Abstract
Aquaporins are known as water channels; however, an additional ion channel function has been observed for several including aquaporin-1 (AQP1). Using primary cultures of rat choroid plexus, a brain tissue that secretes CSF and abundantly expresses AQP1, we confirmed the ion channel function of AQP1 and assessed its functional relevance. The cGMP-gated cationic conductance associated with AQP1 is activated by an endogenous receptor guanylate cyclase for atrial natriuretic peptide (ANP). Fluid transport assays with confluent polarized choroid plexus cultures showed that AQP1 current activation by 4.5 μm ANP decreases the normal basal-to-apical fluid transport in the choroid plexus; conversely, AQP1 block with 500 μm Cd2+ restores fluid transport. The cGMP-gated conductance in the choroid plexus is lost with targeted knockdown of AQP1 by small interfering RNA (siRNA), as confirmed by immunocytochemistry and whole-cell patch electrophysiology of transiently transfected cells identified by enhanced green fluorescent protein. The properties of the current (permeability to Na+, K+, TEA+, and Cs+; voltage insensitivity; and dependence on cGMP) matched properties characterized previously in AQP1-expressing oocytes. Background K+ and Cl− currents in the choroid plexus were dissected from AQP1 currents using Cs-methanesulfonate recording salines; the background currents recorded in physiological salines were not affected by AQP1–siRNA treatment. These results confirm that AQP1 can function as both a water channel and a gated ion channel. The conclusion that the AQP1-associated cation current contributes to modulating CSF production resolves a lingering concern as to whether an aquaporin ionic conductance can have a physiologically relevant function.
- CSF
- cyclic nucleotide-gated channel
- major intrinsic protein
- atrial natriuretic peptide
- patch-clamp electrophysiology
- small interfering RNA
Introduction
Aquaporin-1 (AQP1) channels in the major intrinsic protein (MIP) family mediate water movement across membranes in the brain, kidney, vascular system, and other tissues (Agre et al., 1993; King and Agre, 1996). AQP1 is abundant in the choroid plexus, a tissue bordering brain ventricles that produces CSF by active Na+ transport and concomitant water flux from blood to brain (Wright and Saito, 1986; Speake et al., 2001). Atrial natriuretic peptide (ANP) receptors in choroid plexus epithelia couple to guanylate cyclase, stimulating cGMP generation (Tsutsumi et al., 1987; Israel et al., 1988) and inhibiting CSF production (Steardo and Nathanson, 1987). AQP1 has been found to have a cGMP-gated cation channel function (Anthony et al., 2000; Saparov et al., 2001), but its physiological relevance has remained unclear. We confirmed ion channel function of AQP1 and tested for possible physiological relevance for CSF production in rat choroid plexus primary cultures.
Although the ion channel function of AQP1 initially was questioned (Agre et al., 1997), the simplest interpretation of all the evidence now in hand is that AQP1 directly mediates a gated cationic current (Yool and Stamer, 2002). Other members of the aquaporin family such as AQP6 (Yasui et al., 1999; Liu et al., 2005) and Drosophila Big Brain (Yanochko and Yool, 2002, 2004) also function as ion channels when expressed in oocytes but differ in mechanisms of activation and ionic selectivities, ruling out a simple explanation as endogenous oocyte ion channels. The lens AQP0 protein shows ion channel function in reconstituted bilayers (Zampighi et al., 1985; Ehring et al., 1990, 1992), although a physiological role for the conductance in the eye remains to be determined.
Modulatory contributions from proteins in signaling complexes with AQP1 (Cowan et al., 2000; Abu-Hamdah et al., 2004; Kelly et al., 2005) seem likely given the tissue-specific variability in channel properties, a concept that might also apply to other aquaporins. Opening probabilities for cGMP-gated AQP1 ion channels expressed in oocytes or reconstituted in bilayers are exceptionally low (Saparov et al., 2001; Yool and Weinstein, 2002) and undetectable in AQP1-transfected HEK cells (Tsunoda et al., 2004). Differences among these studies suggested that AQP1 ion channel activity might depend on the expression system, perhaps involving differentially expressed unidentified factors. We hypothesized that the appropriate conditions for full functionality might best be seen for AQP1 expressed in a native tissue.
