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The Journal of Neuroscience, September 27, 2006, 26(39):9851-9859; doi:10.1523/JNEUROSCI.1862-06.2006
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Cellular/Molecular
Na+, Cl–, and pH Dependence of the Human Choline Transporter (hCHT) in Xenopus Oocytes: The Proton Inactivation Hypothesis of hCHT in Synaptic Vesicles
Hideki Iwamoto, Randy D. Blakely, andLouis J. De Felice Department of Pharmacology and Center for Molecular Neuroscience, Vanderbilt University School of Medicine, Nashville Tennessee 37232-8548
Abstract
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Abstract
Introduction
The recent cloning of the human choline transporter (hCHT) has allowed its expression in Xenopus laevis oocytes and the simultaneous measurement of choline transport and choline-induced current under voltage clamp. hCHT currents and choline transport are evident in cRNA-injected oocytes and significantly enhanced by the hCHT trafficking mutant L530A/V531A. The charge/choline ratio of hCHT varies from 10e/choline at –80 mV to 3e/choline at –20 mV, in contrast with the reported fixed stoichiometry of the Na+-coupled glucose transporter in the same gene family. Ion substitution shows that the choline uptake and choline-induced current are Na+ and Cl– dependent; however, the reversal potential of the induced current suggests a Na+-selective mechanism, consigning Cl– to a regulatory role rather than a coupled, cotransported-ion role. The hCHT-specific inhibitor hemicholinium-3 (HC-3) blocks choline uptake and choline-induced current; in addition, HC-3 alone reveals a constitutive, depolarizing leak current through hCHT. We show that external protons reduce hCHT current, transport, and binding with a similar pKa of 7.4, suggesting proton titration of residue(s) that support choline binding and transport. Given the localization of the choline transporter to synaptic vesicles, we propose that proton inactivation of hCHT prevents acetylcholine and proton leakage from the acidic interior of cholinergic synaptic vesicles. This mechanism would allow cholinergic, activity-triggered delivery of silent choline transporters to the plasma membrane, in which normal pH would reactivate the transporters for choline uptake and subsequent acetylcholine synthesis.
Key words: choline transporter; Xenopus oocyte; choline-induced current; Na+; Cl–; pH
Introduction
Cholinergic neurons release acetylcholine (ACh) for autonomic functions in sympathetic and parasympathetic neurons as well as cognitive activity associated with central pathways (Dani and DeBiasi, 2001; Bymaster et al., 2003
Cholinergic neurons increase choline uptake via CHT in proportion to ACh demand and resynthesis (Simon and Kuhar, 1975
The low density of CHT in mammalian cholinergic neurons hampered efforts to clone and characterize CHT. However, the cloning of CHT cDNA (cho-1) from Caenorhabtiditis elegans (Okuda et al., 2000
Materials and Methods
hCHT expression in Xenopus leavis oocytes. The isolation of oocytes and cRNA preparation were described previously (Ramsey and DeFelice, 2002Two-electrode voltage clamp. Whole-cell currents were measured with two-electrode voltage-clamp techniques using a GeneClamp 500 (Molecular Devices, Palo Alto, CA). Microelectrodes were pulled using a programmable puller (model P-87; Sutter Instruments, Novato, CA) and filled with 3 M KCl (0.5–3 M
resistance). A 16-bit analog-to-digital converter (Digidata 1322A; Molecular Devices) interfaced to a personal computer (PC) running Clampex 9 software (Molecular Devices) was used to control membrane voltage and to acquire data. To induce hCHT-associated current, oocytes were perfused with choline chloride dissolved in modified Ringer's solution (in mM: 100 NaCl, 5 potassium gluconate, 5 HEPES, 1 MgSO4, and 0.5 calcium acetate, pH 7.4) using a gravity-flow system (4–5 ml/min flow rate). pH of buffer was adjusted with N-methyl-D-glucamine or phosphoric acid. To minimize liquid junction potentials, chloride substitution experiments were performed using a salt bridge to isolate the Ag–AgCl electrode from the bath. For constant-voltage recordings, data were low-pass filtered at 10 Hz and digitized at 20 Hz. For current–voltage (I–V) recordings, the voltage was changed stepwise every 500 ms. Currents were low-pass filtered at 100 Hz and digitized at 200 Hz. All analyses were performed using Origin 7 (Microcal, Northampton, MA).
