Your search keyword '"NaChBac"' showing total 32 results

1. Molecular mechanism of the spider toxin κ-LhTx-I acting on the bacterial voltage-gated sodium channel NaChBac.

Author

Zhen Xiao, Yaqi Li, Piao Zhao, Xiangyue Wu, Guoqing Luo, Shuijiao Peng, Hongrong Liu, Cheng Tang, and Zhonghua Liu

Subjects

SODIUM channels, TOXINS, POTASSIUM channels, BRUGADA syndrome, SITE-specific mutagenesis, SPIDERS, MOLECULAR docking

Abstract

The bacterial sodium channel NaChBac is the prokaryotic prototype for the eukaryotic NaV and CaV channels, which could be used as a relatively simple model to study their structure-function relationships. However, few modulators of NaChBac have been reported thus far, and the pharmacology of NaChBac remains to be investigated. In the present study, we show that the spider toxin κ-LhTx-1, an antagonist of the KV4 family potassium channels, potently inhibits NaChBac with an IC50 of 491.0 ± 61.7 nM. Kinetics analysis revealed that κ-LhTx-1 inhibits NaChBac by impeding the voltage-sensor activation. Site-directed mutagenesis confirmed that phenylalanine-103 (F103) in the S3-S4 extracellular loop of NaChBac was critical for interacting with κ-LhTx-1. Molecular docking predicts the binding interface between κ-LhTx-1 and NaChBac and highlights a dominant hydrophobic interaction between W27 in κ-LhTx-1 and F103 in NaChBac that stabilizes the interface. In contrast, κ-LhTx-1 showed weak activity on the mammalian NaV channels, with 10 μM toxin slightly inhibiting the peak currents of NaV1.2-1.9 subtypes. Taken together, our study shows that κ-LhTx-1 inhibits the bacterial sodium channel, NaChBac, using a voltage-sensor trapping mechanism similar to mammalian NaV site 4 toxins. κ-LhTx-1 could be used as a ligand to study the toxin-channel interactions in the native membrane environments, given that the NaChBac structure was successfully resolved in a nanodisc. [ABSTRACT FROM AUTHOR]

Published

2022

2. Regulation and drug modulation of a voltage-gated sodium channel: Pivotal role of the S4-S5 linker in activation and slow inactivation.

Author

Jinglei Xiao, Bondarenko, Vasyl, Yali Wang, Suma, Antonio, Wells, Marta, Qiang Chen, Tillman, Tommy, Yan Luo, Buwei Yu, Dailey, William P., Eckenhoff, Roderic, Pei Tang, Carnevale, Vincenzo, Klein, Michael L., and Yan Xu

Subjects

*SODIUM channels, *DRUG laws, *MAGNETIZATION transfer, *MOLECULAR dynamics, *PHARMACODYNAMICS, *COMMERCIAL products

Abstract

Voltage-gated sodium (NaV) channels control excitable cell functions. While structural investigations have revealed conformation details of different functional states, the mechanisms of both activation and slow inactivation remain unclear. Here, we identify residue T140 in the S4-S5 linker of the bacterial voltage-gated sodium channel NaChBac as critical for channel activation and drug effects on inactivation. Mutations at T140 either attenuate activation or render the channel nonfunctional. Propofol, a clinical anesthetic known to inhibit NaChBac by promoting slow inactivation, binds to a pocket between the S4-S5 linker and S6 helix in a conformation-dependent manner. Using 19F-NMR to quantify site-specific binding by saturation transfer differences (STDs), we found strong STDs in inactivated, but not activated, NaChBac. Molecular dynamics simulations show a highly dynamic pocket in the activated conformation, limiting STD buildup. In contrast, drug binding to this pocket promotes and stabilizes the inactivated states. Our results provide direct experimental evidence showing distinctly different associations between the S4-S5 linker and S6 helix in activated and inactivated states. Specifically, an exchange occurs between interaction partners T140 and N234 of the same subunit in activation, and T140 and N225 of the domainswapped subunit in slow inactivation. The drug action on slow inactivation of prokaryotic NaV channels seems to have a mechanism similar to the recently proposed "door-wedge" action of the isoleucine-phenylalanine-methionine (IFM) motif on the fast inactivation of eukaryotic NaV channels. Elucidating this gating mechanism points to a possible direction for conformation-dependent drug development. [ABSTRACT FROM AUTHOR]

Published

2021

3. Employing NaChBac for cryo-EM analysis of toxin action on voltage-gated Na+ channels in nanodisc.

Author

Shuai Gao, Valinsky, William C., Nguyen Cam On, Houlihan, Patrick R., Qian Qu, Lei Liu, Xiaojing Pan, Clapham, David E., and Nieng Yan

Subjects

*TOXIN analysis, *ELECTRON cryomicroscopy, *BILAYER lipid membranes, *TOXINS

Abstract

NaChBaC, the first bacterial voltage-gated Na+ (Nav) channel to be characterized, has been the prokaryotic prototype for studying the structure-function relationship of Nav channels. Discovered nearly two decades ago, the structure of NaChBac has not been determined. Here we present the single particle electron cryomicroscopy (cryo-EM) analysis of NaChBac in both detergent micelles and nanodiscs. Under both conditions, the conformation of NaChBac is nearly identical to that of the potentially inactivated NavAb. Determining the structure of NaChBac in nanodiscs enabled us to examine gating modifier toxins (GMTs) of Nav channels in lipid bilayers. To study GMTs in mammalian Nav channels, we generated a chimera in which the extracellular fragment of the S3 and S4 segments in the second voltage-sensing domain from Nav1.7 replaced the corresponding sequence in NaChBac. Cryo-EM structures of the nanodisc-embedded chimera alone and in complex with HuwenToxin IV (HWTX-IV) were determined to 3.5 and 3.2 Å resolutions, respectively. Compared to the structure of HWTX-IV-bound human Nav1.7, which was obtained at an overall resolution of 3.2 Å, the local resolution of the toxin has been improved from ~6 to ~4 Å. This resolution enabled visualization of toxin docking. NaChBac can thus serve as a convenient surrogate for structural studies of the interactions between GMTs and Nav channels in a membrane environment. [ABSTRACT FROM AUTHOR]

Published

2020

4. Theory and Experiments on Multi-Ion Permeation and Selectivity in the NaChBac Ion Channel.

Author

Gibby, W. A. T., Barabash, M. L., Guardiani, C., Luchinsky, D. G., Fedorenko, O. A., Roberts, S. K., and McClintock, P. V. E.