Results here confirm that natively expressed AQP1 is a cGMP-gated ion channel activated by ANP and that activation decreases fluid transport across confluent choroid plexus in culture. Selective loss of the cGMP-stimulated cationic current after two methods of AQP1–small interfering RNA (siRNA) treatment confirms that the conductance cannot be attributed to other endogenous ion channels in the choroid plexus (Hung et al., 1993; Speake et al., 2001, 2004). Our data are the first to show ion channel function in a native aquaporin and suggest the promise that aquaporin ionic conductances have physiologically relevant functions in regulatory mechanisms of transmembrane fluid transport in brain and other tissues.
Materials and Methods
Primary culture.
Anesthetized 5-d-old Sprague Dawley rats were decapitated. Dissected lateral and fourth ventricle choroid plexi were triturated in Hanks’ solution with 0.25% trypsin. DMEM/Ham’s F-12 (1:1) medium with 10% (v/v) fetal bovine serum stopped enzyme activity; cells were filtered (100 μm), centrifuged (400 rpm; 15 min, 6°C), and resuspended in DMEM/Ham’s F-12 (1:1) containing 10% (v/v) fetal bovine serum, 4 mm l-glutamine, 5 μg/ml insulin, 1.0 U/ml penicillin, and 0.1 mg/ml streptomycin. Cells seeded on murine laminin (20 μg/ml) plates were maintained at 37°C in humidified 5% CO2. Cytosine arabinoside (20 μm) was applied through day 4 in culture. From day 5, cells were maintained in DMEM/Ham’s F-12 (1:1) medium (5% v/v fetal bovine serum), refreshed every 2–3 d. Culture supplies were from Invitrogen (Carlsbad, CA).
Immunocytochemistry.
Brains rapidly frozen in OCT medium were cryostat sectioned (17 μm), fixed (4% paraformaldehyde; 1 h), washed in 50 mm glycine buffer, pH 7.4, and blocked with 1% donkey serum in PBS (pH 7.4, 0.1% Triton X-100). The following primary antibodies were applied overnight: anti-AQP1 (rabbit polyclonal) (Stamer et al., 1995) at 400 ng/ml; or anti-prealbumin (goat polyclonal; Santa Cruz Biotechnology, Santa Cruz, CA) at 1:250. Slides were washed in blocking solution and incubated 2 h with secondary antibodies: fluorescein-conjugated donkey anti-rabbit IgG (1:100); or Cy5-conjugated donkey anti-goat IgG (1:200) (Jackson ImmunoResearch, West Grove, PA). Negative controls omitted primary antibodies. Sections were washed, mounted in Dako (Carpinteria, CA) medium, and viewed by confocal microscopy. Cultured cells on laminin-coated glass coverslips were fixed in MEM/HEPES, pH 7.0, containing 4% sucrose and 4% paraformaldehyde, washed in PBS (pH 7.4; 0.05% Triton X-100 and 5% donkey serum), and incubated with primary antibodies (as described above). After primary incubation, the cell cultures were washed with buffer (three times, 5 min each) and incubated for 1 h at room temperature with secondary antibodies. For double-staining experiments, the secondary antibodies used were the same as described for cryostat sections. For transfected cells, the secondary biotin-labeled donkey anti-rabbit antibody was used at 1:500 (for 1 h at room temperature) and washed three times with PBS (as above), and the cells were incubated for 30 min with Alexafluor555/streptavidin at 1:4000 in the dark at room temperature. Finally, the cells were washed in PBS solution, pH 7.4, and mounted for microscopic visualization.
Reverse transcriptase- PCR.
Total RNA was isolated from primary choroid plexus cultures (Qiagen kit; Qiagen,Santa Clarita, CA). After DNase digestion, reverse transcription was done using 2 μg of total RNA, 1 μg of random primer, 0.2 μg of oligodeoxythymidine primer, 40 U of RNase inhibitor, and 50 U of reverse transcriptase (Moloney murine leukemia virus; Boehringer Mannheim, Indianapolis, IN) in a 35 μl total volume (37°C, 1 h). Reverse-transcribed cDNA was used for PCR amplification with sequence-specific primers. For AQP1, the sequences were as follows: sense 5′-CCGAATTCATGGCCAGCGAGTTCAAGAAGAA-3′ (31–61 bp) and antisense 5′-CGGGGGTGTTATCCGGGGTGGGTCTTTTAGGTCAC-3′ (663–697 bp), for a product of 669 bp. For cyclophilin, the sequences were as follows: sense 5′-GGGGAGAAAGGATTTGGCTA-3′ and antisense 5′-GCCACTGTGGTCAGTGTCAT-3′, for a product of 259 bp. Each PCR amplification (50 μl final volume) contained 50 pmol of each primer, 0.2 mm each of deoxynucleotides, and 2.5 U of TaqDNA polymerase (Promega, Madison, WI). The reactions were performed in a PerkinElmer (Wellesley, MA) 9600 thermocycler using the following program: denaturation (94°C, 120 s), annealing (60°C, 90 s), and polymerization (72°C, 120 s) for 35 cycles, ending with 5 min at 72°C and storage at 4°C. For electrophoresis, 2 μl of PCR products were run on a 2% agarose gel (80 V, 2 h) and stained with ethidium bromide.
siRNA synthesis and transfection.
