Abstract
The endogenous volume-regulated anion channel (VRAC) from HEK293 cells was pharmacologically characterized using the whole-cell patch-clamp technique. Under isotonic conditions a small (1.3 nS), Ca2+-independent Cl conductance was measured. However, swelling at 75% tonicity activated a VRAC identified as an outward-rectifying anion current (P l > P Cl > P gluconate), which was ATP-dependent and showed inactivation at positive potentials. Activation of this current followed a sigmoid time course, reaching a plateau conductance of 42.6 nS after 12–15 min (t 1/2 = 7 min). The pharmacology of this VRAC was investigated using standard Cl−-channel blockers (NPPB, DIDS, and tamoxifen) as well as a new group (acidic di-aryl ureas) of Cl−-channel blockers (NS1652, NS3623, NS3749, and NS3728). The acidic di-aryl ureas were originally synthezised for inhibition of the human erythrocyte Cl− conductance in vivo. NS3728 was the most potent VRAC blocker in this series (IC 50 = 0.40 µM) and even more potent than tamoxifen (2.2 µM). NS3728 accelerated channel inactivation at positive potentials. These results show that acidic di-aryl ureas constitute a promising starting point for the synthesis of potent inhibitors of VRAC.
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Introduction
Volume-regulated anion channels (VRACs) comprise a class of chloride channels that contribute to the experimental regulatory volume decrease (RVD) response: Acute cell swelling in hypotonic media is counteracted by increased Cl− and K+ effluxes, which osmotically drive water efflux and restore cell volume (Hoffmann & Simonsen, 1989). Functional expression of VRACs seems to correlate closely with cell proliferation and migration in many cell types, possibly reflecting the need for subtle volume control during these processes. It has been suggested that VRAC inhibitors are anti-angiogenic agents having a therapeutic potential in cancer treatment (Chou, Shen & Wu, 1995; Voets et al., 1995; Shen et al., 2000; Ransom, O’Neil & Sontheimer, 2001; Wondergem et al., 2001). However, in vivo validation of this concept suffers strongly from the lack of non-toxic and metabolically stable blockers of VRACs.
In whole-cell patch-clamp experiments, VRACs are identified as a swelling-activated, outward-rectifying anion conductance with an Eisenman type I halide selectivity sequence. Despite years of investigation, the molecular nature of VRACs remains elusive, and it is questionable if it represents a single entity or a family of channels. The family of mammalian ClC channels was cloned in continuation of the identification of the skeletal muscle Cl− channel (ClC-0) from Torpedo electroplaques, where it is highly expressed. Several genes, including ClC-2 and ClC-3, have been considered as the molecular correlate of the VRAC (Duan et al., 1997; Grunder et al., 1992; Paulmichl et al., 1992). However, it is now widely assumed that VRACs belong to a distinct family. One problem with Cl− channels in general and VRACs in particular is the lack of selective high-affinity blockers, such as peptide constituents of animal or plant venoms to be used as tools in the purification and cloning process. A number of small organic molecules with VRAC blocking properties have been described, but they are neither very potent nor selective.
In the present paper a novel class of simple, small molecule compounds (acidic substituted di-aryl-ureas) is compared with the classical Cl− channel blockers DIDS, NPPB, and tamoxifen. The experiments were performed using VRACs endogenously expressed in HEK293. NS1652 and NS3623 have previously been shown to exhibit a potent block of the human erythrocyte Cl− conductance in vitro. Furthermore, NS3623 has been tested in a transgenic mouse model for sickle cell anemia, where it blocked the erythrocyte Cl− conductance in vivo and stabilized erythrocyte volume after oral administration (Bennekou et al., 2000, 2001). NS3749 and NS3728 are new compounds but belong to the same structural class as NS3623. The compounds NS1652, NS3623, NS3749 and NS3728 inhibited the VRAC with IC 50s of 97 µM, 1.8 µM, 1.4 µM and 0.40 µM, respectively. The structure–activity relation (SAR) of these four NeuroSearch (NS) compounds on the VRAC is distinct from the SAR obtained for the human erythrocyte Cl− conductance, indicating that the activities can be separated. The observations may serve as a starting point for the synthesis of selective VRAC blockers as tools for cloning as well as for development of anti-angiogenesis drugs for in vivo proof-of-concept investigations.
