Effects of Kv1.2 Intracellular Regions on Activation of Kv2.1 Channels

doi:10.1529/biophysj.104.040550

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Effects of Kv1.2 Intracellular Regions on Activation of Kv2.1 Channels

Annette Scholle^*, Thomas Zimmer^*, Rolf Koopmann^*, Birgit Engeland, Olaf Pongs and Klaus Benndorf^*

^* Institut für Physiologie II, Friedrich-Schiller-Universität, 07740 Jena, Germany; and Zentrum für Molekulare Neurobiologie, Institut für Neurale Signalverarbeitung, UKE Hamburg, 20251 Hamburg, Germany

Correspondence: Address reprint requests to Dr. Klaus Benndorf, Institut für Physiologie II, Friedrich-Schiller-Universität Jena, D-07740 Jena, Germany. Tel.: 49-3641-934351; Fax: 49-3641-933202; E-mail: klaus.Benndorf{at}mti.uni-jena.de.

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

Depolarizing voltage steps activate voltage-dependent K⁺ (Kv)channels by moving the voltage sensor, which triggers a couplingreaction leading to the opening of the pore. We constructedchimeric channels in which intracellular regions of slowly activatingKv2.1 channels were replaced by respective regions of rapidlyactivating Kv1.2 channels. Substitution of either the N-terminus,S4–S5 linker, or C-terminus generated chimeric Kv2.1/1.2channels with a paradoxically slow and approximately exponentialactivation time course consisting of a fast and a slow component.Using combined chimeras, each of these Kv1.2 regions furtherslowed activation at the voltage of 0 mV, irrespective of thenature of the other two regions, whereas at the voltage of 40mV both slowing and accelerating effects were observed. Theseresults suggest voltage-dependent interactions of the threeintracellular regions. This observation was quantified by double-mutantcycle analysis. It is concluded that interactions between N-terminus,S4–S5 linker, and/or C-terminus modulate the activationtime course of Kv2.1 channels and that part of these interactionsis voltage dependent.

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

Voltage-gated K⁺ channels (Kv channels) are formed by tetramersof ${alpha}$ -subunits (MacKinnon, 1991; Heginbotham and MacKinnon, 1992;Liman et al., 1992) and each subunit was proposed to containsix transmembrane helices (S1–S6; for review see Yellen,2002). Segments S5–S6 contribute to the pore and the selectivityfilter of the channel, whereas segments S1–S4 make upthe voltage sensor. Tetramerization specificity of the subunitsis mainly controlled by a highly conserved and subfamily-specificdomain in the N-terminus close to the S1 segment (Li et al.,1992; Sheng et al., 1993). The activation of Kv channels iscontrolled by the membrane voltage, which imposes an electricfield across the membrane controlling the position of gatingcharges in the voltage sensor. The S4 segment has been identifiedas a major element of the voltage sensor (Liman et al., 1991;Papazian et al., 1991; Logothetis et al., 1992; Perozo et al.,1994; Larsson et al., 1996; Yusaf et al., 1996; Starace et al.,1997; Cha and Bezanilla, 1997). The S2 and S3 segments alsocontribute to the voltage sensor (Papazian et al., 1995; Planells-Caseset al., 1995; Seoh et al., 1996; Tiwari-Woodruff et al., 1997;Cha and Bezanilla, 1997; Milligan and Wray, 2000). Recently,the first crystal structure of a voltage-gated K⁺ channel, thebacterial KvAP channel, has been reported (Jiang et al., 2003a)and the authors also suggest a contribution of these three segmentsto the voltage sensor (Jiang et al., 2003b).

The coupling reaction, which transmits movements of the voltagesensor to pore opening, is not well understood. Structure-functionstudies have implicated the S3–S4 linker (Mathur et al.,1997), the S4–S5 linker (McCormack et al., 1991; Shiehet al., 1997; Lu et al., 2002), and/or the inner part of thepore-lining S6 segment (del Camino and Yellen, 2001). Otherexperimental results show that also the intracellularly locatedtermini modulate activation; mutations in the N-terminal tetramerizationdomain modulate both steady-state activation and activationkinetics in Kv1 channels (Minor et al., 2000; Cushman et al.,2000) and Kv2 channels (VanDongen et al., 1990; Chiara et al.,1999). VanDongen et al. (1990) also showed a modulatory effectof the C-terminus on Kv2.1 channels and, in a recent study,Ju and co-workers (2003) identified the residues 67 and 75 inthe Kv2.1 N-terminus and a domain in the C-terminus (residues741–853) to be involved in determining Kv2.1 activationkinetics. Moreover, Ju and co-workers (2003) presented evidencethat the N-terminal Kv2.1 residues interact with the C-terminaldomain.

