XB-ART-2832
J Gen Physiol
2004 Nov 01;1245:587-603. doi: 10.1085/jgp.200409023.
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Polyvalent cations constitute the voltage gating particle in human connexin37 hemichannels.
Puljung MC
,
Berthoud VM
,
Beyer EC
,
Hanck DA
.
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Connexins oligomerize to form intercellular channels that gate in response to voltage and chemical agents such as divalent cations. Historically, these are believed to be two independent processes. Here, data for human connexin37 (hCx37) hemichannels indicate that voltage gating can be explained as block/unblock without the necessity for an independent voltage gate. hCx37 hemichannels closed at negative potentials and opened in a time-dependent fashion at positive potentials. In the absence of polyvalent cations, however, the channels were open at relatively negative potentials, passing current linearly with respect to voltage. Current at negative potentials could be inhibited in a concentration-dependent manner by the addition of polyvalent cations to the bathing solution. Inhibition could be explained as voltage-dependent block of hCx37, with the field acting directly on polyvalent cations, driving them through the pore to an intracellular site. At positive potentials, in the presence of polyvalent cations, the field favored polyvalent efflux from the intracellular blocking site, allowing current flow. The rate of appearance of current depended on the species and valence of the polyvalent cation in the bathing solution. The rate of current decay upon repolarization depended on the concentration of polyvalent cations in the bathing solution, consistent with deactivation by polyvalent block, and was rapid (time constants of tens of milliseconds), implying a high local concentration of polyvalents in or near the channel pore. Sustained depolarization slowed deactivation in a flux-dependent, voltage- and time-independent fashion. The model for hCx37 voltage gating as polyvalent block/unblock can be expanded to account for observations in the literature regarding hCx37 gap junction channel behavior.
???displayArticle.pubmedLink??? 15504903
???displayArticle.pmcLink??? PMC2234009
???displayArticle.link??? J Gen Physiol
???displayArticle.grants??? [+]
DA-07255 NIDA NIH HHS , F31NS-42972 NINDS NIH HHS , HL-45466 NHLBI NIH HHS , R01 HL059199-05A2 NHLBI NIH HHS , R01 HL059199 NHLBI NIH HHS , T32 DA007255 NIDA NIH HHS , R01 HL045466 NHLBI NIH HHS , F31 NS042972 NINDS NIH HHS
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Figure 1. . Nonjunctional currents from hCx37 expressed in Xenopus laevis oocytes. (A, top) Currents resulting from a series of voltage steps from a holding potential of â40 mV in 10-mV increments to a potential of +90 mV in an oocyte injected with RNA encoding hCx37 plus AntiCx38. (A, bottom) Currents from an oocyte injected only with AntiCx38. Currents were recorded in 0DivOR2 plus 1 mM Ca2+. (B) Average, isochronal (see materials and methods) currentâvoltage relationship for oocytes injected with hCx37 RNA plus AntiCx38 (âª, n = 10) and oocytes injected only with AntiCx38 (â, n = 3). Currents were recorded in 0DivOR2 plus 0.5 mM Ca2+. (C) Normalized, average, isochronal currentâvoltage relationships for oocytes injected with hCx37 RNA plus AntiCx38, recorded in 0DivOR2 plus 0.5 mM Ca2+ in the presence (â¢, n = 3) or absence (âª, n = 10) of 10 mM 1-heptanol. Currents in the absence of heptanol were corrected by subtracting the mean of the oocytes injected only with AntiCx38. Currents in the presence of heptanol were not corrected by the control currents, since the endogenous sodium current in oocytes was completely inhibited by 10 mM 1-heptanol (not depicted). All currents were normalized to the peak current at +90 mV in the absence of 1-heptanol. The currentâvoltage relationships were all leak corrected. |
