Autoimmune destruction of pancreatic B cells in type I, insulin-dependent diabetes mellitus (IDDM) results in the loss of endogenous insulin secretion, which is incompletely replaced by exogenous insulin administration. The functional restoration provided by allogeneic B-cell transplantation is limited by adverse effects of immunosuppression. To pursue an insulin replacement therapy based on autologous, engineered human non- B cells, we generated a retroviral vector encoding a genetically modified human proinsulin, cleavable to insulin in non-B cells, and a human nonfunctional cell surface marker. Here we report that this vector efficiently transduced primary human cells, inducing the synthesis of a modified proinsulin that was processed and released as mature insulin. This retrovirally derived insulin displayed in vitro biological activity, specifically binding to and phosphorylation of the insulin receptor, comparable to human insulin. In vivo, the transplantation of insulin-producing fibroblasts reverted hyperglycemia in a murine model of diabetes, whereas proinsulin-producing cells were ineffective. These results support the possibility of developing insulin production machinery in human non-B cells for gene therapy of IDDNI.
Reversal of diabetes in mice by implantation of human fibroblasts genetically engineered to release mature human insulin / L. Falqui, S. Martinenghi, G.M. Severini, P. Corbella, M.V Taglietti, C. Arcelloni, E. Sarugeri, L.D Monti, R. Paroni, N. Dozio, G. Pozza, C. Bordignon. - In: HUMAN GENE THERAPY. - ISSN 1043-0342. - 10:11(1999 Jul 20), pp. 1753-1762.
Reversal of diabetes in mice by implantation of human fibroblasts genetically engineered to release mature human insulin
R. Paroni;
1999
Abstract
Autoimmune destruction of pancreatic B cells in type I, insulin-dependent diabetes mellitus (IDDM) results in the loss of endogenous insulin secretion, which is incompletely replaced by exogenous insulin administration. The functional restoration provided by allogeneic B-cell transplantation is limited by adverse effects of immunosuppression. To pursue an insulin replacement therapy based on autologous, engineered human non- B cells, we generated a retroviral vector encoding a genetically modified human proinsulin, cleavable to insulin in non-B cells, and a human nonfunctional cell surface marker. Here we report that this vector efficiently transduced primary human cells, inducing the synthesis of a modified proinsulin that was processed and released as mature insulin. This retrovirally derived insulin displayed in vitro biological activity, specifically binding to and phosphorylation of the insulin receptor, comparable to human insulin. In vivo, the transplantation of insulin-producing fibroblasts reverted hyperglycemia in a murine model of diabetes, whereas proinsulin-producing cells were ineffective. These results support the possibility of developing insulin production machinery in human non-B cells for gene therapy of IDDNI.
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