Subjects

*STATISTICAL equilibrium, *MOLE fraction, *ION channels, *HUMAN behavior models, *THEORY

Abstract

The highly selective permeation of ions through biological ion channels is an unsolved problem of noise and fluctuations. In this paper, we motivate and introduce a non-equilibrium and self-consistent multi-species kinetic model, with the express aims of comparing with experimental recordings of current versus voltage and concentration and extracting important permeation parameters. For self-consistency, the behavior of the model at the two-state, i.e., selective limit in linear response, must agree with recent results derived from an equilibrium statistical theory. The kinetic model provides a good fit to data, including the key result of an anomalous mole fraction effect. [ABSTRACT FROM AUTHOR]

Published

2019

5. Application of a Statistical and Linear Response Theory to Multi-Ion Na+ Conduction in NaChBac

Author

William A. T. Gibby, Olena A. Fedorenko, Carlo Guardiani, Miraslau L. Barabash, Thomas Mumby, Stephen K. Roberts, Dmitry G. Luchinsky, and Peter V. E. McClintock

Subjects

ion channel, statistical theory, linear response, ionic transport, NaChBac, Science, Astrophysics, QB460-466, Physics, QC1-999

Abstract

Biological ion channels are fundamental to maintaining life. In this manuscript we apply our recently developed statistical and linear response theory to investigate Na+ conduction through the prokaryotic Na+ channel NaChBac. This work is extended theoretically by the derivation of ionic conductivity and current in an electrochemical gradient, thus enabling us to compare to a range of whole-cell data sets performed on this channel. Furthermore, we also compare the magnitudes of the currents and populations at each binding site to previously published single-channel recordings and molecular dynamics simulations respectively. In doing so, we find excellent agreement between theory and data, with predicted energy barriers at each of the four binding sites of ∼4,2.9,3.6, and 4kT.

Published

2021

6. Divergent effects of anesthetics on lipid bilayer properties and sodium channel function.

Author

Herold, Karl, Andersen, Olaf, and Hemmings, Hugh

Subjects

*ANESTHETICS, *MEDICAL care, *HYPOTHESIS, *CRYSTALLOGRAPHY, *BILAYER lipid membranes, *THERAPEUTICS

Abstract

General anesthetics revolutionized medicine by allowing surgeons to perform more complex and much longer procedures. This widely used class of drugs is essential to patient care, yet their exact molecular mechanism(s) are incompletely understood. One early hypothesis over a century ago proposed that nonspecific interactions of anesthetics with the lipid bilayer lead to changes in neuronal function via effects on membrane properties. This model was supported by the Meyer-Overton correlation between anesthetic potency and lipid solubility and despite more recent evidence for specific protein targets, in particular ion-channels, lipid bilayer-mediated effects of anesthetics is still under debate. We therefore tested a wide range of chemically diverse general anesthetics on lipid bilayer properties using a sensitive and functional gramicidin-based assay. None of the tested anesthetics altered lipid bilayer properties at clinically relevant concentrations. Some anesthetics did affect the bilayer, though only at high supratherapeutic concentrations, which are unlikely relevant for clinical anesthesia. These results suggest that anesthetics directly interact with membrane proteins without altering lipid bilayer properties at clinically relevant concentrations. Voltage-gated Na channels are potential anesthetic targets and various isoforms are inhibited by a wide range of volatile anesthetics. They inhibit channel function by reducing peak Na current and shifting steady-state inactivation toward more hyperpolarized potentials. Recent advances in crystallography of prokaryotic Na channels, which are sensitive to volatile anesthetics, together with molecular dynamics simulations and electrophysiological studies will help identify potential anesthetic interaction sites within the channel protein itself. [ABSTRACT FROM AUTHOR]

Published

2017

7. Ionic Coulomb blockade and anomalous mole fraction effect in the NaChBac bacterial ion channel and its charge-varied mutants.

Author

Kaufman, Igor Kh., Fedorenko, Olena A., Luchinsky, Dmitri G., Gibby, William A. T., Roberts, Stephen K., McClintock, Peter V. E., and Eisenberg, Robert S.

Subjects

BIOPHYSICS, CARBENES, ION channels, ACTIVE biological transport, ION-permeable membranes

Abstract

Background. The selectivity of biological cation channels is defined by a short, narrow selectivity filter, having a negative net fixed charge Qf. Voltage gated bacterial channels (NaChBac and some others) are frequently used in biophysics as simplified models of mammalian calcium and sodium channels. We report an experimental, analytic and numerical study of the effects of Qf and bulk ionic concentrations of Ca2+ and Na+ on conduction and selectivity of NaChBac channels, wild type and Qf-varied mutants. Methods. Site-directed mutagenesis and voltage clamp recordings were used to investigate the Na+/Ca2+ selectivity, divalent blockade and anomalous mole fraction effect (AMFE) for different NaChBac wild type/ mutants channels and the properties dependence on Qf. Experimental results were compared with Brownian dynamics simulations and with analytic predictions of the ionic Coulomb blockade (ICB) model, which was extended to encompass bulk concentration effects. Results. It was shown that changing of Qf from -4e (for LESWAS wild type) to -8e (for LEDWAS mutant) leads to strong divalent blockade of the Na+ current by micromolar amounts of Ca2+ ions, similar to the effects seen in mammalian calcium channels. The BD simulations revealed a concentration-related logarithmic shift of the conduction bands. These results were shown to be consistent with ICB model predictions. Conclusions. The extended ICB model explains the experimental (divalent blockade and AMFE) and simulated (multi-ion bands and their concentration-related shifts) selectivity phenomena of NaChBac channel and its charge-varied mutants. These results extend the understanding of ion channel selectivity and may also be applicable to biomimetic nanopores with charged walls. [ABSTRACT FROM AUTHOR]

Published

2017

8. Estudio de caracterización de la línea celular Neuro-2A tras la sobreexpresión ectópica de NaChBac

Author

Llobet Serra, Enrique Javier, Moreno Manzano, Victoria, Paniagua Soriano, Gillem, and Hingorani Jai Prakask, Sonia

Subjects

AKT/PKB, SCI, 2409 Genética, mTOR, 2415 Biología Molecular, Neuro-2A, Neurite, NaChBac, Neurita, LME