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Figure 2. . hCx37 hemichannel currents lose their voltage and time-dependent properties in oocytes following wash-out of divalent cations. (A) Representative currents resulting from a series of steps from a holding potential of â40 mV to potentials ranging from â100 to +90 mV in 10-mV increments for an oocyte injected with hCx37 RNA along with AntiCx38 (left) and an oocyte injected with AntiCx38 alone (right) stored in 0DivOR2. (B) Average, isochronal currentâvoltage relationships over the voltage range from â100 to +90 mV for oocytes injected with hCx37 RNA plus AntiCx38 (âª, n = 6) and oocytes injected only with AntiCx38 (â, n = 5). (C) Average, isochronal currentâvoltage relationships over the voltage range from â100 to +10 mV for oocytes injected with hCx37 RNA plus AntiCx38 (âª, n = 30) and oocytes injected only with AntiCx38 (â, n = 20). (D) Bar graph showing macroscopic hCx37 hemichannel conductance (assessed between â60 and 0 mV) as a function of the amount of hCx37 RNA injected into the oocyte (n = 2, 60 ng; n = 3, 12 ng; n = 4, 6 ng; n = 4, 3 ng; n = 4, 0.3 ng). The asterisk corresponds to current levels that were significantly larger than those with 0.3 ng injected (P < 0.0001, Student's t test). |
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Figure 3. . hCx37 hemichannel currents are reversibly inhibited by divalent cations. Representative currents resulting from a series of voltage steps from a holding potential of â40 mV to potentials ranging from â100 to +10 mV in 10-mV increments for oocytes injected with hCx37 RNA along with AntiCx38 (A and C) and an oocyte injected only with AntiCx38 (B). (A) Currents from hCx37 hemichannels before (left), during treatment with (middle), and after wash-out of (right) 1 mM Ca2+. (B) Currents from an oocyte injected only with AntiCx38 before (left), during treatment with (middle), and after wash-out of (right) 1 mM Ca2+. (C) Currents from hCx37 hemichannels before (left), during treatment with (middle), and after wash-out of (right) 20 mM Mg2+. (D) Average, isochronal currentâvoltage relationships for oocytes injected with hCx37 RNA plus AntiCx38 and stored in 0DivOR2. Recordings were made before (âª, n = 8), during treatment with (â¢, n = 8), and after wash-out of (â´, n = 8) 1 mM Ca2+. (E) Average, isochronal currentâvoltage relationships for oocytes injected with AntiCx38 alone and stored in 0DivOR2. Recordings were made before (âª, n = 3), during treatment with (â¢, n = 3), and after wash-out of (â´, n = 3) 1 mM Ca2+. (F) Average, isochronal currentâvoltage relationships for oocytes injected with hCx37 RNA plus AntiCx38 and stored in 0DivOR2. Recordings were made before (âª, n = 6), during treatment with (â¢, n = 6), and after wash-out of (â´, n = 6) 20 mM Mg2+. (G) Concentrationâresponse curves (see materials and methods) showing inhibition of hCx37 hemichannel current at â40 mV as a function of [Ca2+] (â¢) and [Mg2+] (âª). The IC50 for Ca2+ was 107 μM with a Hill coefficient of 3.1 ± 0.5 (20 μM, n = 3; 100 μM, n = 3; 200 μM, n = 5; 1 mM, n = 4; 2 mM, n = 6). The IC50 for Mg2+ was 1.30 mM with a Hill coefficient of 4.5 ± 1.1 (500 μM, n = 5; 1 mM, n = 6; 2 mM, n = 4; 5 mM, n = 3; 10 mM, n = 5; 20 mM, n = 4). |
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Figure 4. . The rate of divalent cation inhibition of hCx37 hemichannel currents was concentration dependent. (A) Representative trace showing current from an individual oocyte injected with hCx37 RNA plus AntiCx38. The disappearance of current (left) is upon wash-in of 1 mM Ca2+. The reappearance of current (right) is upon wash-out of Ca2+. These recordings were performed at a holding potential of â40 mV. Both wash-in and wash-out traces were fit with single exponential curves to determine kmod. The time courses were fit with an equation of the form I = Iâ â Aeâkt, where I is the current, Iâ is the amount of current at steady state, A is the amplitude, t is time, and k is kmod (see results). The concentration dependence of kmod for hCx37 hemichannel current at â40 mV is shown for Ca2+ (B) and Mg2+ (C). Both plots were fit with straight lines. For Ca2+, r = 0.86; 0 mM, n = 4; 0.1 mM, n = 2; 0.2 mM, n = 5; 1 mM, n = 5; 2 mM, n = 3. For Mg2+, r = 0.82; 0 mM, n = 2; 1 mM, n = 4; 2 mM, n = 1; 5 mM, n = 4; 10 mM, n = 5, 20 mM, n = 2. |
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Figure 5. . Gd3+ inhibits hCx37 hemichannel current. (A) Representative currents resulting from a series of steps from a holding potential of â40 mV to potentials ranging from â100 to +10 mV in 10-mV increments for an oocyte injected with hCx37 RNA along with AntiCx38. The currents were recorded before (left) and after (right) the addition of 100 μM Gd3+ to the bath. (B) Bar graph showing kmod for hCx37 hemichannel current inhibition by two different concentrations of Gd3+, 100 μM (n = 4) and 200 μM (n = 4). |