Surface-biotinylation Western blotting. The full procedures were described previously (Ramsey and DeFelice, 2002
[3H]Choline transport assays. Choline uptake in WT- or LV-expressing oocytes was measured by incubation with 10 µM choline chloride containing 1% of [3H]choline chloride (86 Ci/mmol; PerkinElmer) in modified Ringer's buffer for 30 min at room temperature. Assays were terminated by washing extensively with ice-cold buffer. Specific uptake was defined by subtracting the uptake obtained in nontransfected, water-injected control oocytes from uptake in cRNA-injected oocytes. Oocytes were solubilized with 1% SDS, and choline accumulation was quantified with a liquid scintillation counter (TopCount NXT; Packard Instrument Company, Meriden, CT).
[3H]Hemicholinium-3 binding assays. Most procedures were the same as those used for choline uptake experiments described above. The WT- or LV-expressing oocytes were incubated with 10 nM [3H]HC-3 (125 Ci/mmol; PerkinElmer) in modified Ringer's solution for 30 min at room temperature (Sandberg and Coyle, 1985
Simultaneous measurement of choline uptake and choline-induced current. Simultaneous measurement of choline uptake and choline-induced current was performed under voltage-clamp conditions, using techniques described previously (Petersen and DeFelice, 1999
Results
Choline induces an inward current in hCHT-expressing oocytes
Oocytes expressing the hCHT WT take up [3H]choline (Fig. 1A) and generate inward currents when choline is added to the bath (Fig. 1B). In mammalian cells, the trafficking mutant LV results in increased surface expression (Ruggiero, Ferguson, and Blakely, unpublished observation). In oocytes, the choline uptake and choline-induced current in LV mutants are approximately three times larger than WT uptake and currents under the same conditions (Fig. 1A,B). In addition, WT and LV oocytes have shifted holding currents for the same voltage, indicating a constitutive depolarization in the absence of choline (leak current) (Fig. 1B, inset). Water-injected oocytes show no detectable choline-induced current. Figure 1B plots the relationship between choline-induced current (bars in inset) and membrane voltage. The I–V curves for WT have no detectable reversal potential, whereas LV reversal potentials are in the range of 45–60 mV. The reversal potential for LV is near the Nernst potential for Na+, 39 mV at room temperature, if we assume that internal Na+ concentration in oocytes is 22 mM (Kusano et al., 1982
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Figure 1. Choline uptake and choline-induced current in hCHT-expressing oocytes. A, Uptake assays were performed with 10 µM choline containing 1% [3H]choline and measured over a period of 30 min in both hCHT WT-expressing and LV-expressing oocytes with and without 10 min preincubation of the hCHT-specific inhibitor HC-3 at 1 µM (n = 5–8). B, The choline-induced I–V curves were generated by brief exposure to 10 µM choline at various membrane potentials (n = 5). Baseline current in the absence of choline was subtracted from the choline-induced current. Inset, Choline at 10 µM induced a significant current when the oocyte was held at –60 mV. Note that the holding currents in WT- and LV-expressing oocyte are shifted compared with control oocyte.
hCHT charge/choline ratio depends on voltage
Choline-induced currents in hCHT oocytes suggest that choline transport is electrogenic, i.e., net charge accompanies choline flux. To examine how many charges attend each choline molecule during transport, we measured choline uptake and choline-induced current simultaneously under voltage clamp. Figure 2A shows that choline uptake depends on membrane voltage. Although charge and uptake both decrease with depolarization, the charge/flux ratio is not constant. Figure 2B shows that the charge/choline ratio varies linearly from10 at –80 mV to 3 at –20 mV.
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Figure 2. Simultaneous measurement of uptake and current. A, Choline at 10 µM containing 1% [3H]choline induced current and promoted choline uptake, which were measured concurrently in the same oocyte under voltage clamp for 500 s (for details, see Materials and Methods). Each point consists of data from three to four different oocytes. The LV mutant was used in this experiment. B, The charge/substrate ratio is plotted as a function of voltage from the data in A.