Abstract

La terapia celular, concretamente el trasplante de células precursoras neuronales (CNP), es una de las principales estrategias que están siendo investigadas para el rescate funcional tras sufrir una lesión de médula espinal (LME). Aunque muy prometedoras, estas estrategias no se encuentran exentas de limitaciones. Una de ellas la encontramos en la supervivencia tras el injerto, que produce una pérdida inicial de las células trasplantadas y la disminución de la eficacia. Con el fin de superar estas limitaciones, hemos sobreexpresado un canal de sodio bacteriano regulado por voltaje, NaChBac, en una línea celular, Neuro-2A (N2A), con el objetivo de caracterizar sus efectos fisiológicos, así como mecanismos moleculares implicados, y poder aplicar la información obtenida como una estrategia en la mejora de la terapia celular para el tratamiento de lesiones medulares. Las N2A fueron transducidas mediante vectores lentivirales, portadores del plásmido pLL 3.7 control y NaChBac, y sometidas a estudios de comportamiento celular con el fin de observar los efectos fisiológicos del canal. Posteriormente se realizaron estudios inmunocitoquímicos para ver los posibles cambios en la morfología y estudios moleculares mediante Western Blot para determinar las vías de señalización involucradas. Tras analizar los resultados, se observó que aquellas células donde se había expresado el canal poseían una mayor capacidad de supervivencia y proliferación, así como la habilidad de generar neuritas de mayor longitud. Los análisis de la vías moleculares mostraron una activación mayor de AKT/PKB y mTOR en las células con NaChBac. Por tanto, la expresión del canal de sodio bacteriano NaChBac se encuentra relacionada con el aumento de actividad de importantes vías moleculares que, a su vez, explicarían los efectos fisiológicos observados. Se puede concluir que la caracterización de NaChBac aporta importantes ventajas que podrían ser aplicadas como estrategias para la mejora celular en LME. Cell therapy, specifically neural precursor cell (NPC) transplantation, is one of the main strategies being investigated for functional rescue after spinal cord injury (SCI). Although very promising, these strategies are not without limitations, one of them being post-transplant survival, which results in an initial loss of transplanted cells and decreased efficacy. To overcome these limitations, we have overexpressed a voltage-regulated bacterial sodium channel, NaChBac, in a cell line, Neuro-2A (N2A), to characterize its physiological effects, as well as molecular mechanisms involved, and to be able to apply the information obtained as a strategy in the improvement of cell therapy for the treatment of spinal cord injury. N2A were transduced using lentiviral vectors, carrying the pLL 3.7 control plasmid and NaChBac, and subjected to cell behavioral studies to observe the physiological effects of the channel. Subsequently, immunocytochemical studies were performed to see possible changes in morphology and molecular studies by Western Blot to determine the signaling pathways involved. After analyzing the results, it was observed that those cells where the channel was expressed had a greater capacity for survival and proliferation, as well as the ability to generate neurites of greater length. Molecular pathway analysis showed higher activation of AKT/PKB and mTOR in cells with NaChBac. Thus, the expression of the bacterial sodium channel NaChBac is related to the increased activity of important molecular pathways that would explain the observed physiological effects. It can be concluded that the characterization of NaChBac provides important advantages that could be applied as strategies for cellular enhancement in SCI. Biotecnología

Published

2022

9. Purification and Characterization of JZTx-14, a Potent Antagonist of Mammalian and Prokaryotic Voltage-Gated Sodium Channels

Author

Jie Zhang, Dongfang Tang, Shuangyu Liu, Haoliang Hu, Songping Liang, Cheng Tang, and Zhonghua Liu

Subjects

NaChBac, mammalian NaVs, peptide toxin, pharmacology, Medicine

Abstract

Exploring the interaction of ligands with voltage-gated sodium channels (NaVs) has advanced our understanding of their pharmacology. Herein, we report the purification and characterization of a novel non-selective mammalian and bacterial NaVs toxin, JZTx-14, from the venom of the spider Chilobrachys jingzhao. This toxin potently inhibited the peak currents of mammalian NaV1.2–1.8 channels and the bacterial NaChBac channel with low IC50 values (

Published

2018

10. Covalent linkage of bacterial voltage-gated sodium channels

Author

Olena Fedorenko, Zeyu Zheng, Stephen K. Roberts, and Huaping Sun

Subjects

0301 basic medicine, Concatenation, Biophysics, NavMs, Western blot, Bacterial sodium channels, Oligomer, law.invention, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Confocal microscopy, law, Patch clamp, lcsh:QH301-705.5, Immunodetection, Sodium channel, Wild type, lcsh:QC1-999, 030104 developmental biology, Monomer, Membrane, chemistry, lcsh:Biology (General), Covalent bond, NavAb, NaChBac, 030217 neurology & neurosurgery, lcsh:Physics, Research Article

Abstract

Background Bacterial sodium channels are important models for understanding ion permeation and selectivity. However, their homotetrameric structure limits their use as models for understanding the more complex eukaryotic voltage-gated sodium channels (which have a pseudo-heterotetrameric structure formed from an oligomer composed of four domains). To bridge this gap we attempted to synthesise oligomers made from four covalently linked bacterial sodium channel monomers and thus resembling their eukaryotic counterparts. Results Western blot analyses revealed NaChBac oligomers to be inherently unstable whereas intact expression of NavMs oligomers was possible. Immunodectection using confocal microscopy and electrophysiological characterisation of NavMs tetramers confirmed plasma membrane localisation and equivalent functionality with wild type NavMs channels when expressed in human embryonic kidney cells. Conclusion This study has generated new tools for the investigation of eukaryotic channels. The successful covalent linkage of four bacterial Nav channel monomers should permit the introduction of radial asymmetry into the structure of bacterial Nav channels and enable the known structures of these channels to be used to gain unique insights into structure-function relationships of their eukaryotic counterparts. Electronic supplementary material The online version of this article (10.1186/s13628-019-0049-5) contains supplementary material, which is available to authorized users.

Published

2019

11. Deciphering voltage-gated Na+ and Ca2+ channels by studying prokaryotic ancestors.

Author

Catterall, William A. and Zheng, Ning

Subjects

*SODIUM ions, *VOLTAGE-gated ion channels, *CALCIUM ions, *NEURAL transmission, *PROKARYOTIC genomes, *MEMBRANE proteins

Abstract

Voltage-gated sodium channels (Na V s) and calcium channels (Ca V s) are involved in electrical signaling, contraction, secretion, synaptic transmission, and other physiological processes activated in response to depolarization. Despite their physiological importance, the structures of these closely related proteins have remained elusive because of their size and complexity. Bacterial Na V s have structures analogous to a single domain of eukaryotic Na V s and Ca V s and are their likely evolutionary ancestor. Here we review recent work that has led to new understanding of Na V s and Ca V s through high-resolution structural studies of their prokaryotic ancestors. New insights into their voltage-dependent activation and inactivation, ion conductance, and ion selectivity provide realistic structural models for the function of these complex membrane proteins at the atomic level. [ABSTRACT FROM AUTHOR]

Published

2015

12. Application of a Statistical and Linear Response Theory to Multi-Ion Na+ Conduction in NaChBac

Author

Olena Fedorenko, Peter V. E. McClintock, Dmitry G. Luchinsky, Carlo Guardiani, Thomas Mumby, Miraslau L. Barabash, Stephen K. Roberts, and W. A. T. Gibby

Subjects

Work (thermodynamics), ion channel, ionic transport, linear response, NaChBac, statistical theory, MathematicsofComputing_GENERAL, General Physics and Astronomy, lcsh:Astrophysics, 01 natural sciences, Molecular physics, Article, Ion, 03 medical and health sciences, Molecular dynamics, 0103 physical sciences, lcsh:QB460-466, Ionic conductivity, Statistical theory, 010306 general physics, Electrochemical gradient, lcsh:Science, Ion channel, 030304 developmental biology, Physics, 0303 health sciences, Thermal conduction, lcsh:QC1-999, lcsh:Q, lcsh:Physics

Abstract

Biological ion channels are fundamental to maintaining life. In this manuscript we apply our recently developed statistical and linear response theory to investigate Na+ conduction through the prokaryotic Na+ channel NaChBac. This work is extended theoretically by the derivation of ionic conductivity and current in an electrochemical gradient, thus enabling us to compare to a range of whole-cell data sets performed on this channel. Furthermore, we also compare the magnitudes of the currents and populations at each binding site to previously published single-channel recordings and molecular dynamics simulations respectively. In doing so, we find excellent agreement between theory and data, with predicted energy barriers at each of the four binding sites of ∼4,2.9,3.6, and 4kT.