Two approaches were used for the RNA interference experiments. The first method used a mixture of siRNAs generated with the Dicer kit (Gene Therapy Systems, San Diego, CA). For this method, double-stranded RNA for AQP1 was synthesized in vitro with T3 and T7 RNA polymerases, from BamHI and HindIII-linearized human AQP1 cDNA (from P. Agre, Duke University, Durham, NC). As a control, a proprietary commercial mixture of siRNAs with “no significant similarity to any known gene sequences from mouse, rat or human” (Silencer Negative Control siRNA; Ambion, Austin, TX) was used. In the second method, sequence-specific siRNAs designated as AQP1-siRNA-a and AQP1-siRNA-b with matching scrambled controls were synthesized (Ambion) based on sequences demonstrated previously to selectively target AQP1 (Splinter et al., 2003).
The sequences used by Splinter et al. (2003) for AQP1 show no predicted cross-reactivity with other protein coding sequences in the choroid plexus; BLAST (Basic Local Alignment Search Tool) searches of the mammalian gene database with the targeted and scrambled sequences resulted in perfect matches exclusively for AQP1 for the sequence siRNA-a and predominantly for AQP1 for the sequence siRNA-b, with several related hits for partial homology with mouse TRAF-interacting protein. The two scrambled sequences showed partial matches predominantly with noncoding genomic DNA, with the exception of one hit for the scrambled-b sequence for partial homology with mouse vomeronasal 1 receptor. TRAF is a tumor necrosis receptor-associated factor (Rothe et al., 1994); TRAF6 is important in transcriptional regulation during CNS development in several specific brain regions not including telencephalon, thymus, and choroid plexus (Dickson et al., 2004). The vomeronasal organ receptors mediate detection of pheromones (Ryba and Tirindelli, 1997; Rodriguez et al., 2002; Halpern and Martinez-Marcos, 2003) but have not been described outside of the olfactory system, suggesting indirect effects of the scrambled siRNA sequence on the choroid plexus are unlikely.
For transfection, cells were plated on 35 × 10 × 12 mm laminin-coated glass-bottom dishes. Between days 4 and 11 in culture, cells were transfected using siPORT-Amine (Ambion) to introduce a plasmid carrying the enhanced green fluorescent protein (eGFP) marker (pEGFP-N1; 100 ng/250 μl; BD Biosciences Clontech, Palo Alto, CA), either alone or with siRNAs (AQP1–siRNA or scrambled sequences). The cells were incubated with the transfection complex for 4–5 h, then 1 ml of normal growth medium without antibiotics was added to each dish. Electrophysiological and immunocytochemical experiments were performed 2–3 d after transfection.
Electrophysiological recordings.
Patch-clamp experiments were performed in whole-cell and excised patch-clamp configurations. Extracellular solutions all contained (in mm) 1 CaCl2, 2 MgCl2, 10 glucose, and 5 HEPES, pH 7.3, and in addition contained 140 NaCl and 5 KCl for the “NaCl saline” and 125 Cs-methanesulfonate and 20 CsCl for the “CsMES saline.” The intracellular (pipette) solutions all contained (in mm) 2 MgCl2, 10 glucose, 5 HEPES, 0.5 EGTA, and 2 Na2ATP, pH 7.2, and in addition contained 120 K-gluconate and 20 KCl for the “KGluc saline,” 140 KCl for the “KCl saline,” 140 tetraethylammonium (TEA)-Cl for the “TEACl saline,” 120 Na-gluconate and 20 NaCl for the “Na Gluc saline,” and 135 Cs-methanesulfonate and 5 CsCl for the CsMES saline. Data were recorded (AxoPatch 200A; Molecular Devices, Foster City, CA) using Sylgard-coated pipettes (4–6 MΩ for whole-cell patches; 3–5 MΩ for excised patches). Data were filtered (2 kHz), digitized (10 kHz), and analyzed by pClamp 9 software (Molecular Devices). Whole-cell recordings were performed at 37°C; single-channel recordings were at room temperature. Sodium nitroprusside (SNP; Sigma, St. Louis, MO) prepared fresh daily in sterile water was kept on ice, light protected. Data are mean ± SEM unless stated otherwise. Statistical comparisons are noted in the text and legends.