LV has increased surface expression, which correlates with transport and current
The choline-induced hCHT current in WT and LV depends on not only voltage but also on choline concentration (Fig. 3A,B). To obtain the apparent affinity (Km) of choline for hCHT, we plotted the current at –100 mV against the choline concentration (Fig. 3C). Fitting these data to a single-binding-site model, the Km is similar for both WT and the LV mutant (0.7 ± 0.1 and 1.0 ± 0.1 µM, respectively; n = 5). The Km obtained from choline-induced current is comparable with that for choline uptake in Xenopus oocytes and mammalian cells (Apparsundaram et al., 2000
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Figure 3. The I–V curves for WT and LV transporters for various choline concentrations. I–V curves measured with choline concentrations from 0.05 to 50 µM for WT (A) and the LV mutant (B) (n = 5). C, From A and B, the currents at –100 mV are plotted for different choline concentrations. These data were then fit to a Michaelis–Menten equation to obtain the apparent affinity (Km) and maximal current (Imax). Km of 0.7 ± 0.1 µM and Imax of –13.3 ± 0.2 nA for WT. Km of 1.0 ± 0.1 µM and Imax of –37.9 ± 0.3 nA for LV. D, Surface biotinylation Western blotting. Water-injected control oocytes show no detectable hCHT expression (CTL). A rectangular box represents hCHT monomers. Band densities of surface fraction at 55 kDa show that LV is 2.6 ± 0.3 times greater than WT (n = 3), consistent with Imax differences between LV and WT. Total expression for WT and LV show no significant differences (Student's t test, p > 0.05; n = 3).
HC-3 reveals leak current in the absence of choline
HC-3 is a potent and specific inhibitor for high-affinity choline uptake (Ki of 5 nM) (Okuda and Haga, 2003
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Figure 4. HC-3 inhibits choline-induced current. A, HC-3 at 1 µM inhibits the choline-induced current (10 µM choline at –60 mV). Perfusion of 1 µM HC-3 alone reveals an apparent outward current (leak) in the transporter (white bar). There was no detectable leak current for control oocytes under the same conditions. A slow baseline drift was removed from A. B, I–V curves for 10 µM choline-induced current and 1 µM HC-3-revealed leak current were obtained from WT and LV mutants (n = 5). C, The ratio of choline-induced current to HC-3-revealed leak current is calculated from B. The ratio is constant at any voltage for either WT or LV. D, Leak current depolarizes oocytes. Resting potentials were assessed in water-injected control oocytes, WT-expressing oocytes, and LV-expressing oocytes in the absence of choline. Compared with the water-injected control oocytes, resting potentials in WT- and LV-expressing oocytes were significantly depolarized (n = 7).
Choline-induced currents depend on external Na+ and Cl–
Na+ and Cl– are necessary for high-affinity choline uptake (Simon and Kuhar, 1976
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Figure 5. The role of cations and anions in the choline-induced current. A, The effect of cation substitutions in control oocytes. NaCl at 100 mM was replaced with equimolar KCl, LiCl, or TEACl. No choline-induced current was observed when 10 µM choline (thick black bars) was perfused onto water-injected control oocytes held at –60 mV. The baseline is normalized to the value in NaCl. B, Effect of cation substitutions in LV oocytes. Choline-induced current is observed only in NaCl. The magnitude of baseline shift with cation substitution is different LV oocytes compared with control oocytes. C, Effect of anion substitutions in LV-expressing oocytes. NaCl at 100 mM was replaced with equimolar NaBr, NaGlu, or NaMS. Choline-induced current was observed only in NaCl and NaBr. No choline-induced current was observed in water-injected control oocytes. The magnitude of baseline shift with anion substitution is different LV oocytes compared with control oocytes (data not shown). D, Summary of cation and anion dependence of choline-induced current (n = 5). Choline-induced current depends strictly on Na+ but less stringently on Cl–, because Br– can partially replace Cl–. Essentially no difference exists in ionic dependence between WT and LV hCHT-expressing oocytes.
