1994 Fiscal Year Final Research Report Summary

Study on the mechanism of insulin action on glucose transport

Research Project

Project/Area Number	05670837
Research Category	Grant-in-Aid for General Scientific Research (C)
Allocation Type	Single-year Grants
Research Field	内分泌・代謝学
Research Institution	Gunma University Institute For Molecular and Cellular Regulation
Principal Investigator	SHIBATA Hiroshi Gunma University, Institute for Molecular and Cellular Regulation, Department of Cell Biology, lecturer, 生体調節研究所, 講師 (20235584)
Project Period (FY)	1993 – 1994
Keywords	insulin / glucose transporter / G-protein
Research Abstract	Effects of guanine nucleotides on either exocytosis or endocytosis of GLUT4 were examined in electrically permeabilized rat adipocytes by using D^k- (62-85), a MHC class l-derived peptide. Reversal of glucose transport activity which had been stimulated with insulin was completely blocked and the activity was rather enhanced 25% in the presence of D^k- (62-85), indicating that the peptide blocked endocytosis of GLUT4. In agreement with this notion, endocytosis of trypsin-cleaved 35 kDa fragment of GLUT4 was almost completely inhibited by the peptide. Therefore, in the presence of the peptide, exclusively exocytotic accumulation of GLUT4 on the cell surface could be measured. Insulin-stimulated glucose transport activity was enhanced about 50% in the presence of D^k- (62-85) while the basal transport activity was stimulated only slightly. Although GTP_<gamma>S augmented glucose transport to the same extent as insulin in the absence of D^k- (62-85), GTPgS-stimulated glucose transport was only 60% of the insulin effect in the presence of the peptide : the effects of insulin was markedly enhanced by the peptide whereas glucose transport induced by GTPgammaS was not affected, suggesting that GTP_<gamma>S has a similar effect to the peptide. In fact, endocytosis of 35kDa fragment of GLUT4 was markedly inhibited by GTPgammaS.In addition, GLUT4 endocytosis was accelerated by GTP but was inhibited by GDPbetaS.These results indicate that GTPgammaS induces translocation of GLUT4 by both stimulating exocytosis and inhibiting endocytosis. Distinct types of GTP-binding proteins are involved in exocytosis and endocytosis of GLUT4.

Research Products
(2 results)

All Other

All Publications (2 results)

[Publications] Shibata,H.,Suzuki,Y.,Omata,W.,Tanaka,S.,Kojima,I.: "Dissection of GLUT4 recycling pathway into exocytosis and endocytosis in rat adipocytes:Evidence that GTP‐binding proteins are involved in both processes." J.Biol.Chem.(印刷中). (1995)
- Description
  「研究成果報告書概要(和文)」より
[Publications] Shibata, H., Suzuki, Y., Omata, W., Tanaka, S.and Kojima, I.: "Dissection of GLUT4 recycling pathway into exocytosis and endocytosis in rat adipocytes : Evidence that GTP-binding proteins are involved in both processes." J.Biol.Chem.1995 (in press).
- Description
  「研究成果報告書概要(欧文)」より

1994 Fiscal Year Final Research Report Summary

Study on the mechanism of insulin action on glucose transport

Principal Investigator

SHIBATA Hiroshi Gunma University, Institute for Molecular and Cellular Regulation, Department of Cell Biology, lecturer, 生体調節研究所, 講師 (20235584)

Research Products

[Publications] Shibata,H.,Suzuki,Y.,Omata,W.,Tanaka,S.,Kojima,I.: "Dissection of GLUT4 recycling pathway into exocytosis and endocytosis in rat adipocytes:Evidence that GTP‐binding proteins are involved in both processes." J.Biol.Chem.(印刷中). (1995)

Description

[Publications] Shibata, H., Suzuki, Y., Omata, W., Tanaka, S.and Kojima, I.: "Dissection of GLUT4 recycling pathway into exocytosis and endocytosis in rat adipocytes : Evidence that GTP-binding proteins are involved in both processes." J.Biol.Chem.1995 (in press).

Description