We showed previously that Kv1.2 channels activate three timesfaster than Kv2.1 channels (Scholle et al., 2000). During theseinvestigations we noticed a paradoxical slowing of activationwhen the S4–S5 linker in Kv2.1 channels was replaced bythe one of Kv1.2. Apparently, the presence of the Kv1.2 S4–S5linker in Kv2.1 channels slowed Kv2.1 channel activation evenfurther. It may therefore be hypothesized that replacement ofthe Kv2.1 S4–S5 linker by the one of Kv1.2 disturbs aconcerted interaction between the S4–S5 linker and otherparts of the Kv2.1 channel, as, e.g., the N- or C-terminus.

To identify such interactions, we systematically replaced thesethree regions of Kv2.1 channels by respective regions of Kv1.2channels and analyzed both steady-state activation and the activationtime course. We present evidence that each of the Kv1.2 regionsconfers pronounced slowing of activation, that the slowing dependson voltage, and that the regions interact. The strength of theseinteractions is energetically characterized by means of double-mutantcycle analysis.

MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

In vitro mutagenesis
Chimeric cDNAs for Ch_N, Ch_L4/5, and Ch_C were obtained byoverlap PCR (PCR; Ho et al., 1989). cDNAs were cloned into thepGEM-HE vector for RNA synthesis (Liman et al., 1992). Suitablerestriction sites in the Kv2.1 sequence of Ch-N, Ch_L4/5, andCh_C were used to obtain Ch_NL4/5 (Bsp 120I), Ch_NC (Bsp 120I),Ch_L4/5C (SapI), and Ch_NL4/5C (Bsp 120I).

Table 1 illustrates names and splice sites of all chimeras used.Based on the fact that only the N-terminus (N), S4–S5linker (L4/5), and C-terminus (C) of Kv1.2 were transferredto Kv2.1, the names of the chimeras (Ch_) were specified byindicating the sequence of these transferred regions in thedirection from the N-terminus to the C-terminus. For example,"Ch_NL4/5" means that the chimera contains the N-terminus andthe S4–S5 linker from Kv1.2 (1.2) in a Kv2.1 (2.1) background.

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TABLE 1 Structure of the Kv2.1/Kv1.2 chimeras

Expression in oocytes
Ovarian lobes from Xenopus laevis were resected under anesthesia(0.4% 3-aminobenzoic acid ethyl ester) and transferred to aPetri dish containing Ca²⁺-free Barth medium (84 mM NaCl, 1mM KCl, 2.4 mM NaHCO₃, 0.82 mM MgSO₄, 7.5 mM Tris, pH = 7.4with HCl). The oocytes were incubated in Ca²⁺-free Barth mediumcontaining 1.2 mg/ml collagenase (type CLSII, Biochrom KG, Berlin,Germany) for 1–2 h. After washing repeatedly with Barthmedium containing in addition 0.33 mM Ca(NO₃)₂, 0.41 mM CaCl₂,4 µg/ml cefuroxim, 50 units/ml penicillin, 50 µg/mlstreptomycin, and 100 µg/ml neomycin, the oocytes wereisolated and defolliculated mechanically. Within 6 h after isolationthe oocytes were injected with $~$ 50 nl cRNA solution. The cRNAconcentration was varied for control of the expression level.The oocytes were incubated at 18°C in Barth medium untilexperimental use within 3 days after injection.

Electrophysiology
Ionic currents were recorded with the two-microelectrode voltageclamp technique (OC725C amplifier, Warner Instrument, Hampden,CT) at room temperature. The microelectrodes were filled with3 M KCl and had a resistance of 0.3–0.7 M ${Omega}$ . The experimentswere performed in modified Barth medium containing 5 mM KCland 80 mM NaCl instead of 1 and 84 mM, respectively. The experimentswere controlled with a personal computer and the ISO2 software(MFK, Niedernhausen, Germany). The holding potential was generally–80 mV. Ionic currents were measured with pulses between–20 and 60 mV spaced 10 mV. Because the activation kineticsamong the chimeras differed by orders of magnitude, both pulseand interpulse duration were appropriately adapted to the activationtime course with the criterion that the ionic currents werefully activated. Used pulse durations were 0.5, 1, 2, 5, 15,and 30 s and the corresponding interpulse times were 2, 2, 5,10, 30, and 60 s. Small linear leakages were removed by subtractingscaled average traces to subthreshold potentials between –70and –40 mV.

Steady-state activation was determined as described previouslyfrom the amplitude of instantaneous currents at 0 mV after depolarizingpulses to variable potentials between –40 and 60 mV (cf.Scholle et al., 2000). The relative amplitude of the tail current,I_rel, was determined from the amplitude ratio of the instantaneouscurrent at the actual potential with respect to the instantaneouscurrent after maximal depolarization. This relationship wasplotted as function of voltage and fitted by the Boltzmann functionwith power 1

(1)
yielding the midpointvoltage V_1/2 of half-maximum activation and the equivalent gatingcharge z. R is the molar gas constant, T the absolute temperaturein Kelvin (K), and F the Faraday constant.

