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The Journal of Neuroscience, May 1, 2003, 23(9):3616
Amiloride-Insensitive Currents of the Acid-Sensing Ion Channel-2a (ASIC2a)/ASIC2b Heteromeric Sour-Taste Receptor Channel
Shinya Ugawa1, Takashi Yamamoto3, Takashi Ueda1, Yusuke Ishida1, 2, Akira Inagaki1, 2, Makoto Nishigaki1, and Shoichi Shimada1 Departments of 1 Anatomy II and 2 Otorhinolaryngology, Nagoya City University Medical School, Nagoya 467-8601, Japan, and 3 Department of Behavioral Physiology, Graduate School of Human Sciences, Osaka University, Suita, Osaka 565-0871, Japan
ABSTRACT
TOP
ABSTRACT
Introduction
Acid-sensing ion channel-2a (ASIC2a) is an amiloride-blockable proton-gated cation channel, probably contributing to sour-taste detection in rat taste cells. To isolate another subtype of the sour-taste receptor, we screened a rat circumvallate papilla cDNA library and identified ASIC2b, an N-terminal splice variant of ASIC2a. Reverse transcription-PCR analyses confirmed the expression of ASIC2b transcripts in the circumvallate papilla and, moreover, demonstrated its expression in the foliate and fungiform papillae. Immunohistochemical analyses revealed that ASIC2b, as well as ASIC2a, was expressed in a subpopulation of taste cells in the circumvallate, foliate, and fungiform papillae, and some of the cells displayed both ASIC2a and ASIC2b immunoreactivities. Subsequent coimmunoprecipitation studies with circumvallate papillae extracts indicated that ASIC2b associated with ASIC2a to form assemblies and, together with our immunohistochemical findings, strongly suggested that both ASIC2 subunits formed heteromeric channels in taste cells in the circumvallate, foliate, and fungiform papillae. Oocyte electrophysiology demonstrated that the ASIC2a/ASIC2b channel generated maximal inward currents at a pH of
2.0, which is in agreement with the in vivo pH sensitivity of rat taste cells, and that the amiloride sensitivity of the heteromer decreased with decreasing pH and was almost completely abolished at a pH of 2.0. These findings provide persuasive explanations for the amiloride insensitivity of acid-induced responses of rat taste cells.
Key words: proton; sour; acid-sensing ion channel (ASIC); immunoprecipitation; electrophysiology; amiloride
Introduction
Sour taste is essentially a proton taste, and proton-sensitive ion channels that are apically and basolaterally located in taste cells are believed to act as sour-taste receptors (Gilbertson et al., 2000
; Lindemann, 2001
Which channel molecule functions as a receptor for sour tastants in mammalian species? In the hamster, amiloride-blockable proton currents were recorded during acid-induced responses in taste cells that also exhibited amiloride-blockable Na+ currents in the absence of external protons. Therefore, amiloride-blockable epithelial sodium channels implicated in the taste of sodium salts have been proposed to contribute to sour-taste transduction (Herness and Gilbertson, 1999
We recently reported that a proton-activated cation channel, acid-sensing ion channel-2a (ASIC2a) [previously called mammalian degenerin-1 (MDEG1) and also known as BNC1a and BNaC1
(Waldmann and Lazdunski, 1998
Using a combination of molecular biological, morphological, and electrophysiological approaches, we show here that ASIC2b associates with ASIC2a to form a heteromeric complex in rat taste cells, modifying the pH sensitivity of the ASIC2a channel. ASIC2b, an N-terminal splice variant of ASIC2a, was first isolated from rat dorsal root ganglion neurons and functions as a modulatory subunit of ASIC channels (Lingueglia et al., 1997
Materials and Methods
The Center of Experimental Animal Sciences at Nagoya City University gave us permission for the following experiments.