Published

2021

13. Molecular mechanism of the spider toxin κ-LhTx-I acting on the bacterial voltage-gated sodium channel NaChBac.

Author

Xiao Z, Li Y, Zhao P, Wu X, Luo G, Peng S, Liu H, Tang C, and Liu Z

Abstract

The bacterial sodium channel NaChBac is the prokaryotic prototype for the eukaryotic Na V and Ca V channels, which could be used as a relatively simple model to study their structure-function relationships. However, few modulators of NaChBac have been reported thus far, and the pharmacology of NaChBac remains to be investigated. In the present study, we show that the spider toxin κ-LhTx-1, an antagonist of the K V 4 family potassium channels, potently inhibits NaChBac with an IC 50 of 491.0 ± 61.7 nM. Kinetics analysis revealed that κ-LhTx-1 inhibits NaChBac by impeding the voltage-sensor activation. Site-directed mutagenesis confirmed that phenylalanine-103 (F103) in the S3-S4 extracellular loop of NaChBac was critical for interacting with κ-LhTx-1. Molecular docking predicts the binding interface between κ-LhTx-1 and NaChBac and highlights a dominant hydrophobic interaction between W27 in κ-LhTx-1 and F103 in NaChBac that stabilizes the interface. In contrast, κ-LhTx-1 showed weak activity on the mammalian Na V channels, with 10 µM toxin slightly inhibiting the peak currents of Na V 1.2-1.9 subtypes. Taken together, our study shows that κ-LhTx-1 inhibits the bacterial sodium channel, NaChBac, using a voltage-sensor trapping mechanism similar to mammalian Na V site 4 toxins. κ-LhTx-1 could be used as a ligand to study the toxin-channel interactions in the native membrane environments, given that the NaChBac structure was successfully resolved in a nanodisc., Competing Interests: The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest., (Copyright © 2022 Xiao, Li, Zhao, Wu, Luo, Peng, Liu, Tang and Liu.)

Published

2022

14. Covalent linkage of bacterial voltage-gated sodium channels

Author

Sun, Huaping, Zheng, Zeyu, Fedorenko, Olena A., and Roberts, Stephen K.

Published

2019

15. Hinge-bending motions in the pore domain of a bacterial voltage-gated sodium channel

Author

Barber, Annika F., Carnevale, Vincenzo, Raju, S.G., Amaral, Cristiano, Treptow, Werner, and Klein, Michael L.

Subjects

*BACTERIAL proteins, *MOLECULAR structure, *CLUSTER analysis (Statistics), *PHENYLALANINE, *CONFORMATIONAL analysis, *PROLINE, *MOLECULAR dynamics

Abstract

Abstract: Computational methods and experimental data are used to provide structural models for NaChBac, the homo-tetrameric voltage-gated sodium channel from the bacterium Bacillus halodurans, with a closed and partially open pore domain. Molecular dynamic (MD) simulations on membrane-bound homo-tetrameric NaChBac structures, each comprising six helical transmembrane segments (labeled S1 through S6), reveal that the shape of the lumen, which is defined by the bundle of four alpha-helical S6 segments, is modulated by hinge bending motions around the S6 glycine residues. Mutation of these glycine residues into proline and alanine affects, respectively, the structure and conformational flexibility of the S6 bundle. In the closed channel conformation, a cluster of stacked phenylalanine residues from the four S6 helices hinders diffusion of water molecules and Na+ ions. Activation of the voltage sensor domains causes destabilization of the aforementioned cluster of phenylalanines, leading to a more open structure. The conformational change involving the phenylalanine cluster promotes a kink in S6, suggesting that channel gating likely results from the combined action of hinge-bending motions of the S6 bundle and concerted reorientation of the aromatic phenylalanine side-chains. [Copyright &y& Elsevier]

Published

2012

16. The C-terminal coiled-coil of the bacterial voltage-gated sodium channel NaChBac is not essential for tetramer formation, but stabilizes subunit-to-subunit interactions

Author

Mio, Kazuhiro, Mio, Muneyo, Arisaka, Fumio, Sato, Masahiko, and Sato, Chikara

Subjects

*SODIUM channels, *PROKARYOTES, *GENOMES, *CELL membranes, *ELECTRON microscopy, *CYTOPLASM, *MOLECULAR structure

Abstract

Abstract: The NaChBac is a prokaryotic homologue of the voltage-gated sodium channel found in the genome of the alkalophilic bacterium Bacillus halodurans C-125. Like a repeating cassette of mammalian sodium channel, the NaChBac possesses hydrophobic domains corresponding to six putative transmembrane segments and a pore loop, and exerts channel function by forming a tetramer although detailed mechanisms of subunit assembly remain unclear. We generated truncated mutants from NaChBac, and investigated their ability to form tetramers in relation to their channel functions. A mutant that deletes almost all of the C-terminal coiled-coil structure lost its voltage-dependent ion permeability, although it was properly translocated to the cell surface. The mutant protein was purified as a tetramer using a reduced concentration of detergent, but the association between the subunits was shown to be much weaker than the wild type. The chemical cross-linking, blue native PAGE, sedimentation velocity experiments, size exclusion chromatography, immunoprecipitation, and electron microscopy all supported its tetrameric assembly. We further purified the C-terminal cytoplasmic domain alone and confirmed its self-oligomerization. These data suggest that the C-terminal coiled-coil structure stabilizes subunit-to-subunit interactions of NaChBac, but is not critical for their tetramer formation. [ABSTRACT FROM AUTHOR]

Published

2010

17. Evidence for lateral mobility of voltage sensors in prokaryotic voltage-gated sodium channels

Author

Nagura, Hitoshi, Irie, Katsumasa, Imai, Tomoya, Shimomura, Takushi, Hige, Toshihide, and Fujiyoshi, Yoshinori

