Rakatzi Irini, Ramrath Stefanie, Ledwig Daniela, Dransfeld Olaf, Bartels Thomas, Seipke Gerhard, Eckel Jürgen
Department of Clinical Biochemistry and Pathobiochemistry, German Diabetes Research Institute, Düsseldorf, Germany.
Diabetes. 2003 Sep;52(9):2227-38. doi: 10.2337/diabetes.52.9.2227.
The potentially enhanced mitogenic activity of insulin analogs represents a safety risk that requires detailed analysis of new analogs considered for therapeutic applications. We assessed the signaling properties and mitogenic potency of two novel rapid-acting insulin analogs, Lys(B3),Glu(B29) insulin (HMR 1964) and Lys(B3),Ile(B28) insulin (HMR 1153) using myoblasts and cardiomyocytes. In myoblasts, both binding and internalization were two- to threefold higher for Asp(B10) insulin and HMR 1153 when compared with HMR 1964 and regular insulin. This finding correlated with a prominent Shc/IGF-I receptor interaction, tyrosine phosphorylation of Shc, activation of extracellular signal-regulated protein kinase (ERK)-1 and -2, and stimulation of DNA synthesis by HMR 1153 and Asp(B10) insulin. In contrast, HMR 1964 produced a marginal activation of the Shc/ERK kinase cascade and was equipotent to insulin in stimulating DNA synthesis in myoblasts. Further, the in vivo growth-promoting activity of this analog was found to be identical to that of regular human insulin. In myoblasts, HMR 1964 produced a minor activation of insulin receptor substrate (IRS)-1 tyrosine phosphorylation, but a prominent activation of IRS-2, with a significantly stronger effect than insulin in human myoblasts. Predominant activation of IRS-2 was also observed in adult cardiomyocytes where HMR 1964 increased 3-O-methylglucose transport and the activation of Akt and glycogen synthase kinase-3 to the same extent as human insulin. We concluded that 1) the mitogenic properties of insulin analogs may result from a series of initial receptor interactions, including internalization and phosphorylation; 2) the mitogenic and metabolic potential of HMR 1964 is identical to that of insulin; and 3) predominant activation of IRS-2 may open new avenues for optimized insulin therapies.
胰岛素类似物潜在增强的促有丝分裂活性代表一种安全风险,这需要对考虑用于治疗应用的新类似物进行详细分析。我们使用成肌细胞和心肌细胞评估了两种新型速效胰岛素类似物,即赖氨酸(B3)、谷氨酸(B29)胰岛素(HMR 1964)和赖氨酸(B3)、异亮氨酸(B28)胰岛素(HMR 1153)的信号传导特性和促有丝分裂效力。在成肌细胞中,与HMR 1964和常规胰岛素相比,天冬氨酸(B10)胰岛素和HMR 1153的结合和内化均高出两到三倍。这一发现与显著的Shc/胰岛素样生长因子-I受体相互作用、Shc的酪氨酸磷酸化、细胞外信号调节蛋白激酶(ERK)-1和-2的激活以及HMR 1153和天冬氨酸(B10)胰岛素对DNA合成的刺激相关。相比之下,HMR 1964对Shc/ERK激酶级联产生微弱激活,并且在刺激成肌细胞中的DNA合成方面与胰岛素等效。此外,发现该类似物的体内促生长活性与常规人胰岛素相同。在成肌细胞中,HMR 1964对胰岛素受体底物(IRS)-1酪氨酸磷酸化产生轻微激活,但对IRS-2产生显著激活,在人成肌细胞中的作用明显强于胰岛素。在成年心肌细胞中也观察到IRS-2的主要激活,其中HMR 1964增加3-O-甲基葡萄糖转运以及Akt和糖原合酶激酶-3的激活程度与人类胰岛素相同。我们得出结论:1)胰岛素类似物的促有丝分裂特性可能源于一系列初始受体相互作用,包括内化和磷酸化;2)HMR 1964的促有丝分裂和代谢潜力与胰岛素相同;3)IRS-2的主要激活可能为优化胰岛素治疗开辟新途径。