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(Received for publication, April 8, 1997, and in revised form, May 14, 1997)
From the Gifford Laboratories for Diabetes Research and Departments
of Biochemistry and Internal Medicine, University of Texas
Southwestern Medical Center, Dallas, Texas 75235
Insulin secretion from beta cells in
the islets of Langerhans can be stimulated by a number of
metabolic fuels, including glucose and glyceraldehyde, and is
thought to be mediated by metabolism of the secretagogues and an
attendant increase in the ATP:ADP ratio. Curiously, glycerol fails to
stimulate insulin secretion, even though it has been reported that
islets contain abundant glycerol kinase activity and oxidize glycerol
efficiently. We have reinvestigated this point and find that rat islets
and the well differentiated insulinoma cell line INS-1 contain
negligible glycerol kinase activity. A recombinant adenovirus
containing the bacterial glycerol kinase gene (AdCMV-GlpK) was
constructed and used to express the enzyme in islets and INS-1 cells,
resulting in insulin secretion in response to glycerol. In
AdCMV-GlpK-treated INS-1 cells a greater proportion of glycerol is
converted to lactate and a lesser proportion is oxidized compared with
glucose. The two fuels are equally potent as insulin secretagogues,
despite the fact that oxidation of glycerol at its maximally effective dose (2-5 mM) occurs at a rate that is similar to
the rate of glucose oxidation at its basal, nonstimulatory
concentration (3 mM). We also investigated the possibility
that glycerol may signal via expansion of the glycerol phosphate pool
to allow enhanced fatty acid esterification and formation of complex
lipids. Addition of Triacsin-C, an inhibitor of long-chain acyl-CoA
synthetase, to AdCMV-GlpK-treated INS-1 cells did not inhibit
glycerol-stimulated insulin secretion despite the fact that it blocked
glycerol incorporation into cellular lipids. We conclude from these
studies that glycerol kinase expression is sufficient to activate
glycerol signaling in beta cells, showing that the failure of normal
islets to respond to this substrate is due to a lack of this enzyme
activity. Further, our studies show that glycerol signaling is not
linked to esterification or oxidation of the substrate, but is likely
mediated by its metabolism in the glycerol phosphate shuttle and/or the
distal portion of the glycolytic pathway, either of which can lead to
production of ATP and an increased ATP:ADP ratio.
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