Subjects

*TETRAMERS (Oligomers), *ELECTRIC potential, *SODIUM channels, *BILAYER lipid membranes, *MEMBRANE proteins, *PROKARYOTES

Abstract

Abstract: Voltage-sensor domains (VSDs) in voltage-gated ion channels are thought to regulate the probability that a channel adopts an open conformation by moving vertically in the lipid bilayer. Here we characterized the movement of the VSDs of the prokaryotic voltage-gated sodium channel, NaChBac. Substitution of residue T110, which is located on the extracellular side of the fourth transmembrane helix of the VSD, by cysteine resulted in the formation of a disulfide bond between adjacent subunits in the channel. Our results suggest that T110 residues in VSDs of adjacent subunits can come into close proximity, implying that the VSDs can move laterally in the membrane and constitute a mechanism that regulates channel activity. [Copyright &y& Elsevier]

Published

2010

18. Motility and chemotaxis in alkaliphilic Bacillus species.

Published

2009

19. Accessibility of Four Arginine Residues on the S4 Segment of the Bacillus halodurans Sodium Channel.

Author

Blanchet, Jonathan and Chahine, Mohamed

Subjects

*ARGININE, *AMINO acids, *MUTAGENESIS, *GENETIC mutation, *ANTIMITOTIC agents

Abstract

The voltage-gated Na+ channel of Bacillus halodurans (NaChBac) is composed of six transmembrane segments (S1–S6), with a pore-forming region composed of segments S5 and S6 and a voltage-sensing domain composed of segments S1–S4. The S4 segment forms the core of the voltage sensor. We explored the accessibility of four arginine residues on the S4 segment of NaChBac, which are positioned at every third position from each other. These arginine residues on the S4 segment were replaced with cysteines using site-directed mutagenesis. Na+ currents were recorded using the whole-cell configuration of the patch-clamp technique. We tested the effect of the sulfhydryl reagents applied from inside and outside the cellular space in the open and closed conformations. Structural models of the voltage sensor of NaChBac were constructed based on the recently crystallized KvAP and Kv1.2 K+ channels to visualize arginine residue accessibility. Our results suggest that arginine accessibility did not change significantly between the open and closed conformations, supporting the idea of a small movement of the S4 segment during gating. Molecular modeling of the closed conformation also supported a small movement of S4, which is mainly characterized by a rotation and a tilt along the periphery of the pore. Interestingly, the second arginine residue of the S4 segment (R114) was accessible to sulfhydryl reagents from both sides of the membrane in the closed conformation and, based on our model, seemed to be at the junction of the intracellular and extracellular water crevices. [ABSTRACT FROM AUTHOR]

Published

2007

20. Role of Arginine Residues on the S4 Segment of theBacillus haloduransNa+ Channel in Voltage-sensing.

Author

Chahine, M., Pilote, S., Pouliot, V., Takami, H., and Sato, C.

Subjects

*ARGININE, *BACILLUS (Bacteria), *SODIUM channels, *AMINO acids, *LYSINE, *MUTAGENESIS

Abstract

The one-domain voltage-gated sodium channel ofBacillus halodurans(NaChBac) is composed of six transmembrane segments (S1-S6) comprising a pore-forming region flanked by segments S5 and S6 and a voltage-sensing element composed of segment S4. To investigate the role of the S4 segment in NaChBac channel activation, we used the cysteine mutagenesis approach where the positive charges of single and multiple arginine (R) residues of the S4 segment were replaced by the neutrally charged amino acid cysteine (C). To determine whether it was the arginine residue itself or its positive charge that was involved in channel activation, arginine to lysine (R to K) mutations were constructed. Wild-type (WT) and mutant NaChBac channels were expressed in tsA201 cells and Na+ currents were recorded using the whole-cell configuration of the patch-clamp technique. The current/voltage (I-V) and conductance/voltage (G-V) relationships steady-state inactivation (h8) and recovery from inactivation were evaluated to determine the effects of the S4 mutations on the biophysical properties of the NaChBac channel. R to C on the S4 segment resulted in a slowing of both activation and inactivation kinetics. Charge neutralization of arginine residues mostly resulted in a shift toward more positive potentials ofG-Vandh8 curves. TheG-Vcurve shifts were associated with a decrease in slope, which may reflect a decrease in the gating charge involved in channel activation. Single neutralization of R114, R117, or R120 by C resulted in a very slow recovery from inactivation. Double neutralization of R111 and R129 confirmed the role of R111 in activation and suggested that R129 is most probably not part of the voltage sensor. Most of the R to K mutants retained WT-like current kinetics but exhibited an intermediateG-Vcurve, a steady-state inactivation shifted to more hyperpolarized potentials, and intermediate time constants of recovery from inactivation. This indicates that R, at several positions, plays an important role in channel activation. The data are consistent with the notion that the S4 is most probably the voltage sensor of the NaChBac channel and that both positive charges and the nature of the arginine residues are essential for channel activation. [ABSTRACT FROM AUTHOR]

Published

2004

21. Application of a Statistical and Linear Response Theory to Multi-Ion Na + Conduction in NaChBac.

Author

Gibby, William A. T., Fedorenko, Olena A., Guardiani, Carlo, Barabash, Miraslau L., Mumby, Thomas, Roberts, Stephen K., Luchinsky, Dmitry G., McClintock, Peter V. E., and Scarfone, Antonio M.

Subjects

*MOLECULAR dynamics, *BINDING sites, *IONIC conductivity, *ACTIVATION energy

Abstract

Biological ion channels are fundamental to maintaining life. In this manuscript we apply our recently developed statistical and linear response theory to investigate Na + conduction through the prokaryotic Na + channel NaChBac. This work is extended theoretically by the derivation of ionic conductivity and current in an electrochemical gradient, thus enabling us to compare to a range of whole-cell data sets performed on this channel. Furthermore, we also compare the magnitudes of the currents and populations at each binding site to previously published single-channel recordings and molecular dynamics simulations respectively. In doing so, we find excellent agreement between theory and data, with predicted energy barriers at each of the four binding sites of ∼ 4 , 2.9 , 3.6 , and 4 k T . [ABSTRACT FROM AUTHOR]

Published

2021

22. Regulation and drug modulation of a voltage-gated sodium channel: Pivotal role of the S4-S5 linker in activation and slow inactivation.

