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首页> 美国卫生研究院文献>Molecular Medicine >GTK tyrosine kinase-induced alteration of IRS-protein signalling in insulin producing cells.
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GTK tyrosine kinase-induced alteration of IRS-protein signalling in insulin producing cells.

机译:GTK酪氨酸激酶诱导胰岛素产生细胞中IRS蛋白信号转导的改变。

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BACKGROUND: Insulin receptor substrate proteins (IRS) mediate various effects of insulin, including regulation of glucose homeostasis, cell growth and survival. To understand the underlying mechanisms explaining the effects of the Src-related tyrosine kinase GTK on beta-cell proliferation and survival, insulin-signalling pathways involving IRS-1 and IRS-2 were studied in islet cells and RINm5F cells overexpressing wild-type and two different mutants of the SRC-related tyrosine kinase GTK. MATERIALS AND METHODS: Islets isolated from transgenic mice and RINm5F cells overexpressing wild-type and mutant GTK were analysed for IRS-1, IRS-2, SHB, AKT and ERK phosphorylation/activity by Western blot analysis. RESULTS: RINm5F cells expressing the kinase active mutant Y504F-GTK and islet cells from GTK(Y504F) -transgenic mice exhibited reduced insulin-induced tyrosine phosphorylation of IRS-1 and IRS-2. In RINm5F cells, the diminished IRS-phosphorylation was accompanied by a reduced insulin-stimulated activation of phosphatidylinositol 3-kinase (PI3K), AKT and Extracellular Signal-Regulated Kinase, partly due to an increased basal activity. In addition, increased tyrosine phosphorylation of the SHB SH2 domain-adaptor protein and its association with IRS-2, IRS-1 and focal adhesion kinase was observed in these cells. RINm5F cells overexpressing wild-type GTK also exhibited reduced activation of IRS-2, PI3K and AKT, whereas cells expressing a GTK mutant with lower kinase activity (GTK(Y394F)) exhibited insignificantly altered responses to insulin compared to the mock transfected cells. Moreover, GTK was shown to associate with and phosphorylate SHB in transiently transfected COS-7 cells, indicating that SHB is a specific substrate for GTK. CONCLUSIONS: The results suggest that GTK signals via SHB to modulate insulin-stimulated pathways in beta cells and this may explain previous results showing an increased beta-cell mass in GTK-transgenic mice.
机译:背景:胰岛素受体底物蛋白(IRS)介导胰岛素的各种作用,包括调节葡萄糖稳态,细胞生长和存活。为了了解解释Src相关酪氨酸激酶GTK对β细胞增殖和存活的影响的潜在机制,在胰岛细胞和过表达野生型的RINm5F细胞中研究了涉及IRS-1和IRS-2的胰岛素信号通路SRC相关酪氨酸激酶GTK的不同突变体。材料与方法:通过Western blot分析从过表达野生型和突变型GTK的转基因小鼠和RINm5F细胞中分离出的胰岛的IRS-1,IRS-2,SHB,AKT和ERK磷酸化/活性。结果:表达激酶活性突变体Y504F-GTK的RINm5F细胞和来自GTK(Y504F)转基因小鼠的胰岛细胞表现出降低的胰岛素诱导的IRS-1和IRS-2酪氨酸磷酸化。在RINm5F细胞中,IRS磷酸化水平的降低伴随着胰岛素刺激的磷脂酰肌醇3-激酶(PI3K),AKT和细胞外信号调节激酶的激活减少,部分原因是基础活性增加。此外,在这些细胞中观察到SHB SH2域适应蛋白酪氨酸磷酸化的增加及其与IRS-2,IRS-1和粘着斑激酶的联系。与模拟转染细胞相比,过表达野生型GTK的RINm5F细胞也表现出IRS-2,PI3K和AKT的激活减少,而表达具有较低激酶活性的GTK突变体(GTK(Y394F))的细胞对胰岛素的反应却微不足道。此外,在瞬时转染的COS-7细胞中,GTK与SHB结合并磷酸化,表明SHB是GTK的特异性底物。结论:该结果表明GTK通过SHB信号调节β细胞中胰岛素刺激的途径,这可能解释了先前的结果,表明GTK转基因小鼠中β细胞质量增加。

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