Internal Na+ reduces choline-induced current, but Cl– has no similar effect
The reversal potential of choline-induced current suggests that hCHT is Na+ selective (Fig. 1B); however, the induced current requires both external Na+ and Cl– (Fig. 5D). This is explained if hCHT uses external Cl– to regulate transport but does not transport Cl–. To test this idea, LiCl was injected into oocytes, which should inhibit the induced current if it is partly carried by Cl–. To test this expectation for Na+, we injected NaGlu into the oocyte. When a high concentration of NaGlu was injected (final concentration is
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Figure 6. Internal Na+, but not Cl–, suppresses the choline-induced current. A, Top row, NaGlu (46 nl of 0.5 M) was injected into LV-expressing oocytes. The final concentration of internal NaGlu is
pH regulates choline-induced current, choline transport, and HC-3 binding
We found that choline-induced current depends not only on Na+ and Cl– but also on external pH. Figure 7A shows pH dependence of 10 µM choline-induced current at –60 mV. The current is abolished at pH 5.5. The activation and deactivation of choline-induced currents by pH is reversible (data not shown). Figure 7B shows the normalized pH dependence of choline-induced current, indicating a pKa of 7.4. No significant difference between WT and LV was observed. We measured I–V curves for 10 µM choline-induced currents for pH between 5.5 and 8.5. The currents at different pH intersect over a narrow range of voltages (30–50 mV) (supplemental figure, available at www.jneurosci.org as supplemental material), which appears to be independent of pH. However, because the induced current is small near reversal and smaller still at low pH, it is difficult to determine relative ionic permeation from reversal potentials. Choline uptake (Fig. 7C) and HC-3-specific binding (Fig. 7D) exhibit similar pH dependences. One concern is that the pKa is close to that of HEPES buffer (pKa of 7.55), and HEPES has structural similarity to choline (both have an N-ethylalcohol moiety). Thus, the possibility exists that HEPES could cause pH-dependent inhibition of hCHT current (Ming et al., 2002
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Figure 7. pH dependence of choline-induced current, choline uptake, and HC-3 binding. A, pH dependence of choline-induced current. Typical data are shown for 10 µM choline-induced current for LV at –60 mV in 100 mM NaCl buffer. The slow baseline drift is removed from the figure. B, pH dependence of 10 µM choline-induced currents at –60 mV are measured for WT and LV (n = 5). The data were normalized to pH 7.4 and fitted to a single-binding-site model. pKa of 7.4 ± 0.1 and Imax of 196.3 ± 10.5% for WT. pKa of 7.3 ± 0.1 and Imax of 174.4 ± 4.0% for LV. C, pH dependence of choline uptake was measured in 10 µM choline (1% [3H]choline) for 30 min (n = 8). pKa of 7.4 ± 0.1 and Vmax of 188.8 ± 3.7% for WT. pKa of 7.3 ± 0.1 and Vmax of 167.0 ± 3.8% for LV. D, pH dependence of HC-3-specific binding was measured in 10 nM [3H]HC-3 for 30 min (n = 6–8). pKa of 7.8 ± 0.1 and maximum binding (Bmax) of 328.0 ± 10.0% for WT. pKa of 7.7 ± 0.2 and Bmax of 283.6 ± 17.8% for LV.
Na+ and Cl– dependence of the choline-induced current at different pH
To further investigate possible pH mechanisms, we measured the effect of protons on choline-induced current under different ionic conditions. Figure 8A shows the effect of pH on the induced current as a function of choline concentration. Whereas the apparent affinity for choline changes only weakly with pH, Imax changes dramatically. Furthermore, Imax changes in <30 s (limited by the solution exchange), which is too fast for insertion of transporters into the membrane. This is consistent with biotinylation data, which reveal no change in transporter surface expression at any pH (data not shown), suggesting that pH affects the catalytic activity of individual transporters already in the membrane. Figure 8, B and C, shows the Na+ and Cl– concentration dependence of the choline-induced current at different pH. Striking differences are evident: whereas the choline-induced current depends linearly on Na+ at concentrations <100 mM (Fig. 8B), Cl– dependence saturates in this range (Fig. 8C), with half-maximal Cl– concentration in the range of 15–35 mM. Figure 8D summarizes the pH-dependent currents for Na+ and Cl– on normalized scales, showing that Na+ or Cl– stimulation of the choline-induced current has the same concentration dependence at any pH. Furthermore, the Na+ and Cl– dependences for induced current are similar to Na+ and Cl– dependences for HC-3-specific binding (Fig. 8E,F). Thus, protons change Imax of choline-induced current but not Km for choline. Similarly, protons change the magnitude of choline-induced current and HC-3 binding titrated against Na+ or Cl– ions but not the shape of the curves.
