Gherzi R, Sesti G, Andraghetti G, De Pirro R, Lauro R, Adezati L, Cordera R
Department of Internal Medicine, University of Genova, Italy.
J Biol Chem. 1989 May 25;264(15):8627-35.
Anti-insulin receptor monoclonal antibody MA-10 inhibits insulin receptor autophosphorylation of purified rat liver insulin receptors without affecting insulin binding (Cordera, R., Andraghetti, G., Gherzi, R., Adezati, L., Montemurro, A., Lauro, R., Goldfine, I. D., and De Pirro, R. (1987) Endocrinology 121, 2007-2010). The effect of MA-10 on insulin receptor autophosphorylation and on two insulin actions (thymidine incorporation into DNA and receptor down-regulation) was investigated in rat hepatoma Fao cells. MA-10 inhibits insulin-stimulated receptor autophosphorylation, thymidine incorporation into DNA, and insulin-induced receptor down-regulation without affecting insulin receptor binding. We show that MA-10 binds to a site of rat insulin receptors different from the insulin binding site in intact Fao cells. Insulin does not inhibit MA-10 binding, and MA-10 does not inhibit insulin binding to rat Fao cells. Moreover, MA-10 binding to down-regulated cells is reduced to the same extent as insulin binding. In rat insulin receptors the MA-10 binding site has been tentatively localized in the extracellular part of the insulin receptor beta-subunit based on the following evidence: (i) MA-10 binds to insulin receptor in intact rat cells; (ii) MA-10 immunoprecipitates isolated insulin receptor beta-subunits labeled with both [35S]methionine and 32P; (iii) MA-10 reacts with rat insulin receptor beta-subunits by the method of immunoblotting, similar to an antipeptide antibody directed against the carboxyl terminus of the insulin receptor beta-subunit. Moreover, MA-10 inhibits autophosphorylation and protein-tyrosine kinase activity of reduced and purified insulin receptor beta-subunits. The finding that MA-10 inhibits insulin-stimulated receptor autophosphorylation and reduces insulin-stimulated thymidine incorporation into DNA and receptor down-regulation suggests that the extracellular part of the insulin receptor beta-subunit plays a role in the regulation of insulin receptor protein-tyrosine kinase activity.
抗胰岛素受体单克隆抗体MA-10可抑制纯化的大鼠肝脏胰岛素受体的胰岛素受体自身磷酸化,而不影响胰岛素结合(科尔德拉,R.,安德拉格蒂,G.,盖尔齐,R.,阿德扎蒂,L.,蒙特穆罗,A.,劳罗,R.,戈德芬,I.D.,和德皮罗,R.(1987年)《内分泌学》121,2007 - 2010)。在大鼠肝癌Fao细胞中研究了MA-10对胰岛素受体自身磷酸化以及两种胰岛素作用(胸苷掺入DNA和受体下调)的影响。MA-10可抑制胰岛素刺激的受体自身磷酸化、胸苷掺入DNA以及胰岛素诱导的受体下调,而不影响胰岛素受体结合。我们发现,在完整的Fao细胞中,MA-10与大鼠胰岛素受体的结合位点不同于胰岛素结合位点。胰岛素不抑制MA-10结合,MA-10也不抑制胰岛素与大鼠Fao细胞的结合。此外,MA-10与下调细胞的结合减少程度与胰岛素结合相同。基于以下证据,在大鼠胰岛素受体中,MA-10结合位点已初步定位在胰岛素受体β亚基的细胞外部分:(i)MA-10在完整的大鼠细胞中与胰岛素受体结合;(ii)MA-10免疫沉淀分离出用[35S]甲硫氨酸和32P标记的胰岛素受体β亚基;(iii)MA-10通过免疫印迹法与大鼠胰岛素受体β亚基反应,类似于针对胰岛素受体β亚基羧基末端的抗肽抗体。此外,MA-10抑制还原和纯化的胰岛素受体β亚基的自身磷酸化和蛋白酪氨酸激酶活性。MA-10抑制胰岛素刺激的受体自身磷酸化并减少胰岛素刺激的胸苷掺入DNA和受体下调这一发现表明,胰岛素受体β亚基的细胞外部分在胰岛素受体蛋白酪氨酸激酶活性的调节中起作用。
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