Inverted allosteric coupling between activation and inactivation gates in K+ channels

The selectivity filter and the activation gate in potassium channels are functionally and structurally coupled. An allosteric coupling underlies C-type inactivation coupled to activation gating in this ion-channel family (i.e., opening of the activation gate triggers the collapse of the channel’s selectivity filter). We have identified the second Threonine residue within the TTVGYGD signature sequence of K+ channels as a crucial residue for this allosteric communication. A Threonine to Alanine substitution at this position was studied in three representative members of the K+-channel family. Interestingly, all of the mutant channels exhibited lack of C-type inactivation gating and an inversion of their allosteric coupling (i.e., closing of the activation gate collapses the channel’s selectivity filter). A state-dependent crystallographic study of KcsA-T75A proves that, on activation, the selectivity filter transitions from a nonconductive and deep C-type inactivated conformation to a conductive one. Finally, we provide a crystallographic demonstration that closed-state inactivation can be achieved by the structural collapse of the channel’s selectivity filter.

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Computational study of non-conductive selectivity filter conformations and C-type inactivation in a voltage-dependent potassium channel

The Journal of General Physiology ◽

10.1085/jgp.202112875 ◽

2021 ◽

Vol 153 (9) ◽

Author(s):

Jing Li ◽

Rong Shen ◽

Ahmed Rohaim ◽

Ramon Mendoza Uriarte ◽

Mikolai Fajer ◽

...

Keyword(s):

Potassium Channel ◽

Computational Study ◽

Homology Model ◽

Selectivity Filter ◽

K Channels ◽

Activation Gate ◽

Voltage Dependent ◽

Signature Sequence ◽

Dynamics Simulations ◽

Pore Domain

C-type inactivation is a time-dependent process of great physiological significance that is observed in a large class of K+ channels. Experimental and computational studies of the pH-activated KcsA channel show that the functional C-type inactivated state, for this channel, is associated with a structural constriction of the selectivity filter at the level of the central glycine residue in the signature sequence, TTV(G)YGD. The structural constriction is allosterically promoted by the wide opening of the intracellular activation gate. However, whether this is a universal mechanism for C-type inactivation has not been established with certainty because similar constricted structures have not been observed for other K+ channels. Seeking to ascertain the general plausibility of the constricted filter conformation, molecular dynamics simulations of a homology model of the pore domain of the voltage-gated potassium channel Shaker were performed. Simulations performed with an open intracellular gate spontaneously resulted in a stable constricted-like filter conformation, providing a plausible nonconductive state responsible for C-type inactivation in the Shaker channel. While there are broad similarities with the constricted structure of KcsA, the hypothetical constricted-like conformation of Shaker also displays some subtle differences. Interestingly, those are recapitulated by the Shaker-like E71V KcsA mutant, suggesting that the residue at this position along the pore helix plays a pivotal role in determining the C-type inactivation behavior. Free energy landscape calculations show that the conductive-to-constricted transition in Shaker is allosterically controlled by the degree of opening of the intracellular activation gate, as observed with the KcsA channel. The behavior of the classic inactivating W434F Shaker mutant is also characterized from a 10-μs MD simulation, revealing that the selectivity filter spontaneously adopts a nonconductive conformation that is constricted at the level of the second glycine in the signature sequence, TTVGY(G)D.

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Role of protein dynamics in ion selectivity and allosteric coupling in the NaK channel

Proceedings of the National Academy of Sciences ◽

10.1073/pnas.1515965112 ◽

2015 ◽

Vol 112 (50) ◽

pp. 15366-15371 ◽

Cited By ~ 8

Author(s):

Joshua B. Brettmann ◽

Darya Urusova ◽

Marco Tonelli ◽

Jonathan R. Silva ◽

Katherine A. Henzler-Wildman

Keyword(s):