Materials and Methods
CELL CULTURE
HEK293 cells (ATCC CRL-1573) were cultured in DMEM medium supplemented with 10% fetal calf serum and 2 mM Glutamax (Gibco, BRL). The cells were grown at 37°C in a humidified atmosphere of 5% CO2 and 95% air. Cells were cultured in T25 flasks (Nunc) and when confluency reached 70–80%, the cells were trypsinized and seeded at 10–20% density in culture flasks or in Petri dishes containing the coverslips (Ø = 3.5 mm) used for the experiments.
ELECTROPHYSIOLOGY
All experiments were performed in the patch-clamp whole-cell configuration. For the pharmacological experiments, cover slips containing HEK293 cells were transferred to a custom-made experimental 15 µl recording chamber, positioned on an Olympus microscope (IX-70), and perfused with solution at a rate of 1 ml/min. For the ion-selectivity experiments a larger commercial chamber (RC-25F, Warner Instruments, Hamden, CT) was used. The reference electrodes consisted of an Ag/AgCl pellet that was connected via an agar salt bridge in the selectivity studies. Pipettes were pulled from borosilicate glass (Modulohm, Denmark) with a DPZ electrode puller (Zeitz Instruments, Germany) and placed in an electrode holder at the headstage of an EPC-9 amplifier (HEKA electronics, Germany). The EPC-9 amplifier was connected to a Macintosh G4 computer via an ITC-16 interface. Data was sampled at 3 times the filter cut-off frequency (3 kHz) with Pulse (HEKA electronics, Germany) and analyzed with IGOR software (WaveMetrics, Lake Oswego, OR). The pipettes, positioned by aid of a remotely controlled micromanipulator (Eppendorf, Germany), had a resistance of 1.5–3 MΩ when filled with the intracellular solution. The electrodes were zeroed just before touching a cell. Capacitative transients were automatically cancelled after establishment of the gigaseal, and again after entering the whole-cell configuration. The series resistance (R S) recorded after breakthroughs to the whole-cell configuration were in the range of 2.5–5 MΩ. R S was compensated 80%, updated between applications of voltage protocols, and never exceeded 8 MΩ. Currents were recorded either by application of a voltage step protocol from −100 to +100 mV with 20-mV step increases (from a holding potential of 0 mV; 200 ms duration) or by application of symmetric voltage ramps applied every 5 s (either ±100 or ±70 mV, 200 ms duration, see legends). Two isotonic extracellular solutions were used. The TEA-Cl solution contained (in mM): TEA-Cl (tetraethylammonium chloride) 142, CaCl2 2, MgCl2 1, and Tris 10 (pH 7.4) was primarily used for the investigation of the small background anion conductance in order to minimize all cation conductances and to avoid a possible Cl-channel block by HEPES. The TEA solution also allowed VRAC activation, but in this paper a slightly more physiological NaCl/CsCl solution was used. This solution contained (mM): NaCl 140, CsCl 4, CaCl2 2, MgCl2 1 and HEPES 10 (pH 7.4). For the ion-selectivity studies, NaCl was substituted with a corresponding concentration of NaI or Na-gluconate. The osmolalities of all extracellular solutions were in the range 280–300 mOsm when measured at The Advanced™ Osmometer (model 3D3, Advanced Instruments, Norwood, MA). The hypotonic solutions were made by adding water (0.25v:0.75v) to the isotonic solutions. All extracellular solutions were adjusted to pH 7.4 before use. The intracellular solutions used in the pipettes contained either 100 nM free calcium with (in mM): CsCl 110, Tris 10, EGTA 10, and CaCl2 5.17, or 1 µM free calcium with CsCl 110, Tris 10, EGTA 1, and CaCl2 0.955. Mg-ATP (4 mM) was added and the pH was adjusted to 7.20 with CsOH before use. The final Cs+ concentration was 147 mM. The measured tonicity of the final intracellular solutions was in the same range as that of the extracellular solutions. The free calcium concentrations were calculated by Eqcal Software (Biosoftware, Cambridge, UK), taking into account the stability constants for all Ca2+-, Mg2+-, and H+-binding ligands in the intracellular solution.