Author

Xiao J, Bondarenko V, Wang Y, Suma A, Wells M, Chen Q, Tillman T, Luo Y, Yu B, Dailey WP, Eckenhoff R, Tang P, Carnevale V, Klein ML, and Xu Y

Subjects

Amino Acid Sequence, Bacterial Proteins genetics, Binding Sites, HEK293 Cells, Humans, Models, Molecular, Mutation genetics, Protein Structure, Secondary, Sodium Channels genetics, Structure-Activity Relationship, Bacterial Proteins chemistry, Bacterial Proteins metabolism, Ion Channel Gating drug effects, Propofol pharmacology, Sodium Channels chemistry, Sodium Channels metabolism

Abstract

Voltage-gated sodium (Na V ) channels control excitable cell functions. While structural investigations have revealed conformation details of different functional states, the mechanisms of both activation and slow inactivation remain unclear. Here, we identify residue T140 in the S4-S5 linker of the bacterial voltage-gated sodium channel NaChBac as critical for channel activation and drug effects on inactivation. Mutations at T140 either attenuate activation or render the channel nonfunctional. Propofol, a clinical anesthetic known to inhibit NaChBac by promoting slow inactivation, binds to a pocket between the S4-S5 linker and S6 helix in a conformation-dependent manner. Using 19 F-NMR to quantify site-specific binding by saturation transfer differences (STDs), we found strong STDs in inactivated, but not activated, NaChBac. Molecular dynamics simulations show a highly dynamic pocket in the activated conformation, limiting STD buildup. In contrast, drug binding to this pocket promotes and stabilizes the inactivated states. Our results provide direct experimental evidence showing distinctly different associations between the S4-S5 linker and S6 helix in activated and inactivated states. Specifically, an exchange occurs between interaction partners T140 and N234 of the same subunit in activation, and T140 and N225 of the domain-swapped subunit in slow inactivation. The drug action on slow inactivation of prokaryotic Na V channels seems to have a mechanism similar to the recently proposed "door-wedge" action of the isoleucine-phenylalanine-methionine (IFM) motif on the fast inactivation of eukaryotic Na V channels. Elucidating this gating mechanism points to a possible direction for conformation-dependent drug development., Competing Interests: The authors declare no competing interest., (Copyright © 2021 the Author(s). Published by PNAS.)

Published

2021

23. Ionic Coulomb blockade and anomalous mole fraction effect in the NaChBac bacterial ion channel and its charge-varied mutants

Author

Peter V. E. McClintock, Olena Fedorenko, Dmitry G. Luchinsky, Stephen K. Roberts, Robert S. Eisenberg, I. Kaufman, and W. A. T. Gibby

Subjects

0301 basic medicine, bacterial channel, Voltage clamp, ionic Coulomb blockade, Analytical chemistry, 01 natural sciences, Divalent, Ion, patch-clamp technique, lcsh:RC321-571, 03 medical and health sciences, electrostatic model, Brownian dynamics simulations, 0103 physical sciences, 010306 general physics, lcsh:Neurosciences. Biological psychiatry. Neuropsychiatry, lcsh:QH301-705.5, Ion channel, chemistry.chemical_classification, Voltage-gated ion channel, Voltage-dependent calcium channel, Sodium channel, Coulomb blockade, 030104 developmental biology, chemistry, lcsh:Biology (General), Biophysics, site-directed mutagenesis, NaChBac

Abstract

Background. The selectivity of biological cation channels is defined by a short, narrow selectivity filter, having a negative net fixed charge Qf . Voltage gated bacterial channels (NaChBac and some others) are frequently used in biophysics as simplified models of mammalian calcium and sodium channels. We report an experimental, analytic and numerical study of the effects of Qf and bulk ionic concentrations of Ca2+ and Na+ on conduction and selectivity of NaChBac channels, wild type and Qf -varied mutants. Methods. Site-directed mutagenesis and voltage clamp recordings were used to investigate the Na+ /Ca2+ selectivity, divalent blockade and anomalous mole fraction effect (AMFE) for different NaChBac wild type/mutants channels and the properties dependence on Qf . Experimental results were compared with Brownian dynamics simulations and with analytic predictions of the ionic Coulomb blockade (ICB) model, which was extended to encompass bulk concentration effects. Results. It was shown that changing of Qf from –4e (for LESWAS wild type) to –8e (for LEDWAS mutant) leads to strong divalent blockade of the Na+ current by micromolar amounts of Ca2+ ions, similar to the effects seen in mammalian calcium channels. The BD simulations revealed a concentration-related logarithmic shift of the conduction bands. These results were shown to be consistent with ICB model predictions. Conclusions. The extended ICB model explains the experimental (divalent blockade and AMFE) and simulated (multi-ion bands and their concentration-related shifts) selectivity phenomena of NaChBac channel and its charge-varied mutants. These results extend the understanding of ion channel selectivity and may also be applicable to biomimetic nanopores with charged walls.

Published

2017

24. Theory and Experiments on Multi-Ion Permeation and Selectivity in the NaChBac Ion Channel

Author

Peter V. E. McClintock, Dmitry G. Luchinsky, Miraslau L. Barabash, Stephen K. Roberts, Olena Fedorenko, W. A. T. Gibby, and Carlo Guardiani

Subjects

Materials science, 010304 chemical physics, General Mathematics, General Physics and Astronomy, Thermodynamics, Permeation, Mole fraction, 01 natural sciences, Noise (electronics), Ion, 0103 physical sciences, kinetic theory, Kinetic theory of gases, anomalous mole fraction effect, Ion channel, NaChBac, Statistical theory, 010306 general physics, Voltage

Abstract

The highly selective permeation of ions through biological ion channels is an unsolved problem of noise and fluctuations. In this paper, we motivate and introduce a non-equilibrium and self-consistent multi-species kinetic model, with the express aims of comparing with experimental recordings of current versus voltage and concentration and extracting important permeation parameters. For self-consistency, the behavior of the model at the two-state, i.e., selective limit in linear response, must agree with recent results derived from an equilibrium statistical theory. The kinetic model provides a good fit to data, including the key result of an anomalous mole fraction effect.

Published

2019

25. Hinge-bending motions in the pore domain of a bacterial voltage-gated sodium channel

Author

Cristiano Amaral, Werner Treptow, Vincenzo Carnevale, Michael L. Klein, Annika F. Barber, and S. G. Raju

Subjects

Models, Molecular, Conformational change, Time Factors, Protein Conformation, Phenylalanine, Glycine, Molecular Conformation, Biophysics, Bacillus, Voltage-Gated Sodium Channels, Gating, Molecular Dynamics Simulation, Biochemistry, Article, Protein Structure, Secondary, Sodium Channels, Membrane Potentials, Motion, 03 medical and health sciences, Molecular dynamics, 0302 clinical medicine, Protein structure, Bacterial Proteins, 030304 developmental biology, Ions, 0303 health sciences, Voltage-gated ion channel, biology, Sodium channel, Chemistry, Sodium, Bacterial channel, Cell Biology, biology.organism_classification, Transmembrane protein, Protein Structure, Tertiary, Crystallography, Voltage gated, Bacillus halodurans, Ion Channel Gating, NaChBac, 030217 neurology & neurosurgery

Abstract

Computational methods and experimental data are used to provide structural models for NaChBac, the homo-tetrameric voltage-gated sodium channel from the bacterium Bacillus halodurans, with a closed and partially open pore domain. Molecular dynamic (MD) simulations on membrane-bound homo-tetrameric NaChBac structures, each comprising six helical transmembrane segments (labeled S1 through S6), reveal that the shape of the lumen, which is defined by the bundle of four alpha-helical S6 segments, is modulated by hinge bending motions around the S6 glycine residues. Mutation of these glycine residues into proline and alanine affects, respectively, the structure and conformational flexibility of the S6 bundle. In the closed channel conformation, a cluster of stacked phenylalanine residues from the four S6 helices hinders diffusion of water molecules and Na+ ions. Activation of the voltage sensor domains causes destabilization of the aforementioned cluster of phenylalanines, leading to a more open structure. The conformational change involving the phenylalanine cluster promotes a kink in S6, suggesting that channel gating likely results from the combined action of hinge-bending motions of the S6 bundle and concerted reorientation of the aromatic phenylalanine side-chains.