Fitting and statistics
The data were fitted with various functions using the ${chi}$ ²-methodof the Origin 6.1 software (OriginLab, Northampton, MA) or theroutines implemented in the ISO2 software. Statistical dataare presented as means ± SE and errors were calculatedaccording to the error propagation law. Statistical significancewas tested with the Student's t-test (P < 0.05).

RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

Kv1.2 N-terminus, S4–S5 linker, and C-terminus slow the activation time course of Kv2.1
We first investigated effects of a replacement of Kv2.1 N-terminus,S4–S5 linker, or C-terminus by the ones of Kv1.2 on theactivation rate of Kv2.1 channels (chimeras Ch_N, Ch_L4/5, Ch_C).None of the cytosolic Kv1.2 regions transferred the typicalfaster activation rate of Kv1.2 channels to Kv2.1 channels.Instead, the three chimeric channels exhibited a considerablyslowed activation rate (Fig. 1 A). In contrast to the pronouncedsigmoidal activation of wild-type channels, those of the chimeraswere dominated by an approximately exponential time course.This is demonstrated in Fig. 1 B where the normalized activationtime courses are compared by adjusting their timescales to makethe rate of rise at the half-maximum current equal (c.f. Zagottaet al., 1994a). The predominant exponential activation in thechimeras suggests that the slowing was caused only in a concertedreaction after the independent gating of the subunits (c.f.Zagotta et al., 1994a).

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FIGURE 1 Activation rate of the ionic current in chimeric channels constructed by inserting either the N-terminus (Ch_N), the S4–S5 linker (Ch_L4/5), or the C-terminus (Ch_C) from Kv1.2 in Kv2.1 channels. (A) Representative current traces at +20 mV. The current amplitude was normalized with respect to that of the steady-state current, which is not reached by the chimeras in the time window shown. The arrows indicate the time intervals, t_a,1/2, between clamp step and half-maximum current (dashed line). (B) Sigmoidicity for Kv2.1 channels and the three chimeras. The sigmoidicity can be defined as the amount of delay relative to the overall rate of activation. The normalized currents were adjusted in their timescales to make the rate of rise at the half-maximum current (dashed line) equal (short lines). (C) Plot of t_a,1/2 as function of voltage. The slowing effects of the transferred intracellular regions showed different voltage dependencies. Here and in the other figures, the numbers of oocytes included are shown in parentheses to the right of the names and the error is indicated by SEM.

Plotting the time interval between the depolarizing clamp stepand the half-maximum current, t_a,1/2, as function of voltage(Fig. 1 C) yielded the following results: The Kv1.2 N-terminusslowed activation of Kv2.1 channels at 0 mV but not at 40 mV,the Kv1.2 C-terminus slowed activation at all voltages by asimilar factor, and the Kv1.2 S4–S5 linker slowed activationat 0 mV more markedly than the Kv1.2 N- or C-terminus whereasat 40 mV the slowing effect was small.

Evaluation of the activation speed by t_a,1/2, however, doesnot reflect all differences of the activation time courses betweenthe chimeras. We therefore determined a mean activation timeconstant for the exponential activation time course after therelatively short initial delay: We first fitted the activationtime course between the inflection point and the end of thedepolarizing pulse with the sum of two exponential componentsaccording to

(2)

A₁, A₂, ${tau}$ ₁, ${tau}$ ₂ are the amplitude and the time constant of thefast and slow exponential, respectively. The relative weightof the fast exponential (A_1,rel = A₁/(A₁ + A₂)) ranged from19 to 61% and the time constants for an individual current tracediffered by less than factor 9. The mean activation time constant ${tau}$ _m was then calculated as the weighted mean of ${tau}$ ₁ and ${tau}$ ₂. In contrastto t_a,1/2, ${tau}$ _m also adequately reflects slow exponential termsof small amplitude. The great benefit of a single parameterdescribing the activation speed is that it allows a direct evaluationof the degree of slowing conferred by the individual Kv1.2 segments.

In the following analysis we also included double chimeras (Ch_NL4/5,Ch_L4/5C, Ch_NC; Table 1) and the triple chimera (Ch_NL4/5C;Table 1). The results showed that cumulative replacement ofKv2.1 regions by the ones of Kv1.2 further enhanced the slowingof current activation, as shown for three related chimeras inFig. 2. To analyze the slowing effects of the Kv1.2 regionssystematically, log( ${tau}$ _m) was plotted as function of voltage (Fig. 3).To the right and left of the log( ${tau}$ _m)-voltage relationship,the effects of the Kv1.2 N-terminus, S4–S5 linker, and/orC-terminus on log( ${tau}$ _m) are schematically illustrated by arrowsfor each combination of the intracellular regions. At 0 mV,log( ${tau}$ _m) increased in four steps with the number of intracellularKv2.1 regions replaced by the ones of Kv1.2: < either terminusalone < both termini or the S4–S5 linker < S4–S5linker plus one of the termini < S4–S5 linker plusboth termini. Considering the effects of the intracellular Kv1.2regions with each combination of the other intracellular regions,the results show that the effects are approximately additive(arrows). At 40 mV, we found a different situation; replacementof the N-terminus (Ch_N) had no effect on log( ${tau}$ _m) whereas replacementof the C-terminus (Ch_C) exerted nearly the maximum slowingeffect, developed by the chimeras Ch_C, Ch_NL4/5C, and Ch_NL4/5.Thus, the approximate additivity for log( ${tau}$ _m) observed at 0 mVwas not seen at 40 mV; the Kv1.2 N-terminus and C-terminus producedeither an increase of log( ${tau}$ _m) or no effect whereas the S4–S5linker generated either an increase or, in one case, a decreaseof log( ${tau}$ _m). The results suggest that at 0 mV the effects of Kv1.2intracellular regions on the activation time course are largelyindependent of the nature of the other two regions. In contrast,specific interactions between particular intracellular regionsmay exist at 40 mV.

