Lentivirus-mediated transduction of connexin cDNAs shows level- and isoform-specific alterations in insulin secretion of primary pancreaticβ-cells

Author:

Caton David1,Calabrese Alessandra1,Mas Christophe1,Serre-Beinier Véronique1,Charollais Anne1,Caille Dorothée1,Zufferey Romain2,Trono Didier2,Meda Paolo1

Affiliation:

1. Department of Morphology, University of Geneva Medical School, 1211 Geneva 4,Switzerland

2. Department of Genetics and Microbiology, University of Geneva Medical School,1211 Geneva 4, Switzerland

Abstract

We have generated novel lentiviral vectors to integrate various connexin cDNAs into primary, non-dividing cells. We have used these vectors to test whether proper control of insulin secretion depends on a specific connexin isoform and/or on its level of expression. We have observed that transduced connexin32, connexin36 and connexin43 were expressed by primary adultβ-cells at membrane interfaces, were packed into typical gap junction plaques and formed functional channels that allowed a variable coupling,depending on the type and level of connexin expressed. The infected cells spontaneously reaggregated into three-dimensional pseudo-islet organs that could be maintained in culture. We have found that pseudo-islets made by cells transduced with either GFP- or connexin43-expressing lentivirus released insulin in response to various secretagogues similarly to controls. By contrast, pseudo-islets made by cells expressing connexin32, a connexin exogenous to pancreatic islets, or over-expressing connexin36, the endogenous islet connexin, featured a marked decrease in the secretory response to glucose. The data show: (1) that lentiviral vectors allow stable modulation of various connexin in primary, non-proliferating cells; (2) that specific connexin isoforms affect insulin secretion differently; and (3) that adequate levels of coupling via connexin36 channels are required for proper β-cell function.

Publisher

The Company of Biologists

Subject

Cell Biology

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