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Figure 6. . Polyvalent cation inhibition of hCx37 hemichannels is voltage dependent. (A) Plot of kmod for hCx37 hemichannel current inhibition by 200 μM Ca2+ as a function of potential (âª; â110 mV, n = 1; â100 mV, n = 4; â90 mV, n = 3; â80 mV, n = 4; â60 mV, n = 5; â40 mV, n = 4; â20 mV, n = 4). The curve is a single exponential decay fit to the data of the form kmod = kpos + AeâV/dV, where kpos is the minimum kmod at more positive potentials, A is the amplitude, V is voltage, an dV is the amount in millivolts necessary to change kmod by a factor of e. The open circles (â) represent koff as a function of potential (â100 mV, n = 2; â80 mV, n = 3; â60 mV, n = 6; â40 mV, n = 5; â20 mV, n = 3). The straight line shows the mean koff of 0.0035 sâ1. The inset shows a plot of the percent inhibition by 200 μM Ca2+ as a function of holding potential (â100 mV, n = 4; â60 mV, n = 4; â40 mV, n = 5; â20 mV, n = 3). The curve in the inset represents the predicted percentage block as a function of potential, based on a model of voltage-dependent block for which steady-state block (ssblock) is given by the equation ssblock = 100/(1 + 10((log(IC50) â log[Ca])*p)), where IC50 is predicted by the fits to the measured kon and koff as a function of potential (A, C, and D) and p is the Hill coefficient for Ca2+ binding (â¼3.1). Data from the inset were leak corrected by the mean of the AntiCx38-injected oocytes from the day each data point was acquired (n = 2â4). The data were normalized to block at â100 mV where close to 100% block is predicted by the above equation for 200 μM Ca2+. (B) Plot of kmod for hCx37 hemichannel current inhibition by 1 mM Mg2+ as a function of potential (âª; â100 mV, n = 2; â90 mV, n = 1; â80 mV, n = 2; â70 mV, n = 1; â60 mV, n = 4; â50 mV, n = 2; â40 mV, n = 9). The curve is a single exponential decay fit to the data of the form shown in A. The open circles (â) represent koff as a function of potential (â60 mV, n = 4; â40 mV, n = 2). The straight line shows the mean koff of 0.0024 sâ1. (C) Plot of kmod for hCx37 hemichannel current inhibition by 100 μM Gd3+ as a function of potential (â110 mV, n = 2; â100 mV, n = 7; â90 mV, n = 3; â80 mV, n = 5; â60 mV, n = 3; â40 mV, n = 4). The curve is a single exponential decay fit to the data of the form shown in A. (D) Plot of kon for Ca2+ (âª), Mg2+ (â¢), and Gd3+ (â´) ions as a function of holding potential. The curves are single exponential decays fit to the data of the form kon = kpos + AeâV/dV (see results). |
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Figure 7. . Activation rate of hemichannel current depends on the ions in the bathing solution. (A) Currents resulting from a series of voltage steps from a holding potential of â40 mV in 10-mV increments to a potential of +90 mV applied to oocytes injected with hCx37 RNA plus AntiCx38, recorded in 0DivOR2 plus 1 mM Ca2+ (left) or 200 μM Gd3+ (right). These currents were fit with the sum of two exponentials to determine rate constants (see results). (B) Fast activation rate constant (kfast) as a function of potential for hCx37-expressing oocytes recorded in 0DivOR2 containing 1 mM Ca2+ (â; +40 mV, n = 8; +50 mV, n = 8; +60 mV, n = 8; +70 mV, n = 9; +80 mV, n = 8; +90 mV, n = 8; +100 mV, n = 8) or 200 μM Gd3+ (âª; +60 mV, n = 15; +70 mV, n = 16; +80 mV, n = 16; +90 mV, n = 16; +100 mV, n = 10). (C) Slow activation rate constant (kslow) as a function of potential for hCx37-expressing oocytes recorded in 0DivOR2 containing 1 mM Ca2+ (â; +40 mV, n = 3; +50 mV, n = 7; +60 mV, n = 6; +70 mV, n = 7; +80 mV, n = 7; +90 mV, n = 8; +100 mV, n = 8) or 200 μM Gd3+ (âª; +60 mV, n = 15; +70 mV, n = 16; +80 mV, n = 16; +90 mV, n = 16; +100 mV, n = 10). (D) kfast (upper) and kslow (lower) for hCx37 hemichannel current recorded in 0DivOR2 containing 1 mM Ca2+ (â) or 0.5 mM Ca2+ (â´). For kfast in 0.5 mM Ca2+, at +40 mV, n = 10; +50 mV, n = 9; +60 mV, n = 10; +70 mV, n = 10; +80 mV, n = 10; +90 mV, n = 9; and +100 mV, n = 10. For kslow in 0.5 mM Ca2+, at +40 mV, n = 1; +50 mV, n = 6; +60 mV, n = 10; +70 mV, n = 10; +80 mV, n = 10; +90 mV, n = 10; and +100 mV, n = 10. (E) kfast (upper) and kslow (lower) for hCx37 hemichannel current recorded in 0DivOR2 containing 200 μM Gd3+ (âª) or 100 μM Gd3+ (â). For kfast in 100 μM Gd3+ at +60 mV, n = 5; +70 mV, n = 6; +80 mV, n = 6; +90 mV, n = 6; and +100 mV, n = 6. For kslow in 100 μM Gd3+ at +60 mV, n = 2; +70 mV, n = 6; +80 mV, n = 6; +90 mV, n = 6; and +100 mV, n = 5. |
