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A Chimeric NaV1.8 Channel Expression System Based on HEK293T Cell Line

Among the nine voltage-gated sodium channel (NaV) subtypes, NaV1.8 is an attractive therapeutic target for pain. The heterologous expression of recombinant NaV1.8 currents is of particular importance for its electrophysiological and pharmacological studies. However, NaV1.8 expresses no or low-level...

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Autores principales: Zhou, Xi, Zhang, Yunxiao, Tang, Dongfang, Liang, Songping, Chen, Ping, Tang, Cheng, Liu, Zhonghua
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Frontiers Media S.A. 2018
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5900924/
https://www.ncbi.nlm.nih.gov/pubmed/29686617
http://dx.doi.org/10.3389/fphar.2018.00337
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author Zhou, Xi
Zhang, Yunxiao
Tang, Dongfang
Liang, Songping
Chen, Ping
Tang, Cheng
Liu, Zhonghua
author_facet Zhou, Xi
Zhang, Yunxiao
Tang, Dongfang
Liang, Songping
Chen, Ping
Tang, Cheng
Liu, Zhonghua
author_sort Zhou, Xi
collection PubMed
description Among the nine voltage-gated sodium channel (NaV) subtypes, NaV1.8 is an attractive therapeutic target for pain. The heterologous expression of recombinant NaV1.8 currents is of particular importance for its electrophysiological and pharmacological studies. However, NaV1.8 expresses no or low-level functional currents when transiently transfected into non-neuronal cell lines. The present study aims to explore the molecular determinants limiting its functional expression and accordingly establish a functional NaV1.8 expression system. We conducted screening analysis of the NaV1.8 intracellular loops by constructing NaV chimeric channels and confirmed that the NaV1.8 C-terminus was the only limiting factor. Replacing this sequence with that of NaV1.4, NaV1.5, or NaV1.7 constructed functional channels (NaV1.8/1.4L5, NaV1.8/1.5L5, and NaV1.8/1.7L5, respectively), which expressed high-level NaV1.8-like currents in HEK293T cells. The chimeric channel NaV1.8/1.7L5 displayed much faster inactivation of its macroscopic currents than NaV1.8/1.4L5 and NaV1.8/1.5L5, and it was the most similar to wild-type NaV1.8 expressed in ND7/23 cells. Its currents were very stable during repetitive depolarizations, while its repriming kinetic was different from wild-type NaV1.8. Most importantly, NaV1.8/1.7L5 pharmacologically resembled wild-type NaV1.8 as revealed by testing their susceptibility to two NaV1.8 selective antagonists, APETx-2 and MrVIB. NaV chimeras study showed that at least the domain 2 and domain 4 of NaV1.8 were involved in binding with APETx-2. Our study provided new insights into the function of NaV1.8 intracellular loops, as well as a reliable and convenient expression system which could be useful in NaV1.8 studies.
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spelling pubmed-59009242018-04-23 A Chimeric NaV1.8 Channel Expression System Based on HEK293T Cell Line Zhou, Xi Zhang, Yunxiao Tang, Dongfang Liang, Songping Chen, Ping Tang, Cheng Liu, Zhonghua Front Pharmacol Pharmacology Among the nine voltage-gated sodium channel (NaV) subtypes, NaV1.8 is an attractive therapeutic target for pain. The heterologous expression of recombinant NaV1.8 currents is of particular importance for its electrophysiological and pharmacological studies. However, NaV1.8 expresses no or low-level functional currents when transiently transfected into non-neuronal cell lines. The present study aims to explore the molecular determinants limiting its functional expression and accordingly establish a functional NaV1.8 expression system. We conducted screening analysis of the NaV1.8 intracellular loops by constructing NaV chimeric channels and confirmed that the NaV1.8 C-terminus was the only limiting factor. Replacing this sequence with that of NaV1.4, NaV1.5, or NaV1.7 constructed functional channels (NaV1.8/1.4L5, NaV1.8/1.5L5, and NaV1.8/1.7L5, respectively), which expressed high-level NaV1.8-like currents in HEK293T cells. The chimeric channel NaV1.8/1.7L5 displayed much faster inactivation of its macroscopic currents than NaV1.8/1.4L5 and NaV1.8/1.5L5, and it was the most similar to wild-type NaV1.8 expressed in ND7/23 cells. Its currents were very stable during repetitive depolarizations, while its repriming kinetic was different from wild-type NaV1.8. Most importantly, NaV1.8/1.7L5 pharmacologically resembled wild-type NaV1.8 as revealed by testing their susceptibility to two NaV1.8 selective antagonists, APETx-2 and MrVIB. NaV chimeras study showed that at least the domain 2 and domain 4 of NaV1.8 were involved in binding with APETx-2. Our study provided new insights into the function of NaV1.8 intracellular loops, as well as a reliable and convenient expression system which could be useful in NaV1.8 studies. Frontiers Media S.A. 2018-04-06 /pmc/articles/PMC5900924/ /pubmed/29686617 http://dx.doi.org/10.3389/fphar.2018.00337 Text en Copyright © 2018 Zhou, Zhang, Tang, Liang, Chen, Tang and Liu. http://creativecommons.org/licenses/by/4.0/ 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 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.
spellingShingle Pharmacology
Zhou, Xi
Zhang, Yunxiao
Tang, Dongfang
Liang, Songping
Chen, Ping
Tang, Cheng
Liu, Zhonghua
A Chimeric NaV1.8 Channel Expression System Based on HEK293T Cell Line
title A Chimeric NaV1.8 Channel Expression System Based on HEK293T Cell Line
title_full A Chimeric NaV1.8 Channel Expression System Based on HEK293T Cell Line
title_fullStr A Chimeric NaV1.8 Channel Expression System Based on HEK293T Cell Line
title_full_unstemmed A Chimeric NaV1.8 Channel Expression System Based on HEK293T Cell Line
title_short A Chimeric NaV1.8 Channel Expression System Based on HEK293T Cell Line
title_sort chimeric nav1.8 channel expression system based on hek293t cell line
topic Pharmacology
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5900924/
https://www.ncbi.nlm.nih.gov/pubmed/29686617
http://dx.doi.org/10.3389/fphar.2018.00337
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