Cell-free synthesis and assembly of connexins into functional gap junction membrane channels
Open Access
- 15 May 1997
- journal article
- research article
- Published by Springer Nature in The EMBO Journal
- Vol. 16 (10) , 2703-2716
- https://doi.org/10.1093/emboj/16.10.2703
Abstract
Several different gap junction channel subunit isotypes, known as connexins, were synthesized in a cell‐free translation system supplemented with microsomal membranes to study the mechanisms involved in gap junction channel assembly. Previous results indicated that the connexins were synthesized as membrane proteins with their relevant transmembrane topology. An integrated biochemical and biophysical analysis indicated that the connexins assembled specifically with other connexin subunits. No interactions were detected between connexin subunits and other co‐translated transmembrane proteins. The connexins that were integrated into microsomal vesicles assembled into homo‐ and hetero‐oligomeric structures with hydrodynamic properties of a 9S particle, consistent with the properties reported for hexameric gap junction connexons derived from gap junctions in vivo . Further, cell‐free assembled homo‐oligomeric connexons composed of β1 or β2 connexin were reconstituted into synthetic lipid bilayers. Single channel conductances were recorded from these bilayers that were similar to those measured for these connexons produced in vivo . Thus, this is the first direct evidence that the synthesis and assembly of a gap junction connexon can take place in microsomal membranes. Finally, the cell‐free system has been used to investigate the properties of α1, β1 and β2 connexin to assemble into hetero‐oligomers. Evidence has been obtained for a selective interaction between individual connexin isotypes and that a signal determining the potential hetero‐oligomeric combinations of connexin isotypes may be located in the N–terminal sequence of the connexins.Keywords
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