The G972R variant of the insulin receptor substrate-1 gene impairs insulin signaling and cell differentiation in 3T3L1 adipocytes; treatment with a PPARgamma agonist restores normal cell signaling and differentiation

F Sentinelli; E Filippi; M G Cavallo; S Romeo; M Fanelli; M G Baroni

doi:10.1677/joe.1.06290

The G972R variant of the insulin receptor substrate-1 gene impairs insulin signaling and cell differentiation in 3T3L1 adipocytes; treatment with a PPARgamma agonist restores normal cell signaling and differentiation

J Endocrinol. 2006 Feb;188(2):271-85. doi: 10.1677/joe.1.06290.

Authors

F Sentinelli¹, E Filippi, M G Cavallo, S Romeo, M Fanelli, M G Baroni

Affiliation

¹ Department of Clinical Sciences, Division of Endocrinology, Policlinico Umberto I, University of Rome 'La Sapienza', Viale del Policlinico 155, 00161 Rome, Italy.

PMID: 16461553
DOI: 10.1677/joe.1.06290

Abstract

The insulin receptor substrate-1 (IRS-1) plays a central role in insulin sensitivity, and association studies have shown that the IRS-1 G972R variant is a risk factor for insulin resistance. However, how this mutation may lead to impaired insulin sensitivity is still to be determined. Our study aimed to evaluate, after transfection of the IRS-1 G972R variant in 3T3L1 adipocytes, the effect of this mutation on insulin signaling and on cell differentiation. The 3T3L1 cells were transfected with pcDNA3 expression vector containing either the human wild-type IRS-1 or the G972R variant. After induction of differentiation, the 3T3L1 transfected with wild-type IRS-1 differentiated in 6-8 days, while the cells transfected with G972R variant did not differentiate. To determine whether the defect in IRS-1 was responsible for this, we analyzed the expression of several genes involved in the insulin signaling pathway. Results showed that PPARgamma expression was significantly reduced in cells transfected with the mutated IRS-1, together with a significant decrease in binding of phosphatidylinositol-3 kinase (PI 3-kinase) to IRS-1 G972R and in PI 3-kinase activity. In addition, we observed that the interaction between the insulin receptor (IR) and the IRS-1 G972R protein was increased and that the autophosphorylation of the IR was significantly inhibited in 3T3L1-G972R cells compared with 3T3L1-WT. Treatment of the 3T3L1-G972R cells with pioglitazone (PIO), a PPARgamma agonist, restored differentiation with higher level of PPARgamma expression and restoration of PI 3-kinase binding to IRS-1 G972R and PI 3-kinase activity. IR autophosphorylation was also increased. Withdrawal of PIO in fully differentiated 3T3L1-G972R cells determined the reappearance of the insulin signaling defect. Finally, we observed higher levels of IRS-2 expression, suggesting that IRS-2 may play a more important role in adipocyte insulin signaling. In conclusion, IRS-1 G972R variant impairs insulin signaling, and treatment with PPARgamma agonist restores the normal phenotype of 3T3L1 cells.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

3T3 Cells
Adipocytes / drug effects
Adipocytes / physiology*
Animals
Cell Differentiation / drug effects
Cell Differentiation / genetics
Cell Differentiation / physiology
Humans
Hypoglycemic Agents / pharmacology*
Insulin / metabolism*
Insulin Receptor Substrate Proteins
Mice
Mitogen-Activated Protein Kinases / metabolism
Mutation
PPAR gamma / agonists*
PPAR gamma / analysis
Phosphatidylinositol 3-Kinases / metabolism
Phosphoproteins / genetics*
Phosphorylation
Pioglitazone
Serine / metabolism
Signal Transduction / drug effects
Signal Transduction / genetics*
Thiazolidinediones / pharmacology*
Threonine / metabolism
Transfection
Tyrosine / metabolism

Substances

Hypoglycemic Agents
IRS1 protein, human
Insulin
Insulin Receptor Substrate Proteins
Irs1 protein, mouse
PPAR gamma
Phosphoproteins
Thiazolidinediones
Threonine
Tyrosine
Serine
Phosphatidylinositol 3-Kinases
Mitogen-Activated Protein Kinases
Pioglitazone