All compounds used were dissolved in 100% DMSO; except DIDS, which was dissolved in distilled water. The compounds were then diluted in the hypotonic solution to the required concentration. The final DMSO concentration did not exceed 0.1%, a concentration range without effect on the recorded currents. For all compounds concentration-response curves were established. Each compound was tested 2–8 times at each of the 4–8 different concentrations used. The mean I c/I 0 ±SEM was plotted as a function of the concentration and these data points were used in the fitting routine. The IC 50 values were calculated at −100 and +100 mV or −70 and +70 mV in order to address the question whether the block showed any voltage dependency.
ERYTHROCYTE EXPERIMENTS
Experiments were performed as previously described (Bennekou et al., 2000, 2001). In short, washed erythrocytes were suspended in a buffer-free extracellular salt solution containing the protonophore CCCP to monitor the erythrocyte membrane potential as change in the extracellular pH. With increasing concentrations of Cl-conductance blockers, valinomycin-induced hyperpolarizations were augmented and the fractional decrease in Cl conductance was calculated.
FITTING PROCEDURES AND CALCULATIONS
IC 50 values were calculated from equilibrium concentration-response experiments. Data were fitted to a Hill equation of the following form:
using a non-linear routine (Simplex). I o is the unblocked current level, I c is the stationary current level at the blocker concentration C, IC 50 is the concentration giving 50% block and n is the Hill coefficient. The erythrocyte data were fitted to a similar equation.
For calculation of permeability ratios from shifts in reversal potentials (V r) the following equation was used (Nilius et al., 1999):
where C is the concentration of anion (Cl or X) in the normal (n) or, respectively, the substituted (s) hypotonic solution. The reversal potential of the gluconate solution was corrected for a measured liquid junction potential of 4.5 mV.
CHEMICALS
DIDS (4,4-Diisothiocyanatostilbene-2,2-disulphonic acid), NPPB (5-Nitro-2-(3-phenyl-propylamino)-benzoic acid) and tamoxifen ((Z)-[4-(1,2-diphenyl-1-butenyl)phenoxy]-N,N-dimethylethanamine) were purchased from Sigma. NS1652 (2-[3-(3-trifluoromethyl-phenyl)-ureido]-benzoic acid), NS3623 (N-[4-bromo-2-(1H-tetrazol-5-yl)-phenyl]-N′-(3-trifluoromethyl-phenyl) urea), NS3749 (N-[4-Bromo-2-(1H-tetrazol-5-yl)-phenyl]-N′-(4-nitro-phenyl) urea) and NS3728 (N-[3,5-Bis(trifluoromethyl)-phenyl]-N′-[4-bromo-2-(1H-tetrazol-5-yl)-phenyl] urea) were synthesized at NeuroSearch A/S (Pederstrupvej 93, Ballerup, Denmark); for details see Christophersen & Pedersen, 1997, 1998; Dahl & Christophersen, 2000. Both the carboxylic acid compound (NS1652) and the tetrazoles (NS3623, NS3749, and NS3728) are acidic compounds (for a discussion of tetrazole chemistry, see Benson, 1947). Calculated pKA values (ChemSketch, Advanced Chemistry Developments, Toronto, Canada), were 3.5 for NS1652 and 3.9 for the other NS-compounds.
All inorganic salts and buffer substances were from various commercial dealers and were of analytical grade or higher.
STATISTICS
Data are presented as mean ± SEM of n experiments and, where appropriate, have been analyzed using Student’s t-test.