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FIGURE 2 Exponential description of representative currents of Kv2.1 channels, the chimera with substituted Kv1.2 C terminus (Ch_C), with substituted Kv1.2 C-terminus and N-terminus (Ch_NC), and with substituted Kv1.2 C-terminus, S4–S5 linker, and N-terminus (Ch_NL4/5C). Representative currents were fitted between the time of the inflection point (arrows) and the end of the depolarizing pulse with two exponentials by Eq. 2. Indicated are the resulting fast and slow time constant, ${tau}$ ₁ and ${tau}$ ₂, and the relative weight of the exponential terms, A_1,rel = A₁/(A₁ + A₂) and A_2,rel = A₂/(A₁ + A₂), respectively. The fitted curves are superimposed to the currents. The mean time constant, ${tau}$ _m, is the weighted mean of ${tau}$ ₁ and ${tau}$ ₂. Each additional intracellular Kv1.2 region further increased ${tau}$ _m. Test pulse voltage 20 mV.

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FIGURE 3 Plot of the mean time constant of activation, ${tau}$ _m, as function of voltage. The groups of four arrows to the left and right of the diagram specify the effects of either the N-terminus, the S4–S5 linker, or the C-terminus (indicated below the parentheses) on the time constants at 0 and 40 mV with each combination of the other two regions, respectively. Black rectangles instead of arrows indicate the absence of an effect. Below each arrow/rectangle, the individual reference for a specific effect is indicated. For example, "-", "45", or "45C" means that either Kv2.1 channels, chimera "Ch_C", or chimera Ch_L4/5C were the reference.

Effects of the intracellular Kv1.2 regions on the rate constants of activation and deactivation of Kv2.1
The slow and exponential activation time course of the chimerasstrongly suggests that only a concerted reaction after the independentgating of the subunits can be slowed. This can either be thereaction coupling the voltage-sensor movement to the pore openingor the pore opening itself. The following simple kinetic modelwas used to obtain a semiquantitative measure of the effectsof the mutations (Li-Smerin et al., 2000

; Yifrach and MacKinnon,2002

)

Scheme 1

C and O are the closed and open state, k₁ and k₂ the respectiveforward and backward rate constants. From Scheme 1 it followsthat ${tau}$ _m equals the relaxation time constant, 1/(k₁+ k₂). We assumedthat the mean time constant ${tau}$ _m, calculated as weighted mean ofthe fast and the slow time constant ${tau}$ ₁ and ${tau}$ ₂, respectively, describesthe activation time course as a first approximation.

The rate constants k₁ and k₂ at 0 and 40 mV were determinedby

(3a)

(3b)

(3c)

(3d)

P_o,0 and P_o,40 are the open probabilities at 0 and 40 mV, respectively.As estimates for P_o we used the I_rel values at the respectivevoltage calculated with Eq. 1. It is evident that k_2,0 for theactivation of the chimeras is relatively invariant and smallerthan for Kv2.1 channels (Fig. 4). Also k_1,0 is smaller for thechimeras than for Kv2.1 channels. In contrast to k_2,0, however,the decrease in k_1,0 is markedly smaller for Ch_N and Ch_C thanfor the other chimeras. Only in Kv2.1 channels and in Ch_C depolarizationto 40 mV generates larger deceleration in k₂ than accelerationin k₁ whereas in all other chimeras k₁ is more accelerated thank₂ is decelerated.

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FIGURE 4 Rate constants k₁ and k₂ for all chimeras at 0 and 40 mV according to Scheme 1.