Ion Selectivity ◽

Selectivity Filter ◽

Structural Basis ◽

Functional Coupling ◽

Dynamic Coupling ◽

Allosteric Coupling ◽

Allosteric Communication ◽

Dependent Inactivation ◽

Ion Binding Sites ◽

Essential Connection

Flux-dependent inactivation that arises from functional coupling between the inner gate and the selectivity filter is widespread in ion channels. The structural basis of this coupling has only been well characterized in KcsA. Here we present NMR data demonstrating structural and dynamic coupling between the selectivity filter and intracellular constriction point in the bacterial nonselective cation channel, NaK. This transmembrane allosteric communication must be structurally different from KcsA because the NaK selectivity filter does not collapse under low-cation conditions. Comparison of NMR spectra of the nonselective NaK and potassium-selective NaK2K indicates that the number of ion binding sites in the selectivity filter shifts the equilibrium distribution of structural states throughout the channel. This finding was unexpected given the nearly identical crystal structure of NaK and NaK2K outside the immediate vicinity of the selectivity filter. Our results highlight the tight structural and dynamic coupling between the selectivity filter and the channel scaffold, which has significant implications for channel function. NaK offers a distinct model to study the physiologically essential connection between ion conduction and channel gating.

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Closed state-coupled C-type inactivation in BK channels

Proceedings of the National Academy of Sciences ◽

10.1073/pnas.1607584113 ◽

2016 ◽

Vol 113 (25) ◽

pp. 6991-6996 ◽

Cited By ~ 2

Author(s):

Jiusheng Yan ◽

Qin Li ◽

Richard W. Aldrich

Keyword(s):

Conformational Changes ◽

Bk Channels ◽

Bk Channel ◽

Membrane Potentials ◽

Selectivity Filter ◽

Open Probability ◽

Closed State ◽

State Dependent ◽

Channel Opening ◽

Activation Gate

Ion channels regulate ion flow by opening and closing their pore gates. K+ channels commonly possess two pore gates, one at the intracellular end for fast channel activation/deactivation and the other at the selectivity filter for slow C-type inactivation/recovery. The large-conductance calcium-activated potassium (BK) channel lacks a classic intracellular bundle-crossing activation gate and normally show no C-type inactivation. We hypothesized that the BK channel’s activation gate may spatially overlap or coexist with the C-type inactivation gate at or near the selectivity filter. We induced C-type inactivation in BK channels and studied the relationship between activation/deactivation and C-type inactivation/recovery. We observed prominent slow C-type inactivation/recovery in BK channels by an extreme low concentration of extracellular K+ together with a Y294E/K/Q/S or Y279F mutation whose equivalent in Shaker channels (T449E/K/D/Q/S or W434F) caused a greatly accelerated rate of C-type inactivation or constitutive C-inactivation. C-type inactivation in most K+ channels occurs upon sustained membrane depolarization or channel opening and then recovers during hyperpolarized membrane potentials or channel closure. However, we found that the BK channel C-type inactivation occurred during hyperpolarized membrane potentials or with decreased intracellular calcium ([Ca2+]i) and recovered with depolarized membrane potentials or elevated [Ca2+]i. Constitutively open mutation prevented BK channels from C-type inactivation. We concluded that BK channel C-type inactivation is closed state-dependent and that its extents and rates inversely correlate with channel-open probability. Because C-type inactivation can involve multiple conformational changes at the selectivity filter, we propose that the BK channel’s normal closing may represent an early conformational stage of C-type inactivation.

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Probing the Structural Dynamics of the Activation Gate of KcsA Using Homo-FRET Measurements

International Journal of Molecular Sciences ◽

10.3390/ijms222111954 ◽

2021 ◽

Vol 22 (21) ◽

pp. 11954

Author(s):

Clara Díaz-García ◽

Maria Lourdes Renart ◽

José Antonio Poveda ◽

Ana Marcela Giudici ◽

José M. González-Ros ◽

...

Keyword(s):