Molecular cloning of ASIC2b. A rat circumvallate papilla cDNA library was screened at low stringency as described previously (Saishin et al., 1997
Reverse transcription-PCR. Male Wistar rats were anesthetized with Nembutal (50 mg/kg, i.p.) and decapitated. Poly(A)+ RNAs were isolated from the circumvallate/foliate/fungiform papillae and tongue epithelial tissue (no taste papillae) using a FastTrack 2.0 Kit (Invitrogen, San Diego, CA). The resulting 1 µg of poly(A)+ RNA from the taste papillae and 2 µg of poly(A)+ RNA from the tongue epithelial tissue were reverse transcribed using SuperScript II reverse transcriptase (Invitrogen), and 1/20th of the sample was amplified by PCR for 35 cycles with oligonucleotide primers: for ASIC2b, 5'-TGGTTCCGCAAACTGGCCGACTT-3' (forward) and 5'-AGGAAAGAAGTCGAGTCCCATCT-3' (reverse); for
-actin, 5'-GATCCTGACCGAGCGTGGCTACA-3' (forward) and 5'-ACGGATGTCAACGTCACACTTCA-3' (reverse). The molecular identity of the resulting PCR fragments was checked by DNA sequencing.
Antibody production. A synthetic peptide containing an N-terminal cysteine and rat ASIC2b residues 49-65 (QGPGVARRGRPSLSRTK) was conjugated to a keyhole limpet hemocyanin using m-maleimidobenzoyl-N-hydroxysuccinimide ester. The conjugated proteins were used to raise polyclonal ASIC2b antibodies in rabbits (female New Zealand rabbits) by standard procedures. The polyclonal rabbit serum reactive with rat ASIC2a residues 1-16 (MDLKESPSEGSLQPSS) was described previously (Ugawa et al., 1998
Western blotting. Rat circumvallate papillae, dorsal root ganglia, and ASIC2b-expressing (or water-injected) oocytes (for details, see section below discussing oocyte electrophysiology) were homogenized in 50 mM Tris-HCl, pH 7.5, 5 mM EDTA, 150 mM NaCl, 1% Triton X-100, and complete protease inhibitors (Roche Diagnostics, Basel, Switzerland). Equal amounts of protein (20 µg) were resolved by SDS-PAGE (10%) and transferred to polyvinylidene difluoride membranes (Immobilon-P; Millipore, Bedford, MA). An ASIC2b preimmune serum and the affinity-purified anti-ASIC2b (or anti-ASIC2a) antibody were diluted 1:1000 and 1:2500 (or 1:500), respectively, in a block solution containing 10% skim milk and 0.3% Tween 20 in Tris-buffered saline (TBS-T), and incubated with membranes overnight at 4°C. After washing three times in TBS-T solution, blots were detected with an alkaline phosphatase-labeled goat antirabbit IgG antibody (Roche Diagnostics) and visualized with a 5-bromo-4-chlor-indolyl-phosphate-nitroblue tetrazolium indicator substrate. Controls included use of water-injected oocytes and preabsorption of the diluted primary antibodies with each synthetic antigen (10
6 M) for 1 hr at room temperature before incubation with the membranes.
Immunohistochemistry. Fresh frozen sections (2-8 µm thick) of the circumvallate, foliate, and fungiform papillae of Wistar rats were fixed in a 4% paraformaldehyde-phosphate buffer for 30 min at 4°C; washed three times in a phosphate buffer; blocked for 4 hr in 5% skim milk, 5% normal goat serum, 1% BSA, and 0.3% Triton X-100; and then incubated overnight at 4°C with the anti-ASIC2b antibody diluted 1:2000 in the block solution. (For ASIC2a, the primary antibody diluted 1:500 in the block solution was used instead.) This was followed by a Cy3-conjugated antirabbit IgG secondary antibody (Amersham Biosciences, Tokyo, Japan), and the slides were observed using a fluorescence microscope (Nikon, Tokyo, Japan). To demonstrate colocalization of both ASIC2 proteins, the same experiments were performed on contiguous semithin sections (2 µm), and images of double-labeled cells were colorized and combined with Adobe Photoshop software (Adobe Systems, San Jose, CA). Neither preimmune sera showed any immunoreactivity (data not shown).
