Biomedicines (Feb 2020)

Addition of K22 Converts Spider Venom Peptide Pme2a from an Activator to an Inhibitor of Na<sub>V</sub>1.7

  • Kathleen Yin,
  • Jennifer R. Deuis,
  • Zoltan Dekan,
  • Ai-Hua Jin,
  • Paul F. Alewood,
  • Glenn F. King,
  • Volker Herzig,
  • Irina Vetter

DOI
https://doi.org/10.3390/biomedicines8020037
Journal volume & issue
Vol. 8, no. 2
p. 37

Abstract

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Spider venom is a novel source of disulfide-rich peptides with potent and selective activity at voltage-gated sodium channels (NaV). Here, we describe the discovery of μ-theraphotoxin-Pme1a and μ/δ-theraphotoxin-Pme2a, two novel peptides from the venom of the Gooty Ornamental tarantula Poecilotheria metallica that modulate NaV channels. Pme1a is a 35 residue peptide that inhibits NaV1.7 peak current (IC50 334 ± 114 nM) and shifts the voltage dependence of activation to more depolarised membrane potentials (V1/2 activation: Δ = +11.6 mV). Pme2a is a 33 residue peptide that delays fast inactivation and inhibits NaV1.7 peak current (EC50 > 10 μM). Synthesis of a [+22K]Pme2a analogue increased potency at NaV1.7 (IC50 5.6 ± 1.1 μM) and removed the effect of the native peptide on fast inactivation, indicating that a lysine at position 22 (Pme2a numbering) is important for inhibitory activity. Results from this study may be used to guide the rational design of spider venom-derived peptides with improved potency and selectivity at NaV channels in the future.

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