Transepithelial flux measurements.
Primary cultures of choroid plexus epithelia were grown 14 d in vitro on porous 0.4 μm polycarbonate membranes (12-mm-diameter transwell plates; Costar, Cambridge, MA), using conditions as described for primary cultures above. One day before the flux assays, cells were fed with reduced-serum media [DMEM/Ham’s F-12 (1:1) supplemented with 0.5% (v/v) fetal bovine serum]. Confluence of monolayers was assessed by net transepithelial electrical resistances (TEERs) ≥50 Ohm cm2 (Zheng et al., 1998), measured using a TEER measurement chamber (ENDOHM-24; World Precision Instruments, Sarasota, FL) in conjunction with a volt-ohmmeter (EVOM; World Precision Instruments). After aspiration of media from apical and basolateral compartments of transwell plates, fluid transport assays began by adding 4000 μl of isotonic media [DMEM/Ham’s F-12 (1:1)] to the lower chamber (basolateral) and 50 μl to the upper chamber (apical). Fluid transport was measured at 2 h intervals as the volume of fluid accumulated against a hydrostatic head in the apical chamber, determined by analytical balance. Net fluid accumulation at the apical side was monitored before and after treatment with 4.5 μm ANP (applied basolaterally), in the presence and absence of 500 μm Cd2+ (applied apically).
Results
AQP1 is abundantly expressed in the choroid plexus in vivo and in vitro
In primary cultures of the choroid plexus isolated from postnatal day 5 rats, expression of AQP1 mRNA was confirmed by reverse transcription (RT)-PCR amplification (Fig. 1a). AQP1 protein is abundantly expressed in rat choroid plexus cells in vivo and in vitro, as detected by immunocytochemistry (Fig. 1b,c) with AQP1-specific polyclonal antibodies recognizing the C-terminal domain (Stamer et al., 1995). Coimmunolabeling with antibodies against prealbumin provided a specific marker for choroid plexus cells (Aleshire et al., 1983).
Transfection of cultured choroid plexus cells with siRNA against AQP1 dramatically decreased expression of AQP1 protein. siRNA-transfected cells were identified by cotransfection with a plasmid vector carrying eGFP (Fig. 1d–f). Control transfection of choroid plexus cells with the eGFP plasmid alone did not alter the expression of AQP1 protein (Fig. 1g,h). These data demonstrated that siRNA against AQP1 effectively knocked down protein expression in choroid plexus cells, confirming the molecular identity of the signal detected by RT-PCR and immunocytochemistry, as well as providing a useful tool for assessing the role of AQP1 in mediating cGMP-induced ionic currents (see below). The correct targeting of AQP1 to the apical membrane was confirmed for cultured choroid plexus cells using z-scanning confocal microscopy of control eGFP-transfected cells (Fig. 1i). The cytoplasmic eGFP fills the cell, whereas the signal for AQP1 is limited to the apical side of the cell.
Properties of SNP-induced ionic currents in choroid plexus cells
Selective activation of ionic current in cultured choroid plexus cells was recorded by whole-cell patch clamp after bath application of SNP, a nitric oxide donor that catalyzes the synthesis of intracellular cGMP. Endogenous K+ and Cl− currents known to be present in the choroid plexus (Garner and Brown, 1992; Kotera and Brown, 1994; Speake et al., 2001, 2002, 2004; Speake and Brown, 2004) were minimized by ionic substitution of NaCl and KCl with Cs-methanesulfonate, resulting in a low initial conductance before application of cGMP agonists (Fig. 2a). A robust SNP-dependent Cs+ current was activated in choroid plexus cells (Fig. 2a–c); the cationic current showed a linear voltage–current relationship and block by external Cd2+, demonstrating properties comparable to those described previously for cloned human AQP1 heterologously expressed in Xenopus oocytes (Anthony et al., 2000; Yool, 2002; Boassa and Yool, 2003).