Conformational Changes ◽

Conformational Dynamics ◽

Resonance Energy Transfer ◽

Resonance Energy ◽

Time Resolved ◽

Allosteric Coupling ◽

Allosteric Communication ◽

Activation Gate ◽

Fret Efficiency ◽

High Degree

The allosteric coupling between activation and inactivation processes is a common feature observed in K+ channels. Particularly, in the prokaryotic KcsA channel the K+ conduction process is controlled by the inner gate, which is activated by acidic pH, and by the selectivity filter (SF) or outer gate, which can adopt non-conductive or conductive states. In a previous study, a single tryptophan mutant channel (W67 KcsA) enabled us to investigate the SF dynamics using time-resolved homo-Förster Resonance Energy Transfer (homo-FRET) measurements. Here, the conformational changes of both gates were simultaneously monitored after labelling the G116C position with tetramethylrhodamine (TMR) within a W67 KcsA background. At a high degree of protein labeling, fluorescence anisotropy measurements showed that the pH-induced KcsA gating elicited a variation in the homo-FRET efficiency among the conjugated TMR dyes (TMR homo-FRET), while the conformation of the SF was simultaneously tracked (W67 homo-FRET). The dependence of the activation pKa of the inner gate with the ion occupancy of the SF unequivocally confirmed the allosteric communication between the two gates of KcsA. This simple TMR homo-FRET based ratiometric assay can be easily extended to study the conformational dynamics associated with the gating of other ion channels and their modulation.

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Gating of two-pore domain K+ channels by extracellular pH

Biochemical Society Transactions ◽

10.1042/bst0340899 ◽

2006 ◽

Vol 34 (5) ◽

pp. 899-902 ◽

Cited By ~ 13

Author(s):

M.I. Niemeyer ◽

F.D. González-Nilo ◽

L. Zúñiga ◽

W. González ◽

L.P. Cid ◽

...

Keyword(s):

Extracellular Ph ◽

Selectivity Filter ◽

Open Probability ◽

K Channels ◽

Task Channels ◽

Pore Mouth ◽

Inactivation Gating ◽

Opening And Closing ◽

Pore Domain ◽

And Task

Potassium channels have a conserved selectivity filter that is important in determining which ions are conducted and at what rate. Although K+ channels of different conductance characteristics are known, they differ more widely in the way their opening and closing, the gating, is governed. TASK and TALK subfamily proteins are two-pore region KCNK K+ channels gated open by extracellular pH. We discuss the mechanism for this gating in terms of electrostatic effects on the pore changing the occupancy and open probability of the channels in a way reminiscent of C-type inactivation gating at the selectivity filter. Essential to this proposed mechanism is the replacement of two highly conserved aspartate residues at the pore mouth by asparagine or histidine residues in the TALK and TASK channels.

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Structural basis of ion permeation gating in Slo2.1 K+ channels

The Journal of General Physiology ◽

10.1085/jgp.201311064 ◽

2013 ◽

Vol 142 (5) ◽

pp. 523-542 ◽

Cited By ~ 16

Author(s):

Priyanka Garg ◽

Alison Gardner ◽

Vivek Garg ◽

Michael C. Sanguinetti

Keyword(s):

Selectivity Filter ◽

Structural Basis ◽

K Channel ◽

Xenopus Laevis Oocytes ◽

Ion Permeation ◽

Channel Activation ◽

K Channels ◽

Voltage Gated ◽

Channel Function ◽

Activation Gate

The activation gate of ion channels controls the transmembrane flux of permeant ions. In voltage-gated K+ channels, the aperture formed by the S6 bundle crossing can widen to open or narrow to close the ion permeation pathway, whereas the selectivity filter gates ion flux in cyclic-nucleotide gated (CNG) and Slo1 channels. Here we explore the structural basis of the activation gate for Slo2.1, a weakly voltage-dependent K+ channel that is activated by intracellular Na+ and Cl−. Slo2.1 channels were heterologously expressed in Xenopus laevis oocytes and activated by elevated [NaCl]i or extracellular application of niflumic acid. In contrast to other voltage-gated channels, Slo2.1 was blocked by verapamil in an activation-independent manner, implying that the S6 bundle crossing does not gate the access of verapamil to its central cavity binding site. The structural basis of Slo2.1 activation was probed by Ala scanning mutagenesis of the S6 segment and by mutation of selected residues in the pore helix and S5 segment. Mutation to Ala of three S6 residues caused reduced trafficking of channels to the cell surface and partial (K256A, I263A, Q273A) or complete loss (E275A) of channel function. P271A Slo2.1 channels trafficked normally, but were nonfunctional. Further mutagenesis and intragenic rescue by second site mutations suggest that Pro271 and Glu275 maintain the inner pore in an open configuration by preventing formation of a tight S6 bundle crossing. Mutation of several residues in S6 and S5 predicted by homology modeling to contact residues in the pore helix induced a gain of channel function. Substitution of the pore helix residue Phe240 with polar residues induced constitutive channel activation. Together these findings suggest that (1) the selectivity filter and not the bundle crossing gates ion permeation and (2) dynamic coupling between the pore helix and the S5 and S6 segments mediates Slo2.1 channel activation.