RESULTS
EVIDENCE OF VRAC EXPRESSION IN HUMAN EMBRYONIC KIDNEY CELLS (HEK293)
HEK293 cells express small whole-cell currents and are often chosen for heterologous expression of ion channels. Under conditions of blocked cation conductances (Fig. 1 A) the I-V relation of the basal current was slightly outward-rectifying and reversed at −2 mV, which is in good agreement with the equilibrium potential for chloride (−5 mV). At 100 mV the normalized mean current was 8.3 ± 0.1 pA/pF (n = 21, Fig. 1 B), corresponding to 98 ± 14 pA in a typical cell (12.0 ± 0.9 pF). These currents did not show any time dependency, as would have been expected for a voltage-dependent channel (Fig. 1 A) and the non-linearity thus probably results from instantaneous open-channel rectification. With 1 µM free Ca2+ in the pipette solution, the currents were similar to those obtained with 100 nM free Ca2+ (Fig. 1 B). We conclude that HEK293 cells do not express a significant number of Ca2+-activated Cl−-channels.
In contrast, by exposing the clamped HEK293 cell to a hypotonic extracellular solution (~220 mOsm compared to ~290 mOsm in the control NaCl/CsCl solution) a large increase in the conductance was observed (Fig. 2). The I-V relation measured from the step protocol shows that the swelling-induced current also exhibited instantaneous outward rectification, but at variance to the basal current it showed clear inactivation at potentials more positive than +40 mV. Some experiments were done without Mg-ATP in the pipette solution, which completely abolished the swelling-induced augmentation of the chloride conductance (data not shown). To establish the basic anion selectivity of the swelling-induced current, the permeability ratios of the iodide ion and gluconate vs. the chloride ion were established (Fig. 3 A). For these studies the voltage protocol was changed from the step protocol employed in the experiments shown in Figs. 1 and 2 to a voltage-ramp protocol: A voltage ramp running from −70 mV to +70 mV in 200 ms was applied from a holding potential of 0 mV every 5 seconds (Fig. 3, inset). In the NaCl/CsCl solution a reversal potential of 6 ± 1 mV (n = 6) was recorded (theoretical E Cl = 2 mV). Upon equimolar exchange of the extracellular Cl− with I− or gluconate (10 mM Cl− remaining), distinct shifts in the reversal potentials towards more negative (ΔV r = −8 ± 0.4 mV, n = 6), respectively positive potentials (ΔV r = 37 ± 3 mV, n = 4), occurred. The observed changes in the reversal potentials correspond to a P I/P Cl of 1.4 and a P gluconate/P Cl of 0.18. Overall these characteristics are similar to those found for volume-regulated anion channels (VRACs) in other cell types and the channel is thus referred to as VRAC in the subsequent paragraphs.
The development of VRAC current as a function of time was established (Fig. 3 B). After obtaining the whole-cell configuration, the ramp currents were recorded in isotonic solution during 3 minutes before application of the hypotonic solution. The current typically started to increase about 1 minute after the exchange of the solution and reached a plateau after about 12–15 minutes (t 1/2 = 7 min). The plot of the mean current (measured at +100 mV) reveals a smooth, sigmoid, time-dependent activation curve, which may reflect cooperativity in the activation process of VRACs. In the hypotonic solution, the current at +100 mV reached 735 ± 44 pA/pF (n = 55) and at −100 mV it was approximately 2/3 smaller (251 ± 14 pA/pF).
PHARMACOLOGICAL CHARACTERIZATION OF VRACS IN HEK293 CELLS
For the pharmacological characterization of the VRACs in HEK293 cells the voltage-ramp protocol was used. Figure 4 A shows the traces obtained in NaCl/CsCl (control; C) solution and in the hypotonic NaCl/CsCl solution (VRAC). In all pharmacological experiments the following procedure was followed: After a stable VRAC current was achieved, the hypotonic solution was changed to a hypotonic solution containing the desired concentration of the compound in question. When a new plateau current level was obtained, the compound was washed off by superfusion with the hypotonic solution alone. An example is shown in Fig. 4 B, where the time course of VRAC activation (measured at −100 mV and at +100 mV from the ramp protocol) was measured and where DIDS and NPPB were tested. The cell was exposed to the hypotonic solution, as indicated by the solid bar, and during the periods indicated by open bars, the Cl− channel blockers DIDS (30 µM) and NPPB (30 µM) were sequentially included in the hypotonic solution. DIDS reduced the current by 43 ± 8% (n = 6) at +100 mV (Fig. 4 B), whereas no effect was observed at −100 mV, indicating a voltage-dependent action by DIDS. In contrast, NPPB reduced the inward and the outward currents to a similar degree (51 ± 22% at −100 mV and 44 ± 21% at +100 mV, respectively (n = 4)). Although the percentage of inhibition for both compounds was similar, DIDS reached steady state faster than NPPB. The effects of both compounds were completely reversible and the recovery showed similar differences in the kinetics as did the inhibition: faster for DIDS than for NPPB.