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Figure 8. Effect of pH on Km and Imax. A, Km and Imax for choline-induced currents measured at different pH and held at –60 mV (n = 3). At pH 6.5, Km of 1.9 ± 0.3 µM and Imax of –3.8 ± 0.1 nA. At pH 7.4, Km of 0.9 ± 0.3 µM and Imax of –21.3 ± 0.4 nA. At pH 8.5, Km of 0.8 ± 0.2 µM and Imax of –32.3 ± 0.5 nA. LV-expressing oocytes were used. As a control, three water-injected oocytes were measured at each pH 6.5, 7.4, and 8.5. B, Na+ dependence of choline-induced current at various pH. In 10 µM choline, the induced current was measured at –60 mV, because LiCl replaced NaCl at different pH (n = 3). The Na dependence is linear at all pH. LV-expressing oocytes were used. C, Cl– dependence of choline-induced current at various pH (n = 3). In 10 µM choline, the induced current at –60 mV is measured at different pH (Na gluconate replacing NaCl). Results at 6.5 were insufficiently precise, although saturation clearly occurs. Km of 67.2 ± 22.5 mM and Imax of –3.8 ± 0.6 nA for pH 6.5. Km of 14.9 ± 3.4 mM and Imax of –16.7 ± 0.7 nA for pH 7.4. Km of 12.8 ± 1.7 mM and Imax of –25.0 ± 0.5 nA for pH 8.5. LV-expressing oocytes were used. D, Na+ and Cl– dependence of the choline-induced current do not depend on pH. Data from B and C are normalized for all pH and averaged. For Cl–, Km of 23.6 ± 5.8 mM and Imax of 122.2 ± 7.6%. E, Na+ dependence of HC-3 binding (n = 6–8). Na+ dependence of HC-3 binding is similar to that of choline-induced current (D). F, Cl– dependence of HC-3 binding (n = 6–8). Cl– dependence of HC-3 binding is similar to that of choline-induced current (D). Cl– dependence is fitted to a single-binding-site model. Km of 31.2 ± 3.8 mM and Bmax of 131.0 ± 4.8% for WT. Km of 17.5 ± 20.4 mM and Bmax of 126.4 ± 30.7% for LV.
Discussion
Choline transport is electrogenic with variable stoichiometry
From this study, choline transport is a voltage-dependent, electrogenic process with variable charge/choline stoichiometry (10 at –80 mV and 3 at –20 mV). Other members of the SLC5 family to which CHT belongs exhibit tight coupling and fixed stoichiometry, e.g., two Na+ ions per substrate molecule (Eskandari et al., 1997The LV mutant increases surface expression without altering WT properties
Stable hCHT WT expression is low in mammalian cells because hCHT is efficiently endocytosed from the plasma membrane (Ferguson and Blakely, 2004Constitutive leak currents through hCHT depolarize oocytes
The selective blocker HC-3 reveals a leak current through hCHT in the absence of choline. Simultaneous measurement of [22Na+] uptake and current demonstrated that leak currents in the related carrier rabbit SGLT1 are carried by Na+ ions (Mackenzie et al., 1998Cl– plays a regulatory role in choline transport
The reversal potential (45–60 mV, depending on choline concentration) (Figs. 1B, 3B) suggests that choline-induced current is Na+ selective; the Nernst potential for Na+ is 40 mV, assuming external Na+ of 100 mM and internal Na+ of 22 mM in oocytes (Kusano et al., 1982Possible pH regulation mechanism
Neurotransmitter transporter pH dependence is well studied in rSERT (Cao et al., 1997Proton inactivation hypothesis of hCHT in synaptic vesicles
Recent immunogold staining data (Ferguson et al., 2003Because vesicles deliver CHTs to the plasma membrane according to need, the question arises whether they are functional in the vesicle; in particular, are CHTs barred from leaking ACh and possibly protons from this compartment. Acidic inactivation of CHTs may provide the mechanism that prevents such leakage from synaptic vesicles in cholinergic neurons. The distribution of transporters on synaptic vesicles has also been observed for glycine transporters (Geerlings et al., 2001
Footnotes
Received May 2, 2006; revised Aug. 11, 2006; accepted Aug. 11, 2006.This work was supported by National Institutes of Health Grants MH-73159 (R.D.B.) and NS-34075 (L.J.D.F.) and an Alzheimer's Association Zenith Award (R.D.B.). We gratefully acknowledge Dr. Alicia Ruggiero for providing us with the hCHT LV mutant and assistance with the biotinylation studies. We also thank Hongping Yuan for plasmid preparations and Drs. Keith Henry, Maureen Hahn, Dawn Matthies, Chongbin Zhu, and Uhna Sung, Katrina Brewer, and Prof. Yuanmou Liu for their help with this project.
Correspondence should be addressed to Dr. Louis J. De Felice, Department of Pharmacology, Center for Molecular Neuroscience, 7130 Medical Research Building III, Vanderbilt University Medical Center, 465 21st Avenue South, Nashville, TN 37232-8548. Email: lou.defelice{at}vanderbilt.edu
Copyright © 2006 Society for Neuroscience 0270-6474/06/269851-09$15.00/0
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