Previous work demonstrated that AQP1 cationic channels expressed in oocytes are permeable to Cs+, Na+, K+, and, to a lesser extent, TEA+ with no appreciable Cl− permeability (Yool et al., 1996). Ionic substitution in the bath and pipette salines showed that the cGMP-dependent current in the choroid plexus is a nonselective cationic conductance with comparable relative permeabilities, as determined by comparison of the reversal potential with predicted equilibrium potentials for Cl− channels and nonselective cation channels (Fig. 2d). Predicted cationic reversal potentials were calculated based on the quantitative relative permeability values defined for AQP1 channels expressed in oocytes (Yool et al., 1996) and superimposed closely with the measured values in the choroid plexus.
The activation of ionic conductance in response to SNP was blocked effectively by the soluble guanylate cyclase inhibitor 1H-[1,2,4]oxadiazolo[4,3-a]quinoxalin-1-one (ODQ). Conversely, ODQ did not affect the conductance response to ANP, which activates an endogenous ODQ-insensitive receptor guanylate cyclase present in the choroid plexus (Fig. 2e). Thus, the SNP-stimulated ionic conductance is induced by generation of cGMP rather than by chemical modifications such as S-nitrosylation (Ahern et al., 2002). It is noteworthy that the cGMP-dependent conductance can be stimulated by an endogenous signaling pathway in the choroid plexus, a necessary feature of a potentially physiologically relevant response.
The conductance induced by ANP, recorded with Cs+ bath and pipette salines, showed properties comparable to those seen for the response induced by SNP. The ANP-evoked current showed a low initial conductance and an agonist-dependent non-voltage-sensitive current with a reversal potential consistent with cationic selectivity (Fig. 2f). The ANP response was not sensitive to the soluble guanylate cyclase inhibitor ODQ (Fig. 2g) and was blocked by Cd2+ (200 μm) (Fig. 2h).
Application of a cGMP agonist (8Br-cGMP) to the internal face of excised inside-out patches from choroid plexus cells resulted in the activation of a large-conductance channel (Fig. 3) measured in symmetrical Cs+ salines (chord conductance, 166 ± 3 pS; mean ± SD, n = 6 patches). The large-conductance channel showed properties of unitary conductance, long open-channel events, and dependence on cGMP similar to those described previously for AQP1 channels in oocytes (Anthony et al., 2000) and was blocked reversibly by 500 μm Cd2+ applied to the internal face of the patch. Two classes of small-conductance channels (∼20 and 50 pS) also were present in patches with and without 8Br-cGMP. In summary, 4 of 11 inside-out patches and 2 of 4 outside patches showed the large-conductance AQP1-like channel activity. These data support the hypothesis that the novel ion channel in the choroid plexus is AQP1; however, molecular confirmation was needed to rule out the possibility that another endogenous choroid plexus ion channel by coincidence showed the same set of properties.
AQP1 knockdown by siRNA eliminates the cGMP-activated current
To determine whether the SNP-activated Cd2+-sensitive current is carried by native AQP1 ion channels in the choroid plexus, we used siRNAs to knock down levels of AQP1 protein expression. We used two different approaches: (1) transfecting the cells with a mixture of siRNAs generated by enzymatic digestion of AQP1 double-stranded RNA, with a commercially available mixed siRNAs as the control; and (2) transfecting with sequence-directed synthetic siRNAs with matched scrambled sequences as controls, characterized previously for AQP1 in cholangiocytes (Splinter et al., 2003).
In whole-cell patch recordings, eGFP-positive cells transfected with 15 nm of the AQP1-mixed siRNAs failed to show a Cs+ current in response to SNP (Fig. 4a). Similarly, inclusion of 10 mm 8Br-cGMP in the pipette saline failed to induce a Cs+ current in the AQP1-mixed siRNA-treated cells (Fig. 4b), consistent with the observation that AQP1 protein levels are reduced by the siRNA treatment (Fig. 1). In contrast, choroid plexus cells transfected with eGFP alone, or with eGFP and the control–siRNA mixture, showed ionic conductances in response to SNP (Fig. 4a) and intracellular cGMP (Fig. 4b) that were not significantly different from the responses measured in nontransfected control cells (Fig. 4c). Two doses (15 and 60 nm) of control commercial siRNA mixture were tested. At a dose equal to that used to knock down AQP1 (15 nm), the control siRNA had no effect. At a fourfold excess, the control siRNA appeared to cause a modest decrease in the amplitude of the conductance response, suggesting high doses might have nonspecific effects. Nonetheless, the conductances measured for both groups of control siRNA-treated cells were significantly greater than that in the AQP1–siRNA-treated group.