Figure 5 compiles the results obtained with the reference compounds. Figure 5 A shows I-V ramps in the control situation and after application of a partially effective concentration of blocker. All compounds were tested at 5–7 concentrations and concentration–response curves were generated (Fig. 5 B) based on current recordings at −100 mV as well as +100 mV in order to elucidate any possible voltage-dependent effects on affinity and/or Hill coefficients. The solid curves represent the best fit to Eq. 1. DIDS inhibited the VRACs with an IC 50 value of 26 µM at +100 mV and 256 µM at −100 mV. The ten-times difference in the IC 50 values represents the voltage-dependent block of this compound, whereas the Hill coefficient for inhibition by DIDS was independent of voltage (0.8 ± 0.1 at +100 mV and 0.9 ± 0.1 at −100 mV). In contrast, NPPB had similar IC 50 values at +100 and −100 mV (21 and 27 µM, respectively) and the Hill coefficient was 1.4 ± 0.2. Finally, tamoxifen was tested. It is an anti-estrogen compound that is extensively used for the treatment of breast cancer. However, it is also a Cl−-channel blocker that has been used in studies of swelling-activated currents and related effects. Interestingly, the compound does exhibit some selectivity among VRACs from different cells. In most cases it is very potent (Wondergem et al., 2001; Chen et al., 2002) but in some cells it has no effect (Winpenny et al., 1996. Leaney, Marsh & Brown, 1997; Mitchell et al., 1997). Therefore, it is important to profile the VRACs expressed in HEK293 cells with respect to tamoxifen sensitivity. With an IC 50 value of 2.2 µM at +100 mV, tamoxifen was by far the most potent reference compound tested, and definitively categorized the HEK293 VRACs as tamoxifen-sensitive. The inhibition by tamoxifen did not show any voltage dependency (IC 50 = 2.6 µM at −100 mV) and the Hill coefficient was 1.3 ± 0.1.
INHIBITION OF VRACS BY SUBSTITUTED DI-ARYL-UREAS
Figure 6 A, B, C and D show representative effects of the various acidic di-aryl-ureas (NS1652, NS3623, NS3749 and NS3728) on VRAC ramp currents. Full concentration–response curves are plotted in Fig. 7. Obviously, NS1652, a carboxy derivative, is much less potent than the tetrazole derivatives NS3623, NS3749 and NS3728. At +100 mV, NS1652 blocks with an IC 50 of 97 µM, whereas NS3623, NS3749 and NS3728 inhibited the VRAC current with IC 50 values of 1.8 µM, 1.4 µM and 0.40 µM, respectively. Like NPPB and tamoxifen, the substituted di-aryl-ureas exhibited only modest, if any, voltage dependency (Table 1) and the Hill coefficients were close to 1.
The affinity of both reference and NS compounds were also tested on the erythrocyte Cl conductance for comparison with the VRAC effect. Hyperpolarizations induced by addition of valinomycin to suspensions of erythrocytes were augmented by sub-micromolar concentrations of DIDS and all NS compounds, whereas no effect of tamoxifen and NPPB was observed at 20 µM. Table 1 shows the obtained IC 50 values.
Finally, in order to elucidate a possible effect on voltage-dependent channel inactivation by this new class of compounds, a swollen cell was voltage-clamped at −50 mV and the inactivation was induced by a 200 ms step to 80 mV (Fig. 8 A). Application of 1 and 3 µM NS3728, the most potent compound, reversibly and dose-dependently (Fig. 8 B and C) reduced both inward and outward currents, as expected. To high-light the effect on the channel inactivation, the peak amplitudes of the current traces obtained with blocker were rescaled to the peak of the control trace (Fig. 8 B, left panel). Clearly, NS3728 dose-dependently accelerate voltage-dependent inactivation. Note also that the compound prolonged the time needed for recovery from inactivation (compare traces at −50 mV). From these experiments, we conclude that NS3623, NS3749 and NS3728 represent a new class of compounds that potently block VRACs in a voltage-independent and reversible manner.