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Figure 8. . Current deactivation depends on polyvalent concentration and flux during channel opening. (A) Fast and slow rate constants of deactivation in 0.5 mM Ca2+ as a function of the length of the depolarizing pulse to +90 mV. At 10 s, n = 10, at 20 s, n = 9, and at 40 s, n = 6. The inset shows representative current traces that are the response to depolarization for 5, 10, 20, and 40 s to +90 mV from a holding potential of â40 mV, followed by repolarization to â40 mV. (B) Fast and slow rate constants of deactivation at â40 mV following 40-s depolarizing pulses to +90 mV as a function of extracellular Ca2+ concentration. The inset shows representative tail currents recorded upon repolarization to â40 mV in 0DivOR2 plus 1.0 mM Ca2+ and 0.5 mM Ca2+. For 0.5 mM Ca2+, n = 6; for 1.0 mM Ca2+, n = 9. (C) Fast (triangles) and slow (circles) rate constants for deactivation at â40 mV as a function of the amount of charge passed during 40-s depolarizing pulses to +90 mV (filled symbols) or +70 mV (open symbols). Each data point represents an individual experiment. A total of six oocytes was used to gather the data. The data were fit to straight lines (kfast, r = 0.9; kslow, r = 0.7). The inset shows representative current traces corresponding to depolarization from a holding potential of â40 to +70 mV and +90 mV followed by repolarization to â40 mV in a single oocyte. Data were acquired at a sampling rate of 100 Hz and filtered at 50 Hz. Rate constants were corrected by the koff for Ca2+ at negative potentials (0.0035 sâ1) to yield a value of kon*[Ca2+]. |
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Figure 9. . Gating model for hCx37 hemichannels. Illustration of the gating process for hCx37 hemichannels. At negative potentials (left) the channel is occupied with several polyvalent cations. These bind to a site on the cytoplasmic side of the channel, blocking current flow. At positive potentials (center) the koff for the polyvalent cations becomes significant, the ions are ejected from the site of block, and current is allowed to flow. Polyvalent cations remain at a high local concentration. Upon extended depolarization (right), the local concentration is depleted as well. Upon repolarization, the polyvalent cations bind the channel again, inhibiting current flow (left). A kinetic model for hCx37 hemichannel gating is shown below. Cx is the blocked hemichannel, Cx* is the unblocked hemichannel, Cx** is the unblocked hemichannel free of any polyvalent cations, M+ is a polyvalent cation, n is the minimum number of polyvalent cations needed to inhibit current (see discussion). |
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Figure 10. . Polyvalent cation effects are not due to surface charge screening. (A) Simulated conductanceâvoltage curves. Each curve is shifted 40 mV relative to the next. Increasing numbers correspond to increasing amounts of polyvalent cations (see discussion). The inset shows currentâvoltage relationships corresponding to the conductanceâvoltage relationships. The bold lines in both the figure and inset correspond to the maximal conductance over the voltage range depicted. (B) Plot of the conductanceâvoltage relationship for hCx37 in 0DivOR2 plus 0.02 mM Ca2+ (âª, n = 6), 0.1 mM Ca2+ (â¢, n = 4), 0.2 mM Ca2+ (â´, n = 6), and 1 mM Ca2+ (â¾, n = 4). The corresponding, isochronal currentâvoltage relationships, shown in the inset, represent current responses to the voltage protocol shown in Fig. 2. Conductance was determined at each potential from the slope of the currentâvoltage relationship between adjacent points. The dashed lines in the inset are predicted currents after 2.5-s voltage pulses based on the expectation from steady-state block in Fig. 6. In brief, the steady-state block was determined for â40 mV, and each new test potential. These values were connected by single exponentials with kmod determined by the measured koff and kon (Fig. 6) and the [Ca2+]. The predicted amount of block at 2.5 s was multiplied by an open-channel, currentâvoltage relationship predicted by a line formed between the current at â40 mV, divided by the fractional block at that potential (Fig. 3 G) and the origin. |
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