Interaction energy of intracellular Kv1.2 regions associated with the activation kinetics
Interaction of substituted intracellular regions associatedwith activation-induced changes of the rate constants k₁ andk₂ was estimated by calculating free-energy differences. Accordingto the absolute reaction rate theory of Eyring (Glasstone etal., 1941

), a rate constant k_x is related to the free-energydifference, ${Delta}$ G_kx, between a transition state and the ground stateby

(4)
where k and h are the Boltzmannand the Planck constant, respectively. ${Delta}$ G_kx was calculated forboth k₁ and k₂ at both 0 and 40 mV. Following the principlesof thermodynamic double-mutant cycle analysis (for reviews seeWells, 1990; Mildvan et al., 1992; Horovitz, 1996), a double-mutantcycle consists of a wild-type protein, two single mutants, andthe corresponding double mutant. In this study, a substitutedintracellular Kv1.2 region is considered a "mutation" and interactionrefers to the sum of interactions between the two regions. Ifthe respective difference of the free energy between the doublechimera with replaced regions A and B and the chimera with replacedregion B ( ${Delta}$ G_AB – ${Delta}$ G_B) differs from that between the chimerawith replaced region A and the Kv2.1 channel ( ${Delta}$ G_A – ${Delta}$ G_2.1),then the two regions A and B interact with the respective interactionenergy ${Delta}$ ${Delta}$ G_Interaction = ${Delta}$ G_AB – ${Delta}$ G_B – ( ${Delta}$ G_A – ${Delta}$ G_2.1).For example, the double-mutant cycle for Kv2.1, Ch_N, Ch_C,and Ch_NC is

Scheme 2
and the interaction energy between the N- and C-terminus is ${Delta}$ ${Delta}$ G_Interaction = ${Delta}$ G_NC – ${Delta}$ G_C – ( ${Delta}$ G_N – ${Delta}$ G_2.1) = ${Delta}$ G_NC– ${Delta}$ G_N – ( ${Delta}$ G_C – ${Delta}$ G_2.1). It should be emphasizedthat ${Delta}$ ${Delta}$ G_Interaction is not the interaction energy between theN- and C-terminus per se, but only the change of interactionenergy associated with activation. Because the above considerationshold for the mutant cycle consisting of the triple chimera,two double chimeras, and the single chimera whose substitutionis also present in both double chimeras, our results also allowus to estimate the effect of the third region on the interactionenergy of the other two regions. In the following, interactionbetween two intracellular regions will be termed "interaction"solely.

First the interaction energies for k₁ are considered (Fig. 5top). At 0 mV and with the Kv2.1 sequence in the third region,there is strong positive interaction energy only for the interactionof the N- and C-terminus. The interaction energy is enhancedat 40 mV. In the presence of the Kv1.2 S4–S5 linker thisinteraction is cancelled (top right; N/C). In the presence ofthe respective other Kv1.2 terminus, the S4–S5 linkerproduces negative interaction energy with either the N- or theC-terminus (top right; L45/C; N/L45). However, only the interactionwith the N-terminus is noticeably voltage dependent.

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FIGURE 5 Interaction energy ( ${Delta}$ ${Delta}$ G_interaction) between mutated Kv1.2 regions in a Kv2.1 background for the change of the forward and backward rate constants of activation, k₁ and k₂, according to Scheme 1. The activation time course was quantified with a single time constant ${tau}$ _m and the values for ${Delta}$ ${Delta}$ G_Interaction were calculated as described in the text. N/C, L45/C, and N/L45 indicate the interaction of N- with C-terminus, S4–S5 linker with C-terminus, and N-terminus with S4–S5 linker, respectively.

Consider now the interaction energies for k₂ (Fig. 5 bottom).With the Kv2.1 sequence in the third region, the interactionenergies are strongly negative at both 0 and 40 mV, except forthe interaction of the S4–S5 linker and the C-terminusat 40 mV, which approximates zero. In the presence of the respectivethird Kv1.2 region, the interaction energy becomes mostly positiveand depolarization further increases the interaction energiesbetween both termini as well as between the C-terminus and theS4–S5 linker. In general, the interaction energies fortwo or three regions substituted, differ markedly less at 0mV than at 40 mV. This result indicates that interactions betweenthe intracellular regions are voltage dependent.

Influence of Kv1.2 N-terminus, S4–S5 linker, and C-terminus on Kv2.1 steady-state activation
To test whether shifts of steady-state activation along thevoltage axis are responsible for the dramatic slowing of activation,steady-state activation was measured and quantified by fittinga Boltzmann function with power 1, yielding the parameters V_1/2and z (see Materials and Methods). The V_1/2 values of the twosingle chimeras, Ch_N and Ch_C, were by 9.4 and 5.5 mV, respectively,more negative whereas those of all other chimeras were by 6.8–14.8mV more positive than for Kv2.1 channels. These shifts are muchtoo small to explain the great slowing of activation describedabove. Interestingly, the equivalent gating charge z was smallestin Kv2.1 channels.

We also quantified the effects of the three regions on steady-stateactivation with each combination of the other two intracellularregions in terms of a difference of the free-energy difference, ${Delta}$ ${Delta}$ G, calculated from the V_1/2 values according to Li-Smerin etal. (2000)

(5)

V_1/2,act, V_1/2,ref, z_act, and z_ref are the actual and referencevalues of V_1/2 and z. Negative values of ${Delta}$ ${Delta}$ G are caused by leftwardshifts in steady-state activation and/or larger z_act and indicatethat the inserted Kv1.2 region has caused a relative stabilizationof the open state over the closed state. The boxes in Fig. 6illustrate the chimeras in the form of cartoons, specifyingthe origin of the N-terminus, the S4–S5 linker, and theC-terminus. The bar graphs below the brackets indicate the effectsof the three regions on ${Delta}$ ${Delta}$ G with each combination of the othertwo intracellular regions. In each group of four bars, the left-mostbar indicates the effect with respect to the pure Kv2.1 background,the two bars in the middle indicate the effect with one Kv1.2region already present, and the right-most bar indicates theeffect with already two Kv1.2 regions present.