Discussion
HEK293, a standard laboratory cell line, was investigated for endogenous expression of functional Cl− channels by the whole-cell patch-clamp technique. Using extracellular and intracellular salt solutions, where the physiological relevant cations Na+ and K+ were exchanged with the impermeant TEA+ and Cs+, only a small Ca2+-independent, outward-rectifying background Cl− conductance was isolated. Absence of Ca2+-activated Cl− channels in HEK293 cells has previously been reported in a single-channel study by Zhu et al. (1998) and HEK293 cells have frequently been used for heterologous expression of proteins suggested to be calcium-activated chloride channels (Gruber et al., 1998; Fuller & Benos, 2000; Leverkoehne & Gruber, 2002).
In contrast, volume-regulated anion channels (VRACs) were abundently expressed. Upon swelling in hypotonic (75%) solution the currents activated with a sigmoid time dependence and reached a stable plateau level after about 10 min. During the swelling the total cell conductance (at 0 mV) increased from 1.3 ± 0.1 nS to 43 ± 3.1 nS (n = 55) as a consequence of channel activation. The VRACs were outward rectifiers exhibiting distinct inactivation at large positive potentials. Exchanging the extracellular solution to iodide- or gluconate salts showed that I− was slightly more permeable than Cl− (1.4 times) and that gluconate was considerably less permeable (0.18 times). These values are consistent with previously published values of VRACs from other cells (e.g., Voets et al., 1997). Intracellular ATP was an absolute requirement for channel activation.
The sigmoid time dependency of activation might solely indicate internal subunit conformational changes during activation. Thus the volume-dependent gating can in principle be modeled according to a classical cooperative model for channel activation. However, previous investigations on the mechanisms of activation of VRACs strongly points towards a very complicated sequence of events and the apparent cooperativity could also include elements of the activation cascade. This seems to involve the rho/rho-kinase pathway, permissive sub-micromolar concentrations of intracellular Ca2+, as well as structural elements such as cytoskeleton and compartmentalization of signaling molecules in membrane caveolae (Szucs et al., 1996; Okada, 1997; Trouet et al., 1999, 2001, for reviews see Shaul & Anderson, 1998 and Eggermont et al., 2001).
The HEK293 VRACs were characterized pharmacologically using the standard Cl− channel blockers DIDS, NPPB and tamoxifen as well as NS1652, NS3623, NS3749 and NS3728, which establish a new class (substituted acidic di-aryl-ureas) of Cl−-conductance blockers. DIDS exhibited a pronounced voltage-dependent inhibition of the VRACs, blocking outward currents more than inward currents. However, the effect was clearly concentration-dependent and detailed analysis of the concentration–response curves revealed that the voltage dependency could be ascribed entirely to an effect on the affinity of the block (IC 50 = 26 µM at +100 mV vs. 256 µM at −100 mV) rather than changed Hill coefficients (n H = 0.8 ± 0.1 at +100 mV vs. n H = 0.9 ± 0.1 at −100 mV). In contrast, NPPB and tamoxifen both blocked voltage-independently, with tamoxifen being the most potent (21 µM vs. 2.2 µM). The di-aryl-ureas tested in this study were voltage-independent, reversible blockers of VRACs. In this series the most potent compound was NS3728 (0.40 µM), NS3623 and NS3749 were equipotent (1.8 µM and 1.4 µM, respectively), whereas NS1652 was a poor blocker (97 µM). NS3728 exhibited a distinct accelerating effect of the voltage-dependent inactivation of VRAC. NS1652 and NS3623 have previously been described as potent sub-micromolar blockers of the human erythrocyte Cl− conductance (molecular identity uncertain) and were suggested to have potential in the prevention of red blood-cell dehydration in sickle-cell patients (Bennekou et al., 2000, 2001). The erythrocyte G Cl block by the acidic di-phenyl-urea compounds was confirmed in the present study and further exemplified by the effect of NS3749 and NS3728. It is noteworthy that NS1652 is a relatively weak blocker of VRACs, whereas NS3623, NS3749 and NS3728 retain a high potency on this channel, meaning that the human erythrocyte Cl− conductance and the VRACs carry different molecular entities at the blocker site. In various cell types, VRACs have been shown to be inhibited by numerous different chemical structures, being only remotely related to each other: A structural unifying concept of the classical Cl−-channel blockers like NPPB, niflumic acid, and DIDS is that they are di-aromatic, 2-substituted acids linked by various chains. However, hitherto this chemical class has not produced very potent VRAC blockers. Tertiary amines, like tamoxifen and verapamil and various phenol-derivatives like gossypol (for a review, see Nilius et al., 1999) are also VRAC blockers and the most potent entities are found in these groups. For compounds containing an alkaline nitrogen it has been argued that the uncharged form of the molecules inhibit the channel (Voets, Droogmans & Nilius, 1996; Maertens et al., 2001), possibly indicating that the binding site for these compounds is exposed to the lipid phase of the membrane.