Published

2012

26. Employing NaChBac for cryo-EM analysis of toxin action on voltage-gated Na + channels in nanodisc.

Author

Gao S, Valinsky WC, On NC, Houlihan PR, Qu Q, Liu L, Pan X, Clapham DE, and Yan N

Subjects

Animals, Bacterial Proteins genetics, Humans, Lipid Bilayers chemistry, Models, Molecular, Protein Conformation, Sodium Channels, Spider Venoms chemistry, Voltage-Gated Sodium Channels genetics, Bacterial Proteins chemistry, Cryoelectron Microscopy methods, Nanostructures chemistry, Voltage-Gated Sodium Channels chemistry, Voltage-Gated Sodium Channels metabolism

Abstract

NaChBac, the first bacterial voltage-gated Na + (Na v ) channel to be characterized, has been the prokaryotic prototype for studying the structure-function relationship of Na v channels. Discovered nearly two decades ago, the structure of NaChBac has not been determined. Here we present the single particle electron cryomicroscopy (cryo-EM) analysis of NaChBac in both detergent micelles and nanodiscs. Under both conditions, the conformation of NaChBac is nearly identical to that of the potentially inactivated Na v Ab. Determining the structure of NaChBac in nanodiscs enabled us to examine gating modifier toxins (GMTs) of Na v channels in lipid bilayers. To study GMTs in mammalian Na v channels, we generated a chimera in which the extracellular fragment of the S3 and S4 segments in the second voltage-sensing domain from Na v 1.7 replaced the corresponding sequence in NaChBac. Cryo-EM structures of the nanodisc-embedded chimera alone and in complex with HuwenToxin IV (HWTX-IV) were determined to 3.5 and 3.2 Å resolutions, respectively. Compared to the structure of HWTX-IV-bound human Na v 1.7, which was obtained at an overall resolution of 3.2 Å, the local resolution of the toxin has been improved from ∼6 to ∼4 Å. This resolution enabled visualization of toxin docking. NaChBac can thus serve as a convenient surrogate for structural studies of the interactions between GMTs and Na v channels in a membrane environment., Competing Interests: The authors declare no competing interest.

Published

2020

27. Role of Arginine Residues on the S4 Segment of the Bacillus halodurans Na+ Channel in Voltage-sensing

Author

Chahine, M., Pilote, S., Pouliot, V., Takami, H., and Sato, C.

Published

2004

28. Purification and Characterization of JZTx-14, a Potent Antagonist of Mammalian and Prokaryotic Voltage-Gated Sodium Channels.

Author

Liu, Shuangyu, Hu, Haoliang, Liang, Songping, Tang, Cheng, Liu, Zhonghua, Zhang, Jie, and Tang, Dongfang

Subjects

*PEPTIDES, *TOXINS, *PHARMACOLOGY, *PROKARYOTES, *VOLTAGE-gated ion channels

Abstract

Exploring the interaction of ligands with voltage-gated sodium channels (NaVs) has advanced our understanding of their pharmacology. Herein, we report the purification and characterization of a novel non-selective mammalian and bacterial NaVs toxin, JZTx-14, from the venom of the spider Chilobrachys jingzhao. This toxin potently inhibited the peak currents of mammalian NaV1.2–1.8 channels and the bacterial NaChBac channel with low IC50 values (<1 µM), and it mainly inhibited the fast inactivation of the NaV1.9 channel. Analysis of NaV1.5/NaV1.9 chimeric channel showed that the NaV1.5 domain II S3–4 loop is involved in toxin association. Kinetics data obtained from studying toxin–NaV1.2 channel interaction showed that JZTx-14 was a gating modifier that possibly trapped the channel in resting state; however, it differed from site 4 toxin HNTx-III by irreversibly blocking NaV currents and showing state-independent binding with the channel. JZTx-14 might stably bind to a conserved toxin pocket deep within the NaV1.2–1.8 domain II voltage sensor regardless of channel conformation change, and its effect on NaVs requires the toxin to trap the S3–4 loop in its resting state. For the NaChBac channel, JZTx-14 positively shifted its conductance-voltage (G–V) and steady-state inactivation relationships. An alanine scan analysis of the NaChBac S3–4 loop revealed that the 108th phenylalanine (F108) was the key residue determining the JZTx-14–NaChBac interaction. In summary, this study provided JZTx-14 with potent but promiscuous inhibitory activity on both the ancestor bacterial NaVs and the highly evolved descendant mammalian NaVs, and it is a useful probe to understand the pharmacology of NaVs. [ABSTRACT FROM AUTHOR]

Published

2018

29. Purification and Characterization of JZTx-14, a Potent Antagonist of Mammalian and Prokaryotic Voltage-Gated Sodium Channels.

Author

Zhang J, Tang D, Liu S, Hu H, Liang S, Tang C, and Liu Z

Subjects

Amino Acid Sequence, Animals, Bacterial Proteins physiology, Cell Line, Humans, Mice, Rats, Sequence Analysis, Protein, Voltage-Gated Sodium Channels physiology, Spider Venoms chemistry, Spider Venoms isolation & purification, Spider Venoms pharmacology, Voltage-Gated Sodium Channel Blockers chemistry, Voltage-Gated Sodium Channel Blockers isolation & purification, Voltage-Gated Sodium Channel Blockers pharmacology

