Irs1 and Irs2 signaling is essential for hepatic glucose homeostasis and systemic growth
Xiaocheng Dong, … , Xianjin Yi, Morris F. White
Xiaocheng Dong, … , Xianjin Yi, Morris F. White
Published January 4, 2006
Citation Information: J Clin Invest. 2006;116(1):101-114. https://doi.org/10.1172/JCI25735.
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Research Article Metabolism

Irs1 and Irs2 signaling is essential for hepatic glucose homeostasis and systemic growth

Abstract

Insulin receptor substrates, including Irs1 and Irs2, integrate insulin and IGF receptor signals with heterologous pathways to coordinate growth and metabolism. Since Irs2 is thought to be especially important in hepatic nutrient homeostasis, we deleted Irs1 from hepatocytes of WT mice (called LKO) or genetically insulin-resistant Irs1–/– mice (called LKO::Irs1–/–). Viable LKO::Irs1–/– mice were 70% smaller than WT or LKO mice, and 40% smaller than Irs1–/– mice. Hepatic insulin receptors were functional in all the mice, but insulin signaling via the Akt—FoxO1 pathway was reduced in Irs1–/– and LKO liver, and undetected in LKO::Irs1–/– liver; however, Gsk3β phosphorylation (Ser9) and hepatic glycogen stores were nearly normal in all of the mice. LKO and Irs1–/– mice developed insulin resistance and glucose intolerance that never progressed to diabetes, whereas LKO::Irs1–/– mice developed hyperglycemia and hyperinsulinemia immediately after birth. Regardless, few hepatic genes changed expression significantly in Irs1–/– or LKO mice, whereas hundreds of genes changed in LKO::Irs1–/– mice — including elevated levels of Pck1, G6pc, Ppargc1, Pparg, and Igfbp1. Thus, signals delivered by Irs1 or Irs2 regulate hepatic gene expression that coordinates glucose homeostasis and systemic growth.

Authors

Xiaocheng Dong, Sunmin Park, Xueying Lin, Kyle Copps, Xianjin Yi, Morris F. White

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Figure 6

Insulin signaling in liver, muscle, and white adipose tissue.

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Insulin signaling in liver, muscle, and white adipose tissue. Mice in ea...
Mice in each experimental group were fasted overnight and stimulated with insulin (Ins) by i.v. injection. Four minutes after injection, the liver, muscle, and perigonadal white adipose tissue were isolated and frozen immediately in liquid nitrogen. (A) Insulin receptor level and tyrosine phosphorylation in liver extracts. Each sample was immunoprecipitated with antibodies against the insulin receptor (αIR), Irs1, or Irs2. After SDS-PAGE, the samples were immunoblotted with αIR, or with antibodies against phosphotyrosine (αpY). (B) Erk1 and Erk2 and their phosphorylated forms (phospho-Thr202/Tyr204) were analyzed with specific antibodies in the liver lysates of each experimental group. (C) PI3K activity was assayed in vitro using the liver extracts from each group after immunoprecipitation with anti-phosphotyrosine antibodies. The data represent the percentage of PI3K activity normalized against that measured for the fIrs2 mice. PIP3, 32P-labeled phosphatidylinositol-3,4,5-triphosphate. (D) The phosphorylation of Akt, FoxO1, and Prkaa1 was determined in the liver lysates of each experimental group. After SDS-PAGE, the samples were immunoblotted with phosphospecific antibodies against Akt (αpAkt, phospho-Ser473), FoxO1 (αpFoxO1, phospho-Ser256), or Prkaa1 (αpPrkaa1, phospho-Thr172). The expressions of Akt and Prkaa1 were also determined in the liver extracts by immunoblotting with specific antibodies. (E and F) Phosphorylation of Akt and Erk1/2 was analyzed by immunoblotting as described for liver using tissue lysates from epididymal fat or hind-limb skeletal muscle of LKO::Irs1–/–, Irs1–/–, LKO, and control fIrs2 mice.