TY - JOUR
T1 - Inhibition of mitochondrial fatty acid oxidation in vivo only slightly suppresses gluconeogenesis but enhances clearance of glucose in mice
AU - Derks, Terry G J
AU - van Dijk, Theo H
AU - Grefhorst, Aldo
AU - Rake, Jan-Peter
AU - Smit, G Peter A
AU - Kuipers, Folkert
AU - Reijngoud, Dirk-Jan
PY - 2008/3
Y1 - 2008/3
N2 - Mitochondrial fatty acid oxidation (mFAO) is considered to be essential for driving gluconeogenesis (GNG) during fasting. However, quantitative in vivo data on de novo synthesis of glucose-6-phosphate upon acute inhibition of mFAO are lacking. We assessed hepatic glucose metabolism in vivo after acute inhibition of mFAO by 30 mg kg(-1) 2-tetradecylglycidic acid (TDGA) in hypoketotic hypoglycemic male C57BL/6J mice by the infusion of [U-C-13]glucose, [2-C-13]glycerol, [1-H-2] galactose, and paracetamol for 6 hours, which was followed by mass isotopomer distribution analysis in blood glucose and urinary paracetamol-glucuronide. During TDGA treatment, endogenous glucose production was unaffected (127 +/- 10 versus 118 +/- 7 mu mol kg(-1) minute(-1), control versus TDGA, not significant), but the metabolic clearance rate of glucose was significantly enhanced (15.9 +/- 0.9 versus 26.3 +/- 1.1 mL kg(-1) minute(-1), control versus TDGA, P <0.05). In comparison with control mice, de novo synthesis of glucose-6-phosphate (G6P) was slightly decreased in TDGA-treated mice (108 +/- 19 versus 85 +/- 6 mu mol kg(-1) minute(-1), control versus TDGA, P <0.05). Recycling of glucose was decreased upon TDGA treatment (26 +/- 14 versus 12 4 mu mol kg(-1) minute(-1), control versus TDGA, P <0.05). Hepatic messenger RNA (mRNA) levels of genes encoding enzymes involved in de novo G6P synthesis were unaltered, whereas glucose-6-phosphate hydrolase mRNA expressions were increased in TDGA-treated mice. Glucokinase and pyruvate kinase mRNA levels were significantly decreased, whereas pyruvate dehydrogenase kinase isozyme 4 expression was increased 30-fold; this suggested decreased glycolytic activity. Conclusion: Acute pharmacological inhibition of mFAO using TDGA had no effect on endogenous glucose production and only a marginal effect on de novo G6P synthesis. Hence, fully active mFAO is not essential for maintenance of hepatic GNG in vivo in fasted mice.
AB - Mitochondrial fatty acid oxidation (mFAO) is considered to be essential for driving gluconeogenesis (GNG) during fasting. However, quantitative in vivo data on de novo synthesis of glucose-6-phosphate upon acute inhibition of mFAO are lacking. We assessed hepatic glucose metabolism in vivo after acute inhibition of mFAO by 30 mg kg(-1) 2-tetradecylglycidic acid (TDGA) in hypoketotic hypoglycemic male C57BL/6J mice by the infusion of [U-C-13]glucose, [2-C-13]glycerol, [1-H-2] galactose, and paracetamol for 6 hours, which was followed by mass isotopomer distribution analysis in blood glucose and urinary paracetamol-glucuronide. During TDGA treatment, endogenous glucose production was unaffected (127 +/- 10 versus 118 +/- 7 mu mol kg(-1) minute(-1), control versus TDGA, not significant), but the metabolic clearance rate of glucose was significantly enhanced (15.9 +/- 0.9 versus 26.3 +/- 1.1 mL kg(-1) minute(-1), control versus TDGA, P <0.05). In comparison with control mice, de novo synthesis of glucose-6-phosphate (G6P) was slightly decreased in TDGA-treated mice (108 +/- 19 versus 85 +/- 6 mu mol kg(-1) minute(-1), control versus TDGA, P <0.05). Recycling of glucose was decreased upon TDGA treatment (26 +/- 14 versus 12 4 mu mol kg(-1) minute(-1), control versus TDGA, P <0.05). Hepatic messenger RNA (mRNA) levels of genes encoding enzymes involved in de novo G6P synthesis were unaltered, whereas glucose-6-phosphate hydrolase mRNA expressions were increased in TDGA-treated mice. Glucokinase and pyruvate kinase mRNA levels were significantly decreased, whereas pyruvate dehydrogenase kinase isozyme 4 expression was increased 30-fold; this suggested decreased glycolytic activity. Conclusion: Acute pharmacological inhibition of mFAO using TDGA had no effect on endogenous glucose production and only a marginal effect on de novo G6P synthesis. Hence, fully active mFAO is not essential for maintenance of hepatic GNG in vivo in fasted mice.
KW - ISOTOPOMER DISTRIBUTION ANALYSIS
KW - CARNITINE PALMITOYL TRANSFERASE
KW - DE-NOVO SYNTHESIS
KW - RAT-LIVER
KW - 2-TETRADECYLGLYCIDIC ACID
KW - HEPATIC GLUCONEOGENESIS
KW - INSULIN SENSITIVITY
KW - BETA-OXIDATION
KW - DEFICIENT MICE
KW - FLUX
U2 - 10.1002/hep.22101
DO - 10.1002/hep.22101
M3 - Article
C2 - 18302288
SN - 0270-9139
VL - 47
SP - 1032
EP - 1042
JO - Hepatology
JF - Hepatology
IS - 3
ER -