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Rapid constriction of the selectivity filter underlies C-type inactivation in the KcsA potassium channel

The Journal of General Physiology ◽

10.1085/jgp.201812082 ◽

2018 ◽

Vol 150 (10) ◽

pp. 1408-1420 ◽

Cited By ~ 27

Author(s):

Jing Li ◽

Jared Ostmeyer ◽

Luis G. Cuello ◽

Eduardo Perozo ◽

Benoît Roux

Keyword(s):

Ionic Conduction ◽

Md Simulations ◽

Umbrella Sampling ◽

Potential Of Mean Force ◽

Selectivity Filter ◽

Truncated Form ◽

Terminal Domain ◽

Activation Gate ◽

Electrophysiological Measurements ◽

Inactivation Gating

C-type inactivation is a time-dependent process observed in many K+ channels whereby prolonged activation by an external stimulus leads to a reduction in ionic conduction. While C-type inactivation is thought to be a result of a constriction of the selectivity filter, the local dynamics of the process remain elusive. Here, we use molecular dynamics (MD) simulations of the KcsA channel to elucidate the nature of kinetically delayed activation/inactivation gating coupling. Microsecond-scale MD simulations based on the truncated form of the KcsA channel (C-terminal domain deleted) provide a first glimpse of the onset of C-type inactivation. We observe over multiple trajectories that the selectivity filter consistently undergoes a spontaneous and rapid (within 1–2 µs) transition to a constricted conformation when the intracellular activation gate is fully open, but remains in the conductive conformation when the activation gate is closed or partially open. Multidimensional umbrella sampling potential of mean force calculations and nonequilibrium voltage-driven simulations further confirm these observations. Electrophysiological measurements show that the truncated form of the KcsA channel inactivates faster and greater than full-length KcsA, which is consistent with truncated KcsA opening to a greater degree because of the absence of the C-terminal domain restraint. Together, these results imply that the observed kinetics underlying activation/inactivation gating reflect a rapid conductive-to-constricted transition of the selectivity filter that is allosterically controlled by the slow opening of the intracellular gate.

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Probing Allosteric Coupling of a Constitutively Open Mutant of the Ion Channel KcsA using Solid State NMR

10.1101/567024 ◽

2019 ◽

Author(s):

Zhiyu Sun ◽

Yunyao Xu ◽

Dongyu Zhang ◽

Ann E McDermott

Keyword(s):

Solid State ◽

Binding Affinity ◽

Solid State Nmr ◽

Selectivity Filter ◽

Wild Type ◽

Allosteric Coupling ◽

Channel Inactivation ◽

Activation Gate ◽

Inactivation Process ◽

Potassium Binding

AbstractTransmembrane allosteric coupling is a feature of many critical biological signaling events. Here we test whether transmembrane allosteric coupling controls the mean open time of the prototypical potassium channel KcsA in the context of C-type inactivation. Activation of KcsA is initiated by proton binding to the pH gate upon an intracellular drop in pH. Numerous studies have suggested that this proton binding also prompts a conformational switch leading to a loss of affinity for potassium ions at the selectivity filter and therefore to channel inactivation. We tested this mechanism for inactivation using a KcsA mutant (H25R/E118A) that has the pH gate open across a broad range of pH values. We present solid-state NMR measurements of this open mutant at neutral pH to probe the affinity for potassium at the selectivity filter. The potassium binding affinity in the selectivity filter of this mutant, 81 mM, is about 4 orders of magnitude weaker than that of wild type KcsA at neutral pH and is comparable to the value for wild type KcsA at low pH (pH ∼ 3.5). This result strongly supports our assertion that the open pH gate allosterically effects the potassium binding affinity of the selectivity filter. In this mutant the protonation state of a glutamate residue (E120) in the pH sensor is sensitive to potassium binding, suggesting that this mutant also has flexibility in the activation gate and is subject to transmembrane allostery.Significance statementInactivation of potassium channels controls mean open times and provides exquisite control over biological processes. In the highly conserved C-type inactivation process, opening of the activation gate causes subsequent inactivation. We test whether the open state of the channel simply has a poor ability to bind the K+ ion. Previously, activated and inactivated states were stabilized using truncations or a significant pH drop. Here, we use the H25R/E118A constitutively open mutant of KcsA and also observe a large drop in potassium binding affinity. This provides strong evidence that channel opening causes an allosteric loss of ion affinity, and that the central feature of this universal channel inactivation process is loss of ion affinity at the selectivity filter.

