oxide values of liver, adipose tissue and heart were 3.3-, 2.5- and 3.4-fold higher in Ai-HC than HC group. Ajuga iva treatment enhanced α-tocopherol contents (+25%) in Ai treated than untreated group. In conclusion, Ajuga iva treatment is more effective to improve the antioxidant capacity of RBC than that of tissues. Indeed, Ai is able to reduce the oxidative stress in hypercholesterolemic rats by increasing the antioxidant enzymes activity.
ISSN:0944-7113
1618-095X
DOI:10.1016/j.phymed.2007.10.001