The sequence-targeted AQP1–siRNAs effectively suppressed the cGMP-induced Cs+ currents in choroid plexus cells (Fig. 4d). The magnitude of the knockdown correlated with the dose of AQP1–siRNA and furthermore showed a differential efficacy between the two AQP1–siRNA sequences that matched published data (Splinter et al., 2003), in that AQP1-siRNA-b was more effective than AQP1-siRNA-a. The matching scrambled control–siRNAs for the two AQP1 sequences (-a and -b) at the higher dose had no effect on the cGMP-induced conductance (Fig. 4d); the control groups were not significantly different from nontransfected cells.
Endogenous currents measured in the absence of cGMP stimulation in physiological saline conditions were not significantly affected by the AQP1-mixed siRNA treatment (Fig. 5). Voltage-dependent currents (primarily K+) were measured in whole-cell patch recordings using an on-line leak subtraction protocol. Total currents, measured as unsubtracted traces, comprised mainly K+ and Cl− currents. The outward rectification of the voltage-sensitive current and the linear current–voltage relationship of the total current were superimposed for the control and siRNA-treated cells, standardized to the maximum outward current at +60 mV for each cell (Fig. 5b). Reversal potentials were not affected by siRNA treatment, indicating that the relative contributions from the ensemble of background ion channels were not altered. The absolute values of the background total currents were comparable for control and siRNA-treated cells, demonstrating that the loss of the voltage-insensitive AQP1-like conductance after siRNA knockdown cannot be attributed to a parallel decrease in a background voltage-insensitive current (Fig. 5c). Although a small decrease in the mean current amplitude for the voltage-sensitive component after siRNA treatment was seen, it was not significantly different from control. These data indicate that the introduction of the mixture of AQP1–siRNAs did not have any substantial effects on other general classes of ion channels found in the choroid plexus. These findings support the specificity of the siRNA knockdown and demonstrate that the cGMP-activated cationic current in the choroid plexus is mediated by AQP1. Contributions of AQP1 channels to the total currents were not observed in these recordings and were not expected in the absence of cGMP stimulation.
AQP1 ion channel activation decreases net fluid transport in the choroid plexus
To assess a possible contribution of AQP1 ion channel function to net fluid movement, primary cultures of choroid plexus epithelial cells were grown on 0.4 μm polycarbonate membranes (12 mm diameter, Costar transwell plates) as confluent monolayers and selected based on attaining an electrical resistance equal or >50 Ohm cm2. At day 14 in culture, isotonic medium was placed on both sides, with 4 ml in the lower chamber (basolateral) and 50 μl in the upper chamber (apical). Net fluid flux was monitored before and after treatment with 4.5 μm ANP applied basolaterally, in the presence and absence of 500 μm Cd2+ applied apically (Fig. 6). Appropriate polarity of the epithelial layer was confirmed by z-scanning confocal microscopy (Fig. 1i) showing AQP1 was limited to the apical membrane (upper) side of the cultured cell layer. Fluid transport in the choroid plexus epithelium is a vectorial process, characterized by the net movement of salt and water from the basolateral to the apical side of the barrier. After a 2 h incubation without drug treatment, the volumes accumulated at the apical sides were measured (providing the baseline flow rate); volumes were measured again for the same filters after a 2 h incubation with ANP (with and without Cd2+). ANP decreased the flow rate to 58.5 ± 13.4% of baseline (n = 4; mean ± SD), and this inhibitory effect was reversed by Cd2+ (85.5 ± 14.9% of baseline; n = 4; mean ± SD), which restored fluid movement to near baseline levels. Further characterization of AQP1 by knockdown with siRNA was not feasible, because the transfection efficiency in the primary choroid plexus cell cultures was, at best, 10% of the cells. Alternatively, we observed that downregulation of AQP1 protein after extended times in culture corresponded with a decreased effectiveness of ANP on transepithelial fluid transport. Immunocytochemical analyses showed that AQP1 consistently was expressed at high levels in apical membrane at 2 weeks in vitro but was substantially downregulated by 3 weeks in vitro. In corresponding transport studies of the choroid plexus at 23 d in vitro, there was no inhibitory effect of ANP on net fluid movement (data not shown).