Coimmunoprecipitation. Rat circumvallate papillae were lysed on ice in 10 vol of a coimmunoprecipitation buffer (20 mM Tris-HCl, 150 mM NaCl, 1% NP-40, 100 µg/ml DNase, 50 µg/ml RNase A, 1 mM PMSF, 1 µg/ml leupeptin, 1 µg/ml N-
Oocyte electrophysiology. The procedures used were basically the same as those described previously (Inoue et al., 1995
70 mV.
Results
Expression of ASIC2b in rat taste cells in the circumvallate, foliate, and fungiform papillae
To solve the discrepancies (see Introduction), we made efforts to isolate another subtype of the sour-taste receptor. We screened a rat circumvallate papilla cDNA library with a partial ASIC2a cDNA probe at low stringency and obtained several independent clones. The longest cDNA clone showed high homology with ASIC2a and turned out to be identical to ASIC2b (previously called MDEG2). To confirm the presence of ASIC2b mRNA in the circumvallate papilla, reverse transcription (RT)-PCR experiments were performed (Fig. 1). It was found that the expected 504 bp fragments were observed in the circumvallate papillae cDNA (lane 1), whereas no detectable signal was seen in the circumvallate papillae sample without reverse transcriptase (lane 2) or in the tongue epithelial tissue (no taste papillae) cDNA (lane 7). Moreover, the experiments revealed that the ASIC2b fragments were detected in the foliate and fungiform papillae cDNAs (lanes 3 and 5, respectively), whereas no signal was seen in any taste papilla sample without reverse transcriptase (lanes 4 and 6). On the basis of these results, we further continued RT-PCR, leading to the isolation of the full-length ASIC2b cDNA from the foliate and fungiform papillae (data not shown). All of these results indicated that the circumvallate papilla clearly expressed ASIC2b transcripts, and that the foliate and fungiform papillae did also. [We cloned the full-length ASIC2a cDNA as well from the foliate and fungiform papillae using an RT-PCR method (data not shown).]
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Figure 1. RT-PCR analysis of ASIC2b mRNA expression. PCR fragments corresponding to the N-terminal region of ASIC2b were observed in the circumvallate, foliate, and fungiform papillae cDNAs (lanes 1, 3, 5), whereas no detectable signal was seen in the circumvallate, foliate, or fungiform papillae sample without reverse transcriptase (lanes 2, 4, 6) or in the tongue epithelial tissue (no taste papillae) cDNA (lane 7). Lane 8, Tongue epithelial tissue sample without reverse transcriptase. Control X174 RF-HaeIII).
ASIC2b expression in the rat tongue at the protein level was confirmed by Western blotting (Fig. 2). Circumvallate samples were subjected to the analyses, because the papilla contains a larger number of taste buds than the foliate and fungiform papillae. Using a rabbit antibody generated against ASIC2b amino acids 49-65, a single prominent band of ~70 kDa was detected in extracts of the circumvallate papillae (lane 2), whereas the preimmune serum did not detect the blots (lane 1). Preabsorption with 10
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Figure 2. Expression of ASIC2b protein in rat circumvallate papilla. ASIC2b expression at the protein level was confirmed by Western blot analyses. Using a rabbit antibody generated against ASIC2b amino acids 49-65, single prominent bands of ~70 kDa blots were detected in extracts of the circumvallate papillae and dorsal root ganglia (lanes 2, 4; Peptide,
Immunohistochemical analyses of ASIC2b expression in the circumvallate papilla were performed. The analyses revealed that ASIC2b-immunoreactive cells occurred in taste buds but were not detected in the surrounding lingual epithelia (Fig. 3A). At the cellular level, intense ASIC2b immunoreactivity was detected in a subset of taste cells (Fig. 3B). As reported previously (Ugawa et al., 1998
