CryoEM structures of the human CLC-2 voltage gated chloride channel reveal a ball and chain gating mechanism

CLC-2 is a voltage-gated chloride channel that contributes to electrical excitability and ion homeostasis in many different mammalian tissues and cell types. Among the nine mammalian CLC homologs, CLC-2 is uniquely activated by hyperpolarization, rather than depolarization, of the plasma membrane. T...

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Autores principales: Xu, Mengyuan, Neelands, Torben, Powers, Alexander S., Liu, Yan, Miller, Steven D., Pintilie, Grigore, Du Bois, J., Dror, Ron O., Chiu, Wah, Maduke, Merritt
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Cold Spring Harbor Laboratory 2023
Materias:
Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10462068/
https://www.ncbi.nlm.nih.gov/pubmed/37645939
http://dx.doi.org/10.1101/2023.08.13.553136
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author Xu, Mengyuan
Neelands, Torben
Powers, Alexander S.
Liu, Yan
Miller, Steven D.
Pintilie, Grigore
Du Bois, J.
Dror, Ron O.
Chiu, Wah
Maduke, Merritt
author_facet Xu, Mengyuan
Neelands, Torben
Powers, Alexander S.
Liu, Yan
Miller, Steven D.
Pintilie, Grigore
Du Bois, J.
Dror, Ron O.
Chiu, Wah
Maduke, Merritt
author_sort Xu, Mengyuan
collection PubMed
description CLC-2 is a voltage-gated chloride channel that contributes to electrical excitability and ion homeostasis in many different mammalian tissues and cell types. Among the nine mammalian CLC homologs, CLC-2 is uniquely activated by hyperpolarization, rather than depolarization, of the plasma membrane. The molecular basis for the divergence in polarity of voltage gating mechanisms among closely related CLC homologs has been a long-standing mystery, in part because few CLC channel structures are available, and those that exist exhibit high conformational similarity. Here, we report cryoEM structures of human CLC-2 at 2.46 – 2.76 Å, in the presence and absence of the potent and selective inhibitor AK-42. AK-42 binds within the extracellular entryway of the Cl(−) -permeation pathway, occupying a pocket previously proposed through computational docking studies. In the apo structure, we observed two distinct apo conformations of CLC-2 involving rotation of one of the cytoplasmic C-terminal domains (CTDs). In the absence of CTD rotation, an intracellular N-terminal 15-residue hairpin peptide nestles against the TM domain to physically occlude the Cl(−)-permeation pathway from the intracellular side. This peptide is highly conserved among species variants of CLC-2 but is not present in any other CLC homologs. Previous studies suggested that the N-terminal domain of CLC-2 influences channel properties via a “ball-and-chain” gating mechanism, but conflicting data cast doubt on such a mechanism, and thus the structure of the N-terminal domain and its interaction with the channel has been uncertain. Through electrophysiological studies of an N-terminal deletion mutant lacking the 15-residue hairpin peptide, we show that loss of this short sequence increases the magnitude and decreases the rectification of CLC-2 currents expressed in mammalian cells. Furthermore, we show that with repetitive hyperpolarization WT CLC-2 currents increase in resemblance to the hairpin-deleted CLC-2 currents. These functional results combined with our structural data support a model in which the N-terminal hairpin of CLC-2 stabilizes a closed state of the channel by blocking the cytoplasmic Cl(−)-permeation pathway.
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spelling pubmed-104620682023-08-29 CryoEM structures of the human CLC-2 voltage gated chloride channel reveal a ball and chain gating mechanism Xu, Mengyuan Neelands, Torben Powers, Alexander S. Liu, Yan Miller, Steven D. Pintilie, Grigore Du Bois, J. Dror, Ron O. Chiu, Wah Maduke, Merritt bioRxiv Article CLC-2 is a voltage-gated chloride channel that contributes to electrical excitability and ion homeostasis in many different mammalian tissues and cell types. Among the nine mammalian CLC homologs, CLC-2 is uniquely activated by hyperpolarization, rather than depolarization, of the plasma membrane. The molecular basis for the divergence in polarity of voltage gating mechanisms among closely related CLC homologs has been a long-standing mystery, in part because few CLC channel structures are available, and those that exist exhibit high conformational similarity. Here, we report cryoEM structures of human CLC-2 at 2.46 – 2.76 Å, in the presence and absence of the potent and selective inhibitor AK-42. AK-42 binds within the extracellular entryway of the Cl(−) -permeation pathway, occupying a pocket previously proposed through computational docking studies. In the apo structure, we observed two distinct apo conformations of CLC-2 involving rotation of one of the cytoplasmic C-terminal domains (CTDs). In the absence of CTD rotation, an intracellular N-terminal 15-residue hairpin peptide nestles against the TM domain to physically occlude the Cl(−)-permeation pathway from the intracellular side. This peptide is highly conserved among species variants of CLC-2 but is not present in any other CLC homologs. Previous studies suggested that the N-terminal domain of CLC-2 influences channel properties via a “ball-and-chain” gating mechanism, but conflicting data cast doubt on such a mechanism, and thus the structure of the N-terminal domain and its interaction with the channel has been uncertain. Through electrophysiological studies of an N-terminal deletion mutant lacking the 15-residue hairpin peptide, we show that loss of this short sequence increases the magnitude and decreases the rectification of CLC-2 currents expressed in mammalian cells. Furthermore, we show that with repetitive hyperpolarization WT CLC-2 currents increase in resemblance to the hairpin-deleted CLC-2 currents. These functional results combined with our structural data support a model in which the N-terminal hairpin of CLC-2 stabilizes a closed state of the channel by blocking the cytoplasmic Cl(−)-permeation pathway. Cold Spring Harbor Laboratory 2023-08-15 /pmc/articles/PMC10462068/ /pubmed/37645939 http://dx.doi.org/10.1101/2023.08.13.553136 Text en https://creativecommons.org/licenses/by/4.0/This work is licensed under a Creative Commons Attribution 4.0 International License (https://creativecommons.org/licenses/by/4.0/) , which allows reusers to distribute, remix, adapt, and build upon the material in any medium or format, so long as attribution is given to the creator. The license allows for commercial use.
spellingShingle Article
Xu, Mengyuan
Neelands, Torben
Powers, Alexander S.
Liu, Yan
Miller, Steven D.
Pintilie, Grigore
Du Bois, J.
Dror, Ron O.
Chiu, Wah
Maduke, Merritt
CryoEM structures of the human CLC-2 voltage gated chloride channel reveal a ball and chain gating mechanism
title CryoEM structures of the human CLC-2 voltage gated chloride channel reveal a ball and chain gating mechanism
title_full CryoEM structures of the human CLC-2 voltage gated chloride channel reveal a ball and chain gating mechanism
title_fullStr CryoEM structures of the human CLC-2 voltage gated chloride channel reveal a ball and chain gating mechanism
title_full_unstemmed CryoEM structures of the human CLC-2 voltage gated chloride channel reveal a ball and chain gating mechanism
title_short CryoEM structures of the human CLC-2 voltage gated chloride channel reveal a ball and chain gating mechanism
title_sort cryoem structures of the human clc-2 voltage gated chloride channel reveal a ball and chain gating mechanism
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10462068/
https://www.ncbi.nlm.nih.gov/pubmed/37645939
http://dx.doi.org/10.1101/2023.08.13.553136
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