The fact that VRACs are blocked by structurally very different compounds raises the concern that some of the effects may be indirectly caused by interference with diverse levels in the activation cascade. However, since the di-aromatic substituted acids are all nearly 100% negatively charged at pH = 7.4 (pK A values usually 3–4, see Materials and Methods), it is tempting to assume that the negative group mimics an anion that would normally pass through the channel. Therefore, these compounds probably interact with the pore region, perhaps even with residues near the selectivity filter. This is consistent with the fact that we find instantaneous voltage-dependent blockers (i.e., DIDS) in this group. It is also possible that the increased rate of voltage-dependent inactivation, shown for niflumic acid and NPPB (Voets et al., 1997) and for NS3728 (present study), may reflect blocker exclusion of ions from an externally-facing, gating-regulatory site in the permeation pathway.
The main problem with the standard acidic di-aryls known and characterized as Cl−-channel blockers so far is their very low potency, usually ranging from 10–1000 µM, which makes them very bad tools for VRAC purification and completely excludes them as in vivo active drugs. The new compounds shown here are chemically different from the classical Cl− blockers in two important aspects: 1) They use the tetrazole moiety as acidic group rather than carboxylic or sulfonic acid groups and 2) they carry the urea moiety as a linker between the two aromatic centers of the molecule. This combination produces compounds that are significantly more potent VRAC blockers than the standard compounds and the results obtained with NS3728 give promise that further optimization will reveal low-nM-potency VRAC blockers. A systematic study on the structure–activity relationship for potency, voltage dependency and inactivation of block is urgently needed to explore this further.
It has previously been shown (Bennekou et al., 2000, 2001) that NS3623 has good in vivo pharmaco-dynamic properties, i.e., long-lasting erythrocyte Cl−-conductance block upon single oral doses and normalization of sickle-cell volume in normal and transgenic mice as well as low toxicity (3 weeks dosing). Further, NS3623 exhibited no activity (10 µM) on 60 different receptor-binding assays, including vascular endothelial growth factor (VEGF). This is promising for the structurally related new potent blocker of VRACs, NS3728, and this compound or a close analogue may be valuable in the elucidation of the role of VRACs as a pharmaceutical target for inhibition of angiogenesis and cancer in vivo.
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Acknowledgements
Vibeke Meyland-Smith is gratefully acknowledged for her expert assistance with patch-clamp electrophysiology. N. Helix was financed by the European Community via the Marie Curie Industrie Host Fellowship (QLK-CT-2000-60044).
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Hélix, N., Strøbaek, D., Dahl, B. et al. Inhibition of the Endogenous Volume-regulated Anion Channel (VRAC) in HEK293 Cells by Acidic Di-Aryl-Ureas . J. Membrane Biol. 196, 83–94 (2003). https://doi.org/10.1007/s00232-003-0627-x
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DOI: https://doi.org/10.1007/s00232-003-0627-x