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Diabetes, Vol 45, Issue 2 190-198, Copyright © 1996 by American Diabetes Association
Evidence for an anaplerotic/malonyl-CoA pathway in pancreatic beta-cell nutrient signaling
T Brun, E Roche, F Assimacopoulos-Jeannet, BE Corkey, KH Kim and M Prentki
Department of Nutrition, University of Montreal Medical School, Quebec, Canada.
A metabolic model of fuel sensing has been proposed in which malonyl-CoA
and long-chain acyl-CoA esters may act as coupling factors in
nutrient-induced insulin release (Prentki M, Vischer S, Glennon MC, Regazzi
R, Deeney J, Corkey BE: Malonyl-CoA and long chain acyl-CoA esters as
metabolic coupling factors in nutrient-induced insulin secretion. J Biol
Chem 267:5802-5810, 1992). To gain further insight into the control of
malonyl-CoA content in islet tissue, we have studied the short- and
long-term regulation of acetyl-CoA carboxylase (ACC) and fatty acid
synthase (FAS) in the beta-cell. These enzymes catalyze the formation of
malonyl-CoA and its usage for de novo fatty acid biogenesis. ACC mRNA,
protein, and enzymatic activity are present at appreciable levels in rat
pancreatic islets and clonal beta-cells (HIT cells). Glucose addition to
HIT cells results in a marked increase in ACC activity that precedes the
initiation of insulin release. Fasting does not modify the ACC content of
islets, whereas it markedly downregulates that of lipogenic tissues. This
indicates differential regulation of the ACC gene in lipogenic tissues and
the islets of Langerhans. FAS is very poorly expressed in islet tissue, yet
ACC is abundant. This demonstrates that the primary function of malonyl-CoA
in the beta-cells is to regulate fatty acid oxidation, not to serve as a
substrate for fatty acid biosynthesis. The anaplerotic enzyme pyruvate
carboxylase, which allows the replenishment of citric acid cycle
intermediates needed for malonyl-CoA production via citrate, is abundant in
islet tissue. Glucose causes an elevation in beta (HIT)-cell citrate that
precedes secretion, and only those nutrients that can elevate citrate
induce effective insulin release. The results provide new evidence in
support of the model and explain why malonyl-CoA rises markedly and rapidly
in islets upon glucose stimulation: 1) glucose elevates citrate, the
precursor of malonyl-CoA; 2) glucose enhances ACC enzymatic activity; and
3) malonyl-CoA is not diverted to lipids. The data suggest that ACC is a
key enzyme in metabolic signal transduction of the beta-cell and provide
evidence for the concept that an anaplerotic/malonyl-CoA pathway is
implicated in insulin secretion.

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E. Roche, F. Assimacopoulos-Jeannet, L. A. Witters, B. Perruchoud, G. Yaney, B. Corkey, M. Asfari, and M. Prentki
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Copyright © 1996 by the American Diabetes Association.
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