Discussion
ANP receptors in the choroid plexus couple to guanylate cyclase, stimulating cGMP (Tsutsumi et al., 1987; Israel et al., 1988) and inhibiting CSF production (Steardo and Nathanson, 1987). We show that natively expressed AQP1 functions as a cGMP-gated ion channel and that the ionic conductance modulates fluid transport in the choroid plexus in a manner consistent with the observed effects in vivo. The similarities between AQP1 channel properties in the choroid plexus and the oocyte expression system, and the effective knockdown by AQP1–siRNAs, confirm that this conductance cannot be attributed to other channels known to be expressed in the choroid plexus (Hung et al., 1993; Speake et al., 2001, 2004).
Aquaporins have four water-selective pores, one in each subunit (Murata et al., 2000; Sui et al., 2001). In AQP1, the ion-conducting pore has been suggested to reside at the tetrameric center (Yool and Weinstein, 2002). The bacterial glycerol facilitator (GlpF), although not known as an ion channel, has ion binding sites in its central cavity that implicate this domain as a candidate ion pore in other ion channel aquaporins (Fu et al., 2000). Molecular dynamic modeling predicts that Na+ ions can, in theory, be pulled through the AQP1 central pore by a driving force (Yu et al., in press), whereas the individual subunit water pores do not allow ion permeation. Pharmacological data show that the AQP1 water and ion pathways are distinct; water permeability is blocked by TEA+ and not Cd2+ (Brooks et al., 2000; Yool et al., 2002), whereas the ionic conductance is blocked by Cd2+ but not TEA (Yool, 2002). An expanding role for aquaporins is becoming evident (Yool and Stamer, 2004). Ion channel function has been demonstrated for AQP0 (Zampighi et al., 1985; Ehring et al., 1990, 1992), AQP1 (Anthony et al., 2000; Boassa and Yool, 2003), AQP6 (Yasui et al., 1999), and a related MIP channel known as Big Brain (Yanochko and Yool, 2002, 2004) that is essential in early nervous system development in Drosophila.
Over the past decade, uncertainty in the AQP field has moved from an initial controversy about whether AQP1 is an ion channel (Agre et al., 1997) to whether or not the ion channel function can serve any meaningful contribution. The observation that AQP1 can serve as a cGMP-gated ion channel (Anthony et al., 2000; Boassa and Yool, 2002, 2003) has been confirmed independently by reconstitution in bilayers (Saparov et al., 2001), but the activity was suggested to be an artifact (i.e., misfolding of the AQP1 channel protein to produce a gain of function as a cGMP-gated cation-selective channel). The basis for uncertain functional relevance stems from the low numbers of AQP1 ion channels found to be active in expression systems. In oocytes, the cGMP-activated current typically ranges 5–10 μA at +40 mV from 1 ng of AQP1 RNA injected, a respectable level compared with other ion channels. However, using the parallel water permeability of the channel, it is possible to estimate the total number of AQP1 channels in the oocyte, which outstrips the number of ion channels by >50,000-fold (Yool and Weinstein, 2002). When reconstituted in bilayers, the proportion of available ion channels is estimated at one per million (Saparov et al., 2001); ion channel activity was undetectable in AQP1-transfected HEK cells (Tsunoda et al., 2004). In lieu of explanation as an accident, these differences could suggest that AQP1 ion channel activity is sensitive to regulatory mechanisms or interactions that vary with the expression system.
What proportion of AQP1 channels in the choroid plexus might contribute to the ionic conductance? A rough estimate is possible using fluid transport and ionic conductance data. A whole-cell cGMP-dependent conductance of ∼100 nS and a single-channel conductance of 166 pS puts the number of active AQP1 ion channels at ∼700 per cell (or more if the open probability is <1). To calculate water-channel number, the area of the 108 μm2 filter covered by confluent choroid plexus cells (∼200 μm2 each) corresponds to ∼5 × 105 cells per filter. The mean net fluid transport rate per filter was 50 μl/h, or ∼10-4 μl/h cell. The AQP1 unitary water permeability is 10−13 cm3/s (Zeidel et al., 1992), or 10−7 μl/h. Thus, the numbers of water pores per cell would be ∼1000 and of tetramers would be ∼250, no doubt an underestimate because total water flux must exceed the net fluid accumulation. If total water flux is 10-fold greater than the measured net, the ratio of AQP1 ion channels to water channels would be ∼1:10. However, it is equally reasonable that the ratio might be 1:100 or 1:1000. An important caveat is that the real number of AQP1 channels per cell remains to be measured. If the level of AQP1 expression in the highly water-permeable kidney proximal tubule (4 × 104 per μm2) (Maeda et al., 1995) is an example of a maximum case, by analogy the estimated number of AQP1 tetramers per choroid plexus cell could be as high as ∼107, which would yield an ion-to-ion channel ratio of ∼1:10,000. Any of these outcomes suggests that the availability of AQP1 to function as an ion channel is increased in the native choroid plexus environment compared with other preparations studied thus far. Precedent for the idea that a majority of channels can be in an inactive mode comes from quantitative analysis of the epithelial Na+ channel ENaC; open-channel probability calculations were found to be one order of magnitude lower when referenced to the total population of ENaC channels, as opposed to assessment only of the electrically active subpopulation (Firsov et al., 1996). The difference for AQP1 is that the electrically silent channels have a known function as water pores, whereas the purpose of silent modes in other classes of ion channels is not equally obvious.
