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The ß3-subunit modulates the effect of venom peptides ProTx-II and OD1 on NaV 1.7 gating.
Salvage, Samantha C; Rahman, Taufiq; Eagles, David A; Rees, Johanna S; King, Glenn F; Huang, Christopher L-H; Jackson, Antony P.
Affiliation
  • Salvage SC; Department of Biochemistry, University of Cambridge, Cambridge, UK.
  • Rahman T; Department of Pharmacology, University of Cambridge, Cambridge, UK.
  • Eagles DA; Institute of Molecular Bioscience, University of Queensland, Brisbane, QLD, Australia.
  • Rees JS; Australian Research Council Centre of Excellence for Innovations in Peptide and Protein Science, The University of Queensland, Brisbane, QLD, Australia.
  • King GF; Department of Biochemistry, University of Cambridge, Cambridge, UK.
  • Huang CL; Institute of Molecular Bioscience, University of Queensland, Brisbane, QLD, Australia.
  • Jackson AP; Australian Research Council Centre of Excellence for Innovations in Peptide and Protein Science, The University of Queensland, Brisbane, QLD, Australia.
J Cell Physiol ; 238(6): 1354-1367, 2023 06.
Article in En | MEDLINE | ID: mdl-37042220
The voltage-gated sodium channel NaV 1.7 is involved in various pain phenotypes and is physiologically regulated by the NaV -ß3-subunit. Venom toxins ProTx-II and OD1 modulate NaV 1.7 channel function and may be useful as therapeutic agents and/or research tools. Here, we use patch-clamp recordings to investigate how the ß3-subunit can influence and modulate the toxin-mediated effects on NaV 1.7 function, and we propose a putative binding mode of OD1 on NaV 1.7 to rationalise its activating effects. The inhibitor ProTx-II slowed the rate of NaV 1.7 activation, whilst the activator OD1 reduced the rate of fast inactivation and accelerated recovery from inactivation. The ß3-subunit partially abrogated these effects. OD1 induced a hyperpolarising shift in the V1/2 of steady-state activation, which was not observed in the presence of ß3. Consequently, OD1-treated NaV 1.7 exhibited an enhanced window current compared with OD1-treated NaV 1.7-ß3 complex. We identify candidate OD1 residues that are likely to prevent the upward movement of the DIV S4 helix and thus impede fast inactivation. The binding sites for each of the toxins and the predicted location of the ß3-subunit on the NaV 1.7 channel are distinct. Therefore, we infer that the ß3-subunit influences the interaction of toxins with NaV 1.7 via indirect allosteric mechanisms. The enhanced window current shown by OD1-treated NaV 1.7 compared with OD1-treated NaV 1.7-ß3 is discussed in the context of differing cellular expressions of NaV 1.7 and the ß3-subunit in dorsal root ganglion (DRG) neurons. We propose that ß3, as the native binding partner for NaV 1.7 in DRG neurons, should be included during screening of molecules against NaV 1.7 in relevant analgesic discovery campaigns.
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Full text: 1 Collection: 01-internacional Database: MEDLINE Main subject: Venoms / Voltage-Gated Sodium Channels Limits: Humans Language: En Journal: J Cell Physiol Year: 2023 Document type: Article Country of publication: Estados Unidos

Full text: 1 Collection: 01-internacional Database: MEDLINE Main subject: Venoms / Voltage-Gated Sodium Channels Limits: Humans Language: En Journal: J Cell Physiol Year: 2023 Document type: Article Country of publication: Estados Unidos