Literature DB >> 24778187

Insulin-regulated Glut4 translocation: membrane protein trafficking with six distinctive steps.

Paul Duffield Brewer1, Estifanos N Habtemichael2, Irina Romenskaia1, Cynthia Corley Mastick3, Adelle C F Coster4.   

Abstract

The trafficking kinetics of Glut4, the transferrin (Tf) receptor, and LRP1 were quantified in adipocytes and undifferentiated fibroblasts. Six steps were identified that determine steady state cell surface Glut4: (i) endocytosis, (ii) degradation, (iii) sorting, (iv) sequestration, (v) release, and (vi) tethering/docking/fusion. Endocytosis of Glut4 is 3 times slower than the Tf receptor in fibroblasts (ken = 0.2 min(-1) versus 0.6 min(-1)). Differentiation decreases Glut4 ken 40% (ken = 0.12 min(-1)). Differentiation also decreases Glut4 degradation, increasing total and cell surface Glut4 3-fold. In fibroblasts, Glut4 is recycled from endosomes through a slow constitutive pathway (kex = 0.025-0.038 min(-1)), not through the fast Tf receptor pathway (kex = 0.2 min(-1)). The kex measured in adipocytes after insulin stimulation is similar (kex = 0.027 min(-1)). Differentiation decreases the rate constant for sorting into the Glut4 recycling pathway (ksort) 3-fold. In adipocytes, Glut4 is also sorted from endosomes into a second exocytic pathway through Glut4 storage vesicles (GSVs). Surprisingly, transfer from endosomes into GSVs is highly regulated; insulin increases the rate constant for sequestration (kseq) 8-fold. Release from sequestration in GSVs is rate-limiting for Glut4 exocytosis in basal adipocytes. AS160 regulates this step. Tethering/docking/fusion of GSVs to the plasma membrane is regulated through an AS160-independent process. Insulin increases the rate of release and fusion of GSVs (kfuseG) 40-fold. LRP1 cycles with the Tf receptor and Glut4 in fibroblasts but predominantly with Glut4 after differentiation. Surprisingly, AS160 knockdown accelerated LRP1 exocytosis in basal and insulin-stimulated adipocytes. These data indicate that AS160 may regulate trafficking into as well as release from GSVs.
© 2014 by The American Society for Biochemistry and Molecular Biology, Inc.

Entities:  

Keywords:  Adipocyte; Endocytosis; Exocytosis; Fibroblast; Glucose; Glucose Transport; Glucose Transporter Type 4 (Glut4); Insulin; Transferrin Receptor

Mesh:

Substances:

Year:  2014        PMID: 24778187      PMCID: PMC4067164          DOI: 10.1074/jbc.M114.555714

Source DB:  PubMed          Journal:  J Biol Chem        ISSN: 0021-9258            Impact factor:   5.157


  43 in total

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Authors:  H S Wiley; D D Cunningham
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Journal:  Mol Biol Cell       Date:  2004-07-14       Impact factor: 4.138

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7.  GLUT4 retention in adipocytes requires two intracellular insulin-regulated transport steps.

Authors:  Anja Zeigerer; Michael A Lampson; Ola Karylowski; David D Sabatini; Milton Adesnik; Mindong Ren; Timothy E McGraw
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8.  Physical properties of human alpha 2-macroglobulin following reaction with methylamine and trypsin.

Authors:  S L Gonias; J A Reynolds; S V Pizzo
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9.  Energy-dependent and protein synthesis-independent recycling of the insulin-sensitive glucose transport mechanism in fat cells.

Authors:  T Kono; K Suzuki; L E Dansey; F W Robinson; T L Blevins
Journal:  J Biol Chem       Date:  1981-06-25       Impact factor: 5.157

10.  Immuno-localization of the insulin regulatable glucose transporter in brown adipose tissue of the rat.

Authors:  J W Slot; H J Geuze; S Gigengack; G E Lienhard; D E James
Journal:  J Cell Biol       Date:  1991-04       Impact factor: 10.539

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8.  Glut4 Is Sorted from a Rab10 GTPase-independent Constitutive Recycling Pathway into a Highly Insulin-responsive Rab10 GTPase-dependent Sequestration Pathway after Adipocyte Differentiation.

Authors:  Paul Duffield Brewer; Estifanos N Habtemichael; Irina Romenskaia; Cynthia Corley Mastick; Adelle C F Coster
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