Tissue-specific control of AQP1 ion channel availability is logical given differences in the functional goals of organs; not all tissues in which AQP1 is highly expressed would benefit from the presence of a large-conductance cationic current. For example, calculations from proximal tubule model suggested that a trace population of active AQP1 ion channels (equivalent to that seen in the oocyte expression system) would be sufficient to measurably influence Na+ reabsorption (Yool and Weinstein, 2002). Thus, the water-to-ion channel ratio of AQP1 might be a target of convergent control mechanisms, influenced by lipid environment, posttranslational modifications, cytoskeletal associations, or protein–protein interactions with molecules such as EphB2 tyrosine receptor kinase, anion transporters, and others (Cowan et al., 2000). Membrane environment and protein interactions govern properties of other ion channels (Konstas et al., 2003; Guggino, 2004; Kimura et al., 2004; Lin et al., 2004; Romanenko et al., 2004; Schreiber et al., 2004; Sorgen et al., 2004; Yanochko and Yool, 2004; Li and Naren, 2005; Song et al., 2005; Wang et al., 2005; Deval et al., 2006).
Ion channels and water channels are distinguished by their substrate specificity. An intriguing combination is seen in AQP1. In future work, it will be interesting to consider how depolarization, localized gradients of Na+ at the water channel vestibules, back-leak of Na+, or other mechanisms involving activated AQP1 ion channels might contribute to the observed decrease in the net transport of fluid across the choroid plexus barrier in response to ANP. In the choroid plexus, unlike most epithelial cells, the Na+-K+-ATPase transporter is located in the apical membrane (Masuzawa et al., 1984) and provides the driving force for fluid secretion into the ventricle. Elevation of cGMP causes inhibition of Na+-K+-ATPase (Ellis et al., 2000), providing a logical mechanism for achieving decreased CSF production by downregulation of Na+ active transport. Our data suggest cGMP-activated AQP1 ion channels also contribute to the regulatory response, because block of the AQP1 ionic conductance with Cd2+ reverses the inhibitory effect on ANP on fluid transport. This effect is opposite to what would be expected from Cd2+ block of the Na+-K+-ATPase pump, which should further suppress CSF production rather than restore it.
Pathologies and injuries associated with an imbalance between production and removal of CSF currently are limited in treatment options such as systemic diuretics or physical shunting. Recognition of AQP1 as a regulated multifunctional channel suggests it is a potential therapeutic target for pathological conditions involving altered fluid homeostasis (edema, hydrocephalus, pseudotumor cerebri, glaucoma, and others) and toxicity. The kidney proximal tubule and choroid plexus both express high levels of AQP1 and, coincidentally, are targets of Cd2+ toxicity (Valois and Webster, 1989; Thevenod, 2003). Expanding our understanding of mechanisms for the selective activation and block of aquaporin channels and their role in transmembrane signaling and transport are areas of compelling interest for advances in research and medicine.
Footnotes
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This work was supported by the Blanceflor Boncompagni-Ludovisi Foundation Fellowship (D.B.), the National Institutes of Health–National Institute of General Medical Sciences (A.J.Y.), and the Research to Prevent Blindness Foundation (W.D.S.). We thank Dr. D. Dulcis for assistance with image processing and A. Marble and E. Erbe for technical support.
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D. Boassa’s present address: National Center for Microscopy and Imaging Research, University of California, San Diego, La Jolla, CA 92093.
- Correspondence should be addressed to Dr. Andrea J. Yool, Department of Physiology, P.O. Box 245051, University of Arizona, Tucson, AZ 85724. Email: ayool{at}u.arizona.edu