
Gap junctions establish direct pathways for cell-to-cell communication through the assembly of twelve connexin subunits that form intercellular channels connecting neighbouring cells. Co-assembly of different connexin isoforms produces channels with unique properties and enables communication across cell types. Here we used single-particle cryo-electron microscopy to investigate the structural basis of connexin co-assembly in native lens gap junction channels composed of connexin 46 and connexin 50 (Cx46/50). We provide the first comparative analysis to connexin 26 (Cx26), which-together with computational studies-elucidates key energetic features governing gap junction permselectivity. Cx46/50 adopts an open-state conformation that is distinct from the Cx26 crystal structure, yet it appears to be stabilized by a conserved set of hydrophobic anchoring residues. 'Hot spots' of genetic mutations linked to hereditary cataract formation map to the core structural-functional elements identified in Cx46/50, suggesting explanations for many of the disease-causing effects.
Connexin 26, Models, Molecular, Cryoelectron Microscopy, Lens, Crystalline, Mutation, Gap Junctions, Humans, Amino Acid Sequence, Article, Cataract, Connexins
Connexin 26, Models, Molecular, Cryoelectron Microscopy, Lens, Crystalline, Mutation, Gap Junctions, Humans, Amino Acid Sequence, Article, Cataract, Connexins
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