A reassessment of copper(II) binding in the full-length prion protein

Abstract

It has been shown previously that the unfolded N-terminal domain of the prion protein can bind up to six Cu²⁺ ions in vitro. This domain contains four tandem repeats of the octapeptide sequence PHGGGWGQ, which, alongside the two histidine residues at positions 96 and 111, contribute to its Cu²⁺ binding properties. At the maximum metal-ion occupancy each Cu²⁺ is co-ordinated by a single imidazole and deprotonated backbone amide groups. However two recent studies of peptides representing the octapeptide repeat region of the protein have shown, that at low Cu²⁺ availability, an alternative mode of co-ordination occurs where the metal ion is bound by multiple histidine imidazole groups. Both modes of binding are readily populated at pH 7.4, while mild acidification to pH 5.5 selects in favour of the low occupancy, multiple imidazole binding mode. We have used NMR to resolve how Cu²⁺ binds to the full-length prion protein under mildly acidic conditions where multiple histidine co-ordination is dominant. We show that at pH 5.5 the protein binds two Cu²⁺ ions, and that all six histidine residues of the unfolded N-terminal domain and the N-terminal amine act as ligands. These two sites are of sufficient affinity to be maintained in the presence of millimolar concentrations of competing exogenous histidine. A previously unknown interaction between the N-terminal domain and a site on the C-terminal domain becomes apparent when the protein is loaded with Cu²⁺. Furthermore, the data reveal that sub-stoichiometric quantities of Cu²⁺ will cause self-association of the prion protein in vitro, suggesting that Cu²⁺ may play a role in controlling oligomerization in vivo.