Nanopore analysis of the interaction of metal ions with prion proteins and peptidesThis paper is one of a selection of papers published in this special issue entitled “Canadian Society of Biochemistry, Molecular & Cellular Biology 52nd Annual Meeting — Protein Folding: Principles and Diseases” and has undergone the Journal's usual peer review process.

Abstract: Nanopore analysis can be used to study conformational changes in individual peptide or protein molecules. Under an applied voltage there is a change in the event parameters of blockade current or time when a molecule bumps into or translocates through the pore. If a molecule undergoes a conformational change upon binding a ligand or metal ion the event parameters will be altered. The objective of this research was to demonstrate that the conformation of the prion protein (PrP) and prion peptides can be modulat… Show more

“…For example, in the absence of metal ions Zn-finger peptides, prion peptides from the octarepeat region and myelin basic protein will readily translocate; but in the presence of Zn(II) or Cu(II) the peptides fold into a compact structure and only bumping events are observed. [38][39][40] These results highlight the capacity of the pore to interrogate the conformation of the peptide at the instant at which it interacts with the pore.…”

Nanopore analysis

“…For example, in the absence of metal ions Zn-finger peptides, prion peptides from the octarepeat region and myelin basic protein will readily translocate; but in the presence of Zn(II) or Cu(II) the peptides fold into a compact structure and only bumping events are observed. [38][39][40] These results highlight the capacity of the pore to interrogate the conformation of the peptide at the instant at which it interacts with the pore.…”

Nanopore analysis

“…As shown previously, the proportion of Type-I events are about 60%. 37 Upon addition of antibody SN6b there was no significant change in the percentage of type-I events as would be expected if the antibody did not bind to the native protein (Fig. 1B).…”

“…35 At present these possibilities cannot be distinguished. Previously, our group has used nanopore analysis to probe various aspects of PrP C behavior, including metal binding 37 and the interaction with PrP C specific-antibodies. 35 As well, it was demonstrated that the event profiles after pre-incubation in 1.5 M guanidinium hydrochloride (Gdn-HCl) of wild-type bPrP and mutant bPrP(T194A) were different as were those of full length human PrP(23-231) and truncated PrP(90-231).…”

“…19,20,45 Previously it was shown that wild-type bPrP generated about 35%−40% of type-II events. 35,37 This decrease in the number of type-II events in PrP C as compared with T194A may be due to the orientation of the molecule that may only thread into the pore through the three negatively charged amino acids (DYEDRYYR) located on the helix α1. 37 The interaction of the T194A mutant of PrP C with SN6b by nanopore analysis was validated through ELISAs and immunopreciptation of the mutant but not the wild-type proteins expressed in bacteria or mammalian cells.…”

Binding of bovine T194A PrP^Cby PrP^Sc-specific antibodies

“…38,39 Previously nanopore analysis has allowed detailed investigation of various aspects of the PrP C structure-activity relationship including the interaction of PrP C with metal ions and characterization of the consequences of disease-associated single amino acid mutations on interaction with a therapeutic PrP Sc -antibody. [42][43][44] Accordingly nanopore analysis was a logical approach to investigate genetic polymorphisms of ovine PrP C that are associated with differential susceptibilities to scrapie infection.…”

Nanopore analysis reveals differences in structural stability of ovine PrP^Cproteins corresponding to scrapie susceptible (VRQ) and resistance (ARR) genotypes