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FIGURE 6 Steady-state parameters of Kv2.1 channels and the seven single and combined chimeras containing intracellular Kv1.2 regions. The V_1/2 and z values were determined with Eq. 1 (see Materials and Methods). The reduced cartoons indicate the origin of N-terminus, S4–S5 linker, and C-terminus by either open (Kv2.1) or solid (Kv1.2) boxes. The brackets to the right of the reduced cartoons indicate an effect of one of the intracellular Kv1.2 regions on steady-state properties of activation at a specific combination of the other intracellular regions. The effects on V_1/2 are indicated as differences of the free-energy difference ${Delta}$ ${Delta}$ G (Eq. 5) in the bar graph below the brackets. The effects on the equivalent gating charge z are shown as ${Delta}$ z in the lower bar graph. For further explanation see text.

The following results can be derived: The N- and the C-terminusgenerated a similar profile of ${Delta}$ ${Delta}$ G values under all conditions(compare left with right group of bars): a negative value of $~$ –4 kJ/mol with respect to the Kv2.1 background (left bar),a large positive value of $~$ 12 kJ/mol when the respective otherKv1.2 terminus was already present (third bar from the left),and only small values when either only the S4–S5 linker(second bar from the left) or the S4–S5 linker plus theother terminus (right bar) of Kv1.2 was/were already present.The S4–S5 linker produced large positive values of $~$ 8 kJ/molwhen either only the N- or only the C-terminus of Kv1.2 wasalready present. However, the S4–S5 linker was ineffectivewhen both termini were already present. Changes of the equivalentgating charge, ${Delta}$ z, inferred by the insertion of a Kv1.2 regioninto Kv2.1, were determined from the difference of the z values(bottom bar graph in Fig. 6). It is noticeable that the profilesof ${Delta}$ z for the N- and C-terminus were also similar to each otherand dissimilar to that of the S4–S5 linker.

Interaction energy of intracellular Kv1.2 regions associated with steady-state activation
We first estimated interaction energies for pairs of intracellularregions at half-maximum steady-state activation. In analogyto the above analysis for the change of the rate constants uponactivation, double-mutant cycle analysis was performed, nowusing the ${Delta}$ ${Delta}$ G values obtained by Eq. 5 to calculate ${Delta}$ ${Delta}$ G_Interaction.The results for pairs of intracellular regions with the Kv2.1sequence in the third region are shown in Fig. 7 A (left). Allinteraction energies are positive. The interaction between theN- and C-terminus is strong whereas that of the S4–S5linker with the C- or N-terminus is weak. Fig. 7 A (right) showsthat the interaction between the N- and C-terminus is lost inthe presence of the Kv1.2 S4–S5 linker. Furthermore, inthe presence of the respective other Kv1.2 terminus the interactionenergy of the S4–S5 linker with either the N- or C-terminusbecomes negative. The energy profiles associated with half-maximumsteady-state activation resemble those calculated for k₁ at0 mV (Fig. 5).

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FIGURE 7 Interaction energy ( ${Delta}$ ${Delta}$ G_Interaction) between the N-terminus, S4–S5 linker, and C-terminus associated with steady-state activation. ${Delta}$ ${Delta}$ G_Interaction was determined with the double-mutant cycle analysis. The abbreviations are explained in the legend to Fig. 5. (A) Interaction energy calculated for the voltages of half-maximum activation. ${Delta}$ ${Delta}$ G_Interaction was determined from energies obtained by Eq. 5 using the parameters in Fig. 6. (B) Interaction energy at 0 and 40 mV. ${Delta}$ ${Delta}$ G_Interaction was determined from energies calculated by Eq. 6. For further explanation see text.

We next considered the interaction energies for pairs of intracellularregions not at the same degree of steady-state activation butat equal voltage. According to Scheme 1, ${Delta}$ G was calculated by

(6)
where L = k₁/k₂ = P_o/(1 – P_o) is the simplifiedequilibrium constant indicating the relative stability of theopen channel. In analogy to the rate constants, we chose thevoltages of 0 and 40 mV and computed L from I_rel/(1 –I_rel) by Eq. 1. As described above, ${Delta}$ ${Delta}$ G_Interaction was obtainedby double-mutant cycle analysis (Fig. 7 B). At 0 mV the interactionenergies are close to those calculated with the V_1/2 valuesspecific for each channel (Fig. 7 A). This result is not surprisingbecause the V_1/2 values are near 0 mV (Fig. 6). With the Kv2.1sequence present in the third region, depolarization from 0to 40 mV did not markedly change the interaction energies. Inthe presence of the respective other Kv1.2 terminus, however,the interaction of the S4–S5 linker with either the N-or C-terminus was markedly weaker at 40 mV than at 0 mV. Thisresult further supports the notion that the S4–S5 linkerinteracts with either the N- or C-terminus in a voltage-dependentfashion and that this interaction depends on the nature of theother respective terminus.

DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

The main results of this work are: 1), Replacement of eitherN-terminus, S4–S5 linker, or C-terminus in slowly activatingKv2.1 channels by respective regions of rapidly activating Kv1.2channels unexpectedly slowed the exponential activation timecourse even further. 2), At the voltage of 0 mV, any furtherinsertion of an intracellular Kv1.2 region produced furtherslowing of activation. In contrast, at the voltage of 40 mVthe intracellular regions produced either slowing, no effect,or in one case acceleration of the activation time course, dependingon the composition of the other intracellular regions. 3), Steady-stateactivation was shifted to more negative potentials by the chimeraswith only the N- or C-terminus replaced whereas all other chimerascaused a shift to more positive potentials. 4), Interactionenergies of the Kv1.2 N- and C-terminus were positive in thepresence of the Kv2.1 S4–S5 linker. However, when theKv1.2 S4–S5 linker was present, this interaction disappeared.The interaction of the S4–S5 linker with the N- and C-terminuswas voltage dependent and depended on the nature of the otherrespective terminus. These results suggest that the N-terminus,the C-terminus, and the S4–S5 linker modulate activationof Kv2.1 channels and these regions interact in a voltage-dependentfashion.

The activation time course
The effects of N- and C-termini on the time course of Kv2.1activation were voltage dependent. At 0 mV, replacement of eitherKv2.1 terminus by the respective Kv1.2 terminus consistentlyslowed the Kv2.1 activation time course, irrespective whetherthe other two intracellular regions originated from Kv1.2 orKv2.1 (Fig. 3). This suggests that the effects of the terminiare independent of the origin of the other two regions. At 40mV, however, replacement of the N-terminus did not slow Kv2.1activation neither in the absence nor presence of the Kv1.2C terminus (Fig. 3; Ch_N versus Kv2.1, Ch_NC versus Ch_C). Onthe other hand, replacement of the C-terminus exerted a strongslowing effect on Kv2.1 activation, in both the absence andpresence of the Kv1.2 N-terminus (Ch_C versus Kv2.1, Ch_NC versusCh_N). These results show that the voltage of 40 mV attenuatesthe slowing effect of the Kv1.2 N-terminus on Kv2.1 activationobserved at 0 mV. The effects of the C-terminus, on the otherhand, are preserved at 40 mV despite the fact that there isstill considerable interaction between N- and C-termini (Fig. 5left).

In the chimeras where the S4–S5 linker of Kv1.2 was present,insertion of the Kv1.2 N-terminus slowed activation at 40 mV(Fig. 5; Ch_NL4/5 versus Ch_L4/5, Ch_NL4/5C versus Ch_L4/5C)whereas insertion of the C-terminus had no slowing effect (Ch_L4/5Cversus Ch_L4/5, Ch_NL4/5C versus Ch_NL4/5). This may indicatethat at 40 mV the N-terminus needs the S4–S5 linker toexert a slowing effect whereas the C-terminus does not.

Energetics of activation
Previous energetic analyses of mutations on Shaker channelswere conducted under the assumption of a simple two-state model(Li-Smerin et al., 2000; Yifrach and MacKinnon, 2002) althoughmuch more sophisticated kinetic models are well substantiated(e.g., Zagotta et al., 1994b; Schoppa and Sigworth, 1998). Thereason for this gross simplification is that only then simpleinterpretations are possible. In this study on Kv2.1 channels,we followed this approach and fitted the steady-state activationversus voltage relationship by a two-state Boltzmann equation.It was therefore only consequential to assume also a singlemean activation time constant, ${tau}$ _m, although the activation timecourses required biexponential functions for description. Ithas to be stated that all energetic estimations performed inthis study, critically depend on these simplifying assumptions,in particular those obtained with the double-mutant cycle analysis.

The ${Delta}$ ${Delta}$ G and ${Delta}$ z values calculated for steady-state activation wereremarkably similar for both termini (Fig. 6); either Kv1.2 terminusproduced negative ${Delta}$ ${Delta}$ G values of $~$ 4 kJ/mol when inserted in Kv2.1channels (Ch_N and Ch_C versus Kv2.1) and positive ${Delta}$ ${Delta}$ G valuesof $~$ 12 kJ/mol when inserted in chimeras with the other Kv1.2terminus present (Ch_NC versus Ch_C and Ch_N), resulting ina, respectively, large positive interaction energy ${Delta}$ ${Delta}$ G_Interactionfor Kv1.2 N- and C-terminus (Fig. 7). This result suggests thatthe negative ${Delta}$ ${Delta}$ G value of –6.23 kJ/mol, calculated for Kv1.2channels with respect to Kv2.1 channels by using Eq. 5, doesnot simply result from the common presence of both termini,but that further channel regions are involved.