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Figure 3. Localization of ASIC2 subunits by immunohistochemistry. A-C, Fluorescence micrographs of circumvallate papillae immunostained with an anti-ASIC2b antibody in the absence (A, B) or presence (C) of 10
We next performed the same experiments on other taste papillae and found that ASIC2b and ASIC2a proteins were localized in a subset of taste cells in the foliate (Fig. 3, G,H and J,K, respectively) and fungiform (Fig. 3, M,N and P,Q, respectively) papillae. Preabsorption with 10
ASIC2a/ASIC2b heteromeric complex in rat taste cells
Immunohistochemistry on contiguous semithin sections (2 µm thick) was performed to determine whether ASIC2a and ASIC2b were colocalized within single taste cells (Fig. 4). It showed that both ASIC2 proteins were coexpressed in a subset of taste cells in the circumvallate (top row), foliate (middle row), and fungiform (bottom row) papillae. Regrettably, we failed to estimate the extent of the colocalization, because preparation of such thin, adjacent, and morphologically fine sections was quite difficult. Our results mean that ASIC2a and ASIC2b proteins were, at least in part, colocalized in a subpopulation of taste cells in the papillae. Heteromeric assemblies of both ASIC2 proteins in heterologous expression systems have been described previously (Lingueglia et al., 1997
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Figure 4. Colocalization of ASIC2a and ASIC2b within single taste cells. Immunohistochemical analyses with anti-ASIC2a and anti-ASIC2b antibodies were performed on contiguous semithin sections (2 µm). Red represents ASIC2a staining in rat circumvallate, foliate, and fungiform papillae (A, D, and G, respectively), and green represents ASIC2b staining in the papillae (B, E, H). Regions of overlap (Merge) are yellow (C, F, I). Both ASIC2a and ASIC2b proteins were, at least in part, colocalized in a subpopulation of taste cells in the circumvallate (top), foliate (middle), and fungiform (bottom) papillae. Scale bars, 25 µm.
We then performed coimmunoprecipitation studies to confirm the ASIC2 assembly biochemically (Fig. 5). Circumvallate papillae extracts were studied. ASIC2a/ASIC2b complexes were detected in immunoprecipitated fractions with an anti-ASIC2b or anti-ASIC2a antibody (lanes 3 and 6, respectively), but not in those with each preimmune antiserum (lanes 1 and 4, respectively) or with a buffer solution used for the purification and dilution of both antibodies (lanes 2 and 5). These results clearly indicate that ASIC2a/ASIC2b complexes were present in the extracts. Together with our immunohistochemical observations, these results strongly suggest that ASIC2a and ASIC2b form heteromeric assemblies in a subset of taste cells in rat circumvallate papillae and also suggest that the ASIC2 assemblies are also located in a subset of taste cells in the foliate and fungiform papillae.
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Figure 5. Coimmunoprecipitation of ASIC2a and ASIC2b. Detergent-solubilized proteins of rat circumvallate papillae were subjected to the immunoprecipitation (I.P.) studies. ASIC2a/ASIC2b heteromeric complexes were detected (Detect.) in immunoprecipitated fractions with an anti-ASIC2b or anti-ASIC2a antibody (Ab.) (lanes 3 and 6, respectively), but not in those with each preimmune antiserum (Pre.) (lanes 1 and 4, respectively) or with a buffer solution used for purification and dilution of both antibodies (Buf.; lanes 2, 5). Molecular mass standards are indicated on the left (Mr).