Abstract

Exploring the interaction of ligands with voltage-gated sodium channels (Na V s) has advanced our understanding of their pharmacology. Herein, we report the purification and characterization of a novel non-selective mammalian and bacterial Na V s toxin, JZTx-14, from the venom of the spider Chilobrachys jingzhao . This toxin potently inhibited the peak currents of mammalian Na V 1.2⁻1.8 channels and the bacterial NaChBac channel with low IC 50 values (<1 µM), and it mainly inhibited the fast inactivation of the Na V 1.9 channel. Analysis of Na V 1.5/Na V 1.9 chimeric channel showed that the Na V 1.5 domain II S3⁻4 loop is involved in toxin association. Kinetics data obtained from studying toxin⁻Na V 1.2 channel interaction showed that JZTx-14 was a gating modifier that possibly trapped the channel in resting state; however, it differed from site 4 toxin HNTx-III by irreversibly blocking Na V currents and showing state-independent binding with the channel. JZTx-14 might stably bind to a conserved toxin pocket deep within the Na V 1.2⁻1.8 domain II voltage sensor regardless of channel conformation change, and its effect on Na V s requires the toxin to trap the S3⁻4 loop in its resting state. For the NaChBac channel, JZTx-14 positively shifted its conductance-voltage (G⁻V) and steady-state inactivation relationships. An alanine scan analysis of the NaChBac S3⁻4 loop revealed that the 108th phenylalanine (F108) was the key residue determining the JZTx-14⁻NaChBac interaction. In summary, this study provided JZTx-14 with potent but promiscuous inhibitory activity on both the ancestor bacterial Na V s and the highly evolved descendant mammalian Na V s, and it is a useful probe to understand the pharmacology of Na V s.

Published

2018

30. Solution NMR Studies of Anesthetic Interactions with Ion Channels.

Author

Bondarenko V, Wells M, Xu Y, and Tang P

Subjects

Bacterial Proteins genetics, Bacterial Proteins metabolism, Binding Sites, Escherichia coli genetics, Escherichia coli metabolism, Fluorine chemistry, Gene Expression, Halothane chemistry, Humans, Isoflurane chemistry, Ketamine chemistry, Membranes, Artificial, Molecular Dynamics Simulation, Protein Binding, Protein Domains, Receptors, Nicotinic genetics, Receptors, Nicotinic metabolism, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins metabolism, Sodium Channels genetics, Sodium Channels metabolism, alpha7 Nicotinic Acetylcholine Receptor genetics, alpha7 Nicotinic Acetylcholine Receptor metabolism, Anesthetics, Inhalation chemistry, Anesthetics, Intravenous chemistry, Bacterial Proteins chemistry, Magnetic Resonance Spectroscopy methods, Receptors, Nicotinic chemistry, Sodium Channels chemistry, Staining and Labeling methods, alpha7 Nicotinic Acetylcholine Receptor chemistry

Abstract

NMR spectroscopy is one of the major tools to provide atomic resolution protein structural information. It has been used to elucidate the molecular details of interactions between anesthetics and ion channels, to identify anesthetic binding sites, and to characterize channel dynamics and changes introduced by anesthetics. In this chapter, we present solution NMR methods essential for investigating interactions between ion channels and general anesthetics, including both volatile and intravenous anesthetics. Case studies are provided with a focus on pentameric ligand-gated ion channels and the voltage-gated sodium channel NaChBac., (© 2018 Elsevier Inc. All rights reserved.)

Published

2018

31. Characterization of NaChBac in Artificial Lipid Bilayer Membrane

Author

Jo, Andrew

Subjects

BLM, NaChBac

Abstract

Abstract: NaChBac is a voltage-gated Na+ channel from the bacterium Bacillus haloduran. Studying this protein channel can help researchers discover potential pharmaceuticals, innovative strategies in eliminating biofilms, and could be used to improve desalinization technologies. This thesis will discuss the charaterization of NaChBac in artifical lipid membrane, including single molecule study on the conductance and ion selectivity using a planar bilayer membrane device and the development of a scattered light based stopped-flow flux assay. Planar lipid bilayer membrane is a common technique to characterize ion channel function. In this thesis, purified NaChBac protein was incorporated into lipid vesicles which were then fused to a planar lipid bilayer. By applying a controllable electrical potential (i.e. voltage) across the protein-embedded bilayer and measuring the resulting current, the conductance, gating behaviour, and ion selectivity of the open channel were studied. NaChBac was found to have three conductance levels at 268.5 ± 45.2 pS (mean ± SEM, n=2), 92.8 ± 18.0 pS (n=3), and 26.4 ± 5.6 pS (n=4), respectively. Its activation gating voltage (V1/2) is -28 mV and its apparent activation gating charge is 15.9 elementary charge. NaChBac tested under asymmetric saline buffer solution conditions was shown to have a relative permeability PNa+/PK+ ranging from 0.86 to 1.35 and PNa+/PCa2+ = 1.43 ± 0.20 (n=3, ±SEM). Conventional flux assay for ion channels requires the use of ion-specific dyes. However, the availability of the dyes and their selectivity limits the spectrum of ion channels that can be tested in a fluorescence flux assay. Instead, stopped-flow spectrometry can be used to monitor the change in size of the protein-incorporating vesicles that is caused by ion flux, which is in turn triggered by the transmembrane electrochemical gradient of the target ion species. With this method, the ion conducting function of purified NaChBac protein was shown. The method can potentially be used to test the functionality of other ion channels.

Published

2016

32. Control of Spontaneous Ca2+ Transients Is Critical for Neuronal Maturation in the Developing Neocortex.

Author

Bando Y, Irie K, Shimomura T, Umeshima H, Kushida Y, Kengaku M, Fujiyoshi Y, Hirano T, and Tagawa Y

Subjects

Animals, Dendrites metabolism, Mice, Neocortex metabolism, Neurogenesis physiology, Neurons physiology, Calcium metabolism, Cell Differentiation physiology, Cell Movement physiology, Neocortex growth & development, Neuroglia cytology, Neurons cytology

Abstract

Neural activity plays roles in the later stages of development of cortical excitatory neurons, including dendritic and axonal arborization, remodeling, and synaptogenesis. However, its role in earlier stages, such as migration and dendritogenesis, is less clear. Here we investigated roles of neural activity in the maturation of cortical neurons, using calcium imaging and expression of prokaryotic voltage-gated sodium channel, NaChBac. Calcium imaging experiments showed that postmigratory neurons in layer II/III exhibited more frequent spontaneous calcium transients than migrating neurons. To test whether such an increase of neural activity may promote neuronal maturation, we elevated the activity of migrating neurons by NaChBac expression. Elevation of neural activity impeded migration, and induced premature branching of the leading process before neurons arrived at layer II/III. Many NaChBac-expressing neurons in deep cortical layers were not attached to radial glial fibers, suggesting that these neurons had stopped migration. Morphological and immunohistochemical analyses suggested that branched leading processes of NaChBac-expressing neurons differentiated into dendrites. Our results suggest that developmental control of spontaneous calcium transients is critical for maturation of cortical excitatory neurons in vivo: keeping cellular excitability low is important for migration, and increasing spontaneous neural activity may stop migration and promote dendrite formation., (© The Author 2014. Published by Oxford University Press. All rights reserved. For Permissions, please e-mail: journals.permissions@oup.com.)

Published

2016