Abstract
BackgroundOnly a fraction of circulating insulin-like activity is due to insulin itself. The aim of this study was to determine total serum insulin-like activity mediated via the insulin receptor isoform A (IR-A) and isoform B (IR-B) by using kinase receptor activation (KIRA) assays specific for the IR-A and IR-B. MethodsThe IR-A and IR-B KIRA assays use human embryonic kidney cells which have been transfected with the human IR-A or IR-B gene and quantify serum-mediated phosphorylation of the IR. ResultsBoth IR KIRA assays were sensitive (detection limit 32pmol/L) and precise (intra- and inter assay CV: <12% and <15%). The EC50s of insulin, IGF-I and IGF-II were 1.4, 11.2 and 6.7nmol/L for the IR-A KIRA assay, and 1.3, 31.0 and 15.7nmol/L for the IR-B KIRA assay.The operational range of both assays allowed for determination of total insulin-like activity in human serum. Analysis of serum samples showed that there was a significant positive correlation between serum insulin-like and immunoreactive insulin concentrations (IR-A: r=0.56, p=0.01, IR-B: r=0.68, p=0.001). Importantly, addition of IGF-I or IGF-II antibodies to human serum samples could substantially decrease the endpoint signal in both KIRA assays. ConclusionsWe showed that serum IGF-I and IGF-II may substantially contribute to IR signalling. Since IR isoform specific KIRA assays also take into account the contribution of IGFs present in serum on IR signalling, they may help to gain more insight into the roles of IGF mediated IR-A and IR-B activation in health and disease.
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