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Voltage-dependent inactivation gating at the selectivity filter of the MthK K+ channel

The Journal of General Physiology ◽

10.1085/jgp.201010507 ◽

2010 ◽

Vol 136 (5) ◽

pp. 569-579 ◽

Cited By ~ 25

Author(s):

Andrew S. Thomson ◽

Brad S. Rothberg

Keyword(s):

Voltage Sensor ◽

Selectivity Filter ◽

K Channel ◽

K Channels ◽

Dependent Inactivation ◽

Wide Range ◽

Voltage Dependent ◽

Inactivation Gating ◽

External K ◽

Conductive State

Voltage-dependent K+ channels can undergo a gating process known as C-type inactivation, which involves entry into a nonconducting state through conformational changes near the channel’s selectivity filter. C-type inactivation may involve movements of transmembrane voltage sensor domains, although the mechanisms underlying this form of inactivation may be heterogeneous and are often unclear. Here, we report on a form of voltage-dependent inactivation gating observed in MthK, a prokaryotic K+ channel that lacks a canonical voltage sensor and may thus provide a reduced system to inform on mechanism. In single-channel recordings, we observe that Po decreases with depolarization, with a half-maximal voltage of 96 ± 3 mV. This gating is kinetically distinct from blockade by internal Ca2+ or Ba2+, suggesting that it may arise from an intrinsic inactivation mechanism. Inactivation gating was shifted toward more positive voltages by increasing external [K+] (47 mV per 10-fold increase in [K+]), suggesting that K+ binding at the extracellular side of the channel stabilizes the open-conductive state. The open-conductive state was stabilized by other external cations, and selectivity of the stabilizing site followed the sequence: K+ ≈ Rb+ > Cs+ > Na+ > Li+ ≈ NMG+. Selectivity of the stabilizing site is weaker than that of sites that determine permeability of these ions, suggesting that the site may lie toward the external end of the MthK selectivity filter. We could describe MthK gating over a wide range of positive voltages and external [K+] using kinetic schemes in which the open-conductive state is stabilized by K+ binding to a site that is not deep within the electric field, with the voltage dependence of inactivation arising from both voltage-dependent K+ dissociation and transitions between nonconducting (inactivated) states. These results provide a quantitative working hypothesis for voltage-dependent, K+-sensitive inactivation gating, a property that may be common to other K+ channels.

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Localization of the Activation Gate of a Voltage-gated Ca2+ Channel

The Journal of General Physiology ◽

10.1085/jgp.200509293 ◽

2005 ◽

Vol 126 (3) ◽

pp. 205-212 ◽

Cited By ~ 25

Author(s):

Cheng Xie ◽

Xiao-guang Zhen ◽

Jian Yang

Keyword(s):

State Dependence ◽

K Channels ◽

Voltage Gated ◽

Closed State ◽

State Dependent ◽

Transmembrane Voltage ◽

Activation Gate ◽

Pore Lining ◽

Ca2 Channels ◽

Α1 Subunit

Ion channels open and close in response to changes in transmembrane voltage or ligand concentration. Recent studies show that K+ channels possess two gates, one at the intracellular end of the pore and the other at the selectivity filter. In this study we determined the location of the activation gate in a voltage-gated Ca2+ channel (VGCC) by examining the open/closed state dependence of the rate of modification by intracellular methanethiosulfonate ethyltrimethylammonium (MTSET) of pore-lining cysteines engineered in the S6 segments of the α1 subunit of P/Q type Ca2+ channels. We found that positions above the putative membrane/cytoplasm interface, including two positions below the corresponding S6 bundle crossing in K+ channels, showed pronounced state-dependent accessibility to internal MTSET, reacting ∼1,000-fold faster with MTSET in the open state than in the closed state. In contrast, a position at or below the putative membrane/cytoplasm interface was modified equally rapidly in both the open and closed states. Our results suggest that the S6 helices of the α1 subunit of VGCCs undergo conformation changes during gating and the activation gate is located at the intracellular end of the pore.

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