Periplasmic expression of 4/7 α-conotoxin TXIA analogs in E. Coli Favors Ribbon Isomer Formation – Suggestion of a Binding Mode at the α7 nAChR

Y E Hamdaoui; X Wu; R J Clark; J Giribaldi; R Anangi; D J Craik; G F King; S Dutertre; Q Kaas; Volker Herzig; A Nicke

doi:10.3389/fphar.2019.00577

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Periplasmic expression of 4/7 α-conotoxin TXIA analogs in E. Coli Favors Ribbon Isomer Formation – Suggestion of a Binding Mode at the α7 nAChR

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Periplasmic expression of 4/7 α-conotoxin TXIA analogs in E. Coli Favors Ribbon Isomer Formation – Suggestion of a Binding Mode at the α7 nAChR

Y E Hamdaoui, X Wu, R J Clark, J Giribaldi, R Anangi, D J Craik, G F King, S Dutertre, Q Kaas, Volker Herzig, …

Frontiers in Pharmacology, Vol.10, 577

2019

DOI: https://doi.org/10.3389/fphar.2019.00577

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Abstract

Peptides derived from animal venoms provide important research tools for biochemical and pharmacological characterization of receptors, ion channels, and transporters. Some venom peptides have been developed into drugs (such as the synthetic ω-conotoxin MVIIA, ziconotide) and several are currently undergoing clinical trials for various clinical indications. Challenges in the development of peptides include their usually limited supply from natural sources, cost-intensive chemical synthesis, and potentially complicated stereoselective disulfide-bond formation in the case of disulfide-rich peptides. In particular, if extended structure-function analysis is performed or incorporation of stable isotopes for NMR studies is required, the comparatively low yields and high costs of synthesized peptides might constitute a limiting factor. Here we investigated the expression of the 4/7 α-conotoxin TxIA, a potent blocker at α3β2 and α7 nicotinic acetylcholine receptors (nAChRs), and three analogs in the form of maltose binding protein fusion proteins in Escherichia coli. Upon purification via nickel affinity chromatography and release of the toxins by protease cleavage, HPLC analysis revealed one major peak with the correct mass for all peptides. The final yield was 1-2 mg of recombinant peptide per liter of bacterial culture. Two-electrode voltage clamp analysis on oocyte-expressed nAChR subtypes demonstrated the functionality of these peptides but also revealed a 30 to 100-fold potency decrease of expressed TxIA compared to chemically synthesized TxIA. NMR spectroscopy analysis of TxIA and two of its analogs confirmed that the decreased activity was due to an alternative disulfide linkage rather than the missing C-terminal amidation, a post-translational modification that is common in α-conotoxins. All peptides preferentially formed in the ribbon conformation rather than the native globular conformation. Interestingly, in the case of the α7 nAChR, but not the α3β2 subtype, the loss of potency could be rescued by an R5D substitution. In conclusion, we demonstrate efficient expression of functional but alternatively folded ribbon TxIA variants in E. coli and provide the first structure-function analysis for a ribbon 4/7-α-conotoxin at α7 and α3β2 nAChRs. Computational analysis based on these data provide evidence for a ribbon α-conotoxin binding mode that might be exploited to design ligands with optimized selectivity.

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Title: Periplasmic expression of 4/7 α-conotoxin TXIA analogs in E. Coli Favors Ribbon Isomer Formation – Suggestion of a Binding Mode at the α7 nAChR
Authors: Y E Hamdaoui (Author)
X Wu (Author) - University of Queensland
R J Clark (Author) - University of Queensland
J Giribaldi (Author)
R Anangi (Author) - University of Queensland
D J Craik (Author) - University of Queensland
G F King (Author) - University of Queensland
S Dutertre (Author)
Q Kaas (Author) - University of Queensland
Volker Herzig (Author) - University of Queensland
A Nicke (Author)
Publication details: Frontiers in Pharmacology, Vol.10, 577; 17
Publisher: Frontiers Research Foundation
Date published: 2019
DOI: 10.3389/fphar.2019.00577
ISSN: 1663-9812
Copyright note: Copyright © 2019 El Hamdaoui, Wu, Clark, Giribaldi, Anangi, Craik, King, Dutertre, Kaas, Herzig and Nicke. This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) and the copyright owner(s) are credited and that the original publication in this journal is cited, in accordance with accepted academic practice. No use, distribution or reproduction is permitted which does not comply with these terms.
Organisation Unit: School of Science and Engineering - Legacy; University of the Sunshine Coast, Queensland; School of Science, Technology and Engineering; Centre for Bioinnovation
Language: English
Record Identifier: 99450974302621
Output Type: Journal article

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