Alteration of the Malonyl-CoA/Carnitine Palmitoyltransferase I Interaction in the β-Cell Impairs Glucose-Induced Insulin Secretion
- Laura Herrero1,
- Blanca Rubí2,
- David Sebastián1,
- Dolors Serra1,
- Guillermina Asins1,
- Pierre Maechler2,
- Marc Prentki3 and
- Fausto G. Hegardt1
- 1Department of Biochemistry and Molecular Biology, University of Barcelona, School of Pharmacy, Barcelona, Spain
- 2Department of Cell Physiology and Metabolism, University Medical Centre, Geneva, Switzerland
- 3Molecular Nutrition Unit, Department of Nutrition, University of Montreal and the Montreal Diabetes Research Center, Montreal, Quebec, Canada
- Address correspondence and reprint requests to Fausto G. Hegardt, Department of BiochemistryMolecular Biology, School of Pharmacy, Diagonal 643, E-08028 Barcelona, Spain. E-mail: fgarciaheg{at}ub.edu
Abstract
Carnitine palmitoyltransferase I, which is expressed in the pancreas as the liver isoform (LCPTI), catalyzes the rate-limiting step in the transport of fatty acids into the mitochondria for their oxidation. Malonyl-CoA derived from glucose metabolism regulates fatty acid oxidation by inhibiting LCPTI. To examine directly whether the availability of long-chain fatty acyl-CoA (LC-CoA) affects the regulation of insulin secretion in the β-cell and whether malonyl-CoA may act as a metabolic coupling factor in the β-cell, we infected INS(832/13) cells and rat islets with an adenovirus encoding a mutant form of LCPTI (Ad-LCPTI M593S) that is insensitive to malonyl-CoA. In Ad-LCPTI M593S–infected INS(832/13) cells, LCPTI activity increased sixfold. This was associated with enhanced fatty acid oxidation, at any glucose concentration, and a 60% suppression of glucose-stimulated insulin secretion (GSIS). In isolated rat islets in which LCPTI M593S was overexpressed, GSIS decreased 40%. The impairment of GSIS in Ad-LCPTI M593S–infected INS(832/13) cells was not recovered when cells were incubated with 0.25 mmol/l palmitate, indicating the deep metabolic influence of a nonregulated fatty acid oxidation system. At high glucose concentration, overexpression of a malonyl-CoA–insensitive form of LCPTI reduced partitioning of exogenous palmitate into lipid esterification products and decreased protein kinase C activation. Moreover, LCPTI M593S expression impaired KATP channel–independent GSIS in INS(832/13) cells. The LCPTI M593S mutant caused more pronounced alterations in GSIS and lipid partitioning (fat oxidation, esterification, and the level of nonesterified palmitate) than LCPTI wt in INS(832/13) cells that were transduced with these constructs. The results provide direct support for the hypothesis that the malonyl-CoA/CPTI interaction is a component of a metabolic signaling network that controls insulin secretion.
- ACC, acetyl-CoA carboxylase
- ASP, acid-soluble product
- CE, cholesterol ester
- CPTI, carnitine palmitoyltransferase I
- DAG, diacylglycerol
- ECF, enhanced chemifluorescence
- FFA, free fatty acid
- GSIS, glucose-stimulated insulin secretion
- KRBH, Krebs-Ringer bicarbonate HEPES
- LC-CoA, long-chain fatty acyl-CoA
- LCPTI, liver carnitine palmitoyltransferase I
- MCD, malonyl-CoA decarboxylase
- MCDc, MCD in the cytosol
- NEFA, nonesterified fatty acid
- NE palm, nonesterified labeled palmitate
- PKC, protein kinase C
Footnotes
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- Accepted October 18, 2004.
- Received July 24, 2004.
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