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A Kowluru, S E Seavey, G Li, R L Sorenson, A J Weinhaus, R Nesher, M E Rabaglia, J Vadakekalam, S A Metz
J Clin Invest. 1996;
98(2):540
doi:10.1172/JCI118822
Abstract |
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everal GTP-binding proteins (G-proteins) undergo post-translational modifications (isoprenylation and carboxyl methylation) in pancreatic beta cells. Herein, two of these were identified as CDC42 and rap 1, using Western blotting and immunoprecipitation. Confocal microscopic data indicated that CDC42 is localized only in islet endocrine cells but not in acinar cells of the pancreas. CDC42 undergoes a guanine nucleotide-specific membrane association and carboxyl methylation in normal rat islets, human islets, and pure beta (HIT or INS-1) cells. GTPgammaS-dependent carboxyl methylation of a 23-kD protein was also demonstrable in secretory granule fractions from normal islets or beta cells. AFC (a specific inhibitor of prenyl-cysteine carboxyl methyl transferases) blocked the carboxyl methylation of CDC42 in five types of insulin-secreting cells, without blocking GTPgammaS-induced translocation, implying that methylation is a consequence (not a cause) of transfer to membrane sites. High glucose (but not a depolarizing concentration of K+) induced the carboxyl methylation of CDC42 in intact cells, as assessed after specific immunoprecipitation. This effect was abrogated by GTP depletion using mycophenolic acid and was restored upon GTP repletion by coprovision of guanosine. In contrast, although rap 1 was also carboxyl methylated, it was not translocated to the particulate fraction by GTPgammaS; furthermore, its methylation was also stimulated by 40 mM K+ (suggesting a role which is not specific to nutrient stimulation). AFC also impeded nutrient-induced (but not K+-induced) insulin secretion from islets and beta cells under static or perifusion conditions, whereas an inactive structural analogue of AFC failed to inhibit insulin release. These effects were reproduced not only by S-adenosylhomocysteine (another methylation inhibitor), but also by GTP depletion. Thus, the glucose- and GTP-dependent carboxyl methylation of G-proteins such as CDC42 is an obligate step in the stimulus-secretion coupling of nutrient-induced insulin secretion, but not in the exocytotic event itself. Furthermore, AFC blocked glucose-activated phosphoinositide turnover, which may provide a partial biochemical explanation for its effect on secretion, and implies that certain G-proteins must be carboxyl methylated for their interaction with signaling effector molecules, a step which can be regulated by intracellular availability of GTP.
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Protein Prenylation Part B
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Glucose activates prenyltransferases in pancreatic islet beta-cells.
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Biochemical and Biophysical Research Communications
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2010 |
Down-regulation of expression and function of nucleoside diphosphate kinase in insulin-secreting β-cells under in vitro conditions of glucolipotoxicity
Rajakrishnan Veluthakal, Madathilparambil V. Suresh, Anjaneyulu Kowluru
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Mol Cell Biochem
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2009 |
Lack of cholesterol mobilization in islets of hormone-sensitive lipase deficient mice impairs insulin secretion
Sara Larsson, Nils Wierup, Frank Sundler, Lena Eliasson, Cecilia Holm
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Biochemical and Biophysical Research Communications
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Emerging roles for protein histidine phosphorylation in cellular signal transduction: lessons from the islet β-cell : J. Cell. Mol. Med. Vol 12, No 5B, 2008
Anjaneyulu Kowluru
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Journal of Cellular and Molecular Medicine
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2008 |
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