Considering the interaction energies of the Kv1.2 regions associatedwith the rate constants k₁ and k₂, it is evident that the valuesdiffer less from each other at 0 mV than at 40 mV (Fig. 5),indicative that the interaction between the three regions issimilarly intensive at 0 mV and more specific at 40 mV. Fork₁, a great depolarization-induced shift to a more positiveinteraction energy was observed only for the interaction ofthe N- with the C-terminus when the S4–S5 linker was notsubstituted. For k₂, a respective shift was observed for theinteraction of the S4–S5 linker with the C-terminus, ineither the absence or presence of the N-terminus, and of theN-terminus with the C-terminus when the S4–S5 linker wassubstituted. A pronounced shift to more negative interactionenergies was observed in only one case for k₁, for the interactionof the N-terminus with the S4–S5 linker when the C-terminuswas also substituted. The other interactions were lesser voltagedependent.

Inspection of the profiles of interaction energies calculatedfor steady-state conditions (Fig. 7, A and B) and those obtainedfor the rate constants k₁ and k₂ (Fig. 5) showed that only thosefor steady-state activation at either V_1/2 or 0 mV and thatfor k₁ at 0 mV were similar. This result suggests that activationat 0 mV essentially involves changed intramolecular interactionsassociated with the forward reaction (k₁ in Scheme 1) whereasat 40 mV also the backward reaction (k₂) is involved.

Relations to previous work
VanDongen and co-workers (1990) were the first to suggest aninteraction between N- and C-termini in Kv2.1 channels. Theyobserved a slowed activation in N-terminally deleted Kv2.1 channelsand reversal of this slowing effect when a sizable part of theC-terminus had been additionally deleted. By itself, however,the C-terminal deletion was without effect on Kv2.1 activationkinetics. An interaction between the Kv2.1 termini was alsosuggested by the result that phosphorylation of the Kv2.1 C-terminusby protein kinase A depends on the N-terminus (Wilson et al.,1994). More detailed insight into this interaction came fromrecent results by Ju and co-workers (2003) who observed effectson the activation time course by two residues in the N-terminalT1 domain (residues 67 and 75) and by up to 15 residues in aC-terminal activation (CTA) domain. The authors presented evidencethat these effects are mediated by an interaction between theN-terminal residues and the CTA domain. They concluded thatnot only the T1 domain but also the CTA domain may contributeto the hanging gondola below the membrane. It was proposed thatthe T1 domain might affect activation by changing first theconformation of the CTA domain and thereby the one of the S6segment, which lines the pore. The authors also concluded thatthe effective residues in the termini cannot interact with theS4 segment or its nearby intracellular loops. Our data, however,also suggest interactions between the S4–S5 linker andthe termini.

Also in Kv1.1 channels an interaction between N- and C-terminihas been hypothesized based on the observation that oxidizingconditions promote the formation of a disulfide bond betweenan N-terminal cysteine, close to the tetramerization T1 domain,and a C-terminal cystein, close to the S6 segment (Schulteiset al., 1996). The fact that interactions between N- and C-terminiare not only present in the Kv2 subfamily but also in the Kv1subfamily might indicate that they are generally important amongKv channels.

Another observation in our study was that the equivalent gatingcharge z of all chimeras exceeded that in Kv2.1 channels, irrespectiveof whether the V_1/2 values were shifted to more positive ornegative voltages (cf. Fig. 6). This result deviates from thoseobserved for a multitude of pore mutations in Shaker channelswhere z decreased with less negative V_1/2 (Yifrach and MacKinnon,2002). A possible interpretation of this result is that theKv1.2 regions indeed confer the property of a steeper steady-stateactivation to Kv2.1 channels whereas the kinetics of activationare hampered by additional interactions.

Perspectives
Although the slowing effects and interaction energies studiedherein were systematic, our results do not unequivocally prove,that the respective cytosolic regions indeed contribute to theactivation time course in wild-type Kv2.1 channels. It is conceivablethat the Kv2.1 channel molecules have been optimized duringevolution to such a high degree that all rate limitation ofthe activation process is caused by reactions in the core region.Nevertheless, the fact that manipulations on the intracellularchannel regions can influence the activation kinetics, stronglysuggests that these regions are targets for the control of theactivation time course, e.g., via the cytoskeleton or by thebinding of other cytosolic or peripheral membrane proteins.

ACKNOWLEDGEMENTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

We thank S. Bernhardt, A. Kolchmeier, K. Schoknecht, and B.Tietsch for excellent technical assistance.

This work was supported by the grant Be1250/4-3 of the DeutscheForschungsgemeinschaft to K.B.

Submitted on January 22, 2004; accepted for publication May 5, 2004.

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MATERIALS AND METHODS
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DISCUSSION
ACKNOWLEDGEMENTS
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