Peroxisome Proliferator-Activated Receptor- - Coactivator-1 ( PGC-1 ) expression in the liver and skeletal muscles soleus and plantaris of male Wistar rats subjected to chronic voluntary exercise

INTRODUCTION: The Peroxisome Proliferator-Activated Receptor- - Coactivator 1 ( PGC-1 e ) is a protein responsible for the connection between environmental stimuli and cell metabolic response. Its presence is important in fat tissue, hepatic and skeletal muscle and in animals on brown fat tissue. Interact with nuclear receptors modulating the mitochondrial biogenesis and maintain thermal energy balance with the environment. Diminished of PGC-1 expression and oxidative phophorylation has been associated to insulin resistance in diseases like Type 2 Diabetes and Metabolic Syndrome. OBJECTIVES: To evaluate the effects of exercise on the PGC-1 expression in target tissues of insulin, such as liver and skeletal muscles soleus (SOL) and plantaris (PLA) of male Wistar rats and correlates with insulin sensitivity. METHODOLOGY: Male Wistar rats 190±15g, n = 24, divided randomly into 2 groups: Ex ( physical exercise ) and Sd ( sedentary ), respectively placed in a voluntary running wheel cage or a standard cage for five weeks. At the end of study, after fasting for 4 hours, blood was collected for measurements of glucose ( GLU ), insulin ( INS ) and free fatty acids ( FFA ) then the animals were submitted to Test of Suppression Endogenous Glucose and Insulin, with infusion during 180 minutes of solution GLU ( 20mg/kg/min ) + INS ( 5mU/kg/min ); blood samples was collected at 140, 150, 160, 170 and 180 minutes. Finished the test and still anesthetized, the tissues were removed: liver ( LIV ), skeletal muscle ( SOL and PLA ) that were immediately frozen in liquid nitrogen and stored at -70ºC until analysis. The PGC-1 expression was evaluated by Western Blotting with polyclonal antibody anti-PGC-1. Statistical analysis by unpaired Students t test with significance level 5%. RESULTS: the data refer to the mean and standard error of individual values. The distance covered per day during last week ( km / day ) by Ex group was efficient ( 5,61 ± 0,67 ). There was no difference in weight ( g ) of rats between Ex and Sd groups ( 355,85 ± 9,51 x 375,68 ± 5,30 ) NS. The values of fasting GLU were similar between groups ( mg/dl ) ( 117,6 ± 3,7 x 122,4 ± 2,6 ) NS. However INS and FFA were lower in group Ex: INS ( ng/ml ) ( 0,68 ± 0,12 x 1,45 ± 0,14 ) p < 0,001 and FFA ( mEq/L ) ( 1,12 ± 0,11 x 1,60 ± 0,11 ) p < 0,006. During the suppression test the values of GLU and INS on stability step were similar between groups ( expressed in area under curve ): AUC GlU ( mg/dl/min ) ( 2,77 ± 0,12 x 2,95 ± 0,07 ) NS; AUC INS ( ng/ml/min ) ( 0,81 ± 0,15 x 0,99 ± 0,09 ) NS. The PGC-1 expression was greater in PLA of rats Ex than Sd group, and there was no difference in LIV and SOL between groups. CONCLUSION: The physical exercise during five weeks in voluntary running wheel increased the insulin sensitivity and fasting free fatty acids oxidation. The improvement of insulin sensitivity was associated with higher PGC-1 expression on PLA muscle only. These data suggest that increasing insulin sensibility on fasting is not associated with increasing of the PGC-1 expression in others targets tissues of insulin action, such as LIV and SOL, in this study model. (AU)