ASIC2b modifies inactivation kinetics and pH dependence of ASIC2a
We analyzed the electrophysiological properties of the ASIC2a/ASIC2b heteromeric complex using an X. laevis oocyte mRNA translation system with a two-electrode voltage clamp. It was confirmed that ASIC2b was inactive by itself but interacted with ASIC2a to form heteromers with new properties, as described previously (Lingueglia et al., 1997
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Figure 6. Functional expression of ASIC2a and ASIC2b. A, B, Representative whole-cell current traces of ASIC2 homomeric and heteromeric channels expressed in X. laevis oocytes. Acidic pH solutions were present in the bath during times indicated by bars. C, Dose-response curves for the extracellular pH. The proton-activated currents increased in a pH-dependent manner with decreasing extracellular pH in the range of 6.5-2.0 in oocytes expressing ASIC2a/ASIC2b heteromers, whereas ASIC2a homomers generated maximal inward currents at pH ~3.0. Shown are mean values ± SEM from 25 experiments, respectively. D, Representative proton (pH 4.0)-induced currents of ASIC2a/ASIC2b-expressing oocytes in the absence or presence of acetic acid. Stimulation by acidic solutions containing 10 mM acetic acid (CH3COOH, pH 4.0) generated a larger amplitude of the peak currents than that induced by hydrochloric acid solutions (HCl, pH 4.0) at equal pH, whereas the 10 mM sucrose solutions, final pH 4.0, showed no apparent effects on the proton-induced currents. E-H, Relationship between stimulating pH values and amiloride sensitivity of the ASIC2a/ASIC2b heteromer. The whole-cell current induced by a rapid pH drop from 7.5 to 5.5 was almost completely blocked by 100 µM amiloride (E), whereas the same amiloride treatment barely reduced the current induced by a rapid pH drop from 7.5 to 3.0 (F). The inhibitory effect of 100 µM amiloride was attenuated in a pH-dependent manner with decreasing pH (G). The x- and y-axes in G represent concentrations of amiloride and percentage of blocked currents (compared with the maximal induced current at each pH value), respectively. The pH dependency of the heteromer was shifted to more acidic pH values in the presence of 100 µM amiloride (H). The values in G and H represent mean ± SEM of at least five experiments.
The ASIC2a channel activity can be enhanced by acetic acid (Ugawa et al., 1998
Relationship between amiloride sensitivity of the ASIC2a/ASIC2b channel and pH values of acidic stimuli
The inhibitory effect of amiloride on the ASIC2a/ASIC2b channel currents evoked by different pH stimuli was investigated on condition that both ASIC2 subunits fulfilled their functions as a heteromer. In response to rapid pH changes from 7.5 to 5.5, the heteromer generated fast-rising and slowly desensitizing inward currents that were almost completely blocked by 100 µM amiloride (Fig. 6E). In contrast, the same amiloride treatment barely reduced the inward currents at a pH of 3.0 (Fig. 6F). The inhibitory effect was attenuated in a pH-dependent manner with decreasing extracellular pH (Fig. 6G). IC50 (inhibition constant) values of the heteromer under pH shifts to 5.5 and 4.0 were 4.5 ± 1.0 µM (mean ± SEM; n = 7) and 22.0 ± 4.2 µM (n = 9), respectively, and the value under the pH shift to 3.0 was likely to range between 700 and 900 µM (n = 5).
We also examined the effect of 100 µM amiloride on the pH dependency of the ASIC2a/ASIC2b heteromeric channel activity (Fig. 6H). Although its maximal whole-cell current was not affected by the amiloride treatment, the pH dependency of the heteromer shifted to more acidic pH values compared with those in the absence of the drug. The half-points for activation of the ASIC2a/ASIC2b channel current in the absence and presence of 100 µM amiloride were pH 3.9 ± 0.2 (n = 7) and pH 3.4 ± 0.2 (n = 9), respectively. It is noteworthy that the amiloride sensitivity of the ASIC2a/ASIC2b channel was markedly reduced at a pH of
Discussion
We successfully isolated the ASIC2b cDNA from the rat tongue using a combination of homology screening and RT-PCR approaches. According to our immunohistochemical and coimmunoprecipitation studies, ASIC2a and ASIC2b were colocalized within a subset of taste cells in the circumvallate, foliate, and fungiform papillae, and both proteins probably formed heteromeric assemblies in the cells. The ASIC2a/ASIC2b channels are likely to be expressed at least in type III cells that make synaptic contacts with gustatory afferent neurons, because ASIC2a is so, as reported previously (Ugawa et al., 1998
As described previously (Lingueglia et al., 1997
Both ASIC2a and ASIC2b subunits belong to the ASIC family of cation channels. Members of this family form proton-activated channels in the mammalian central and peripheral nervous systems (Waldmann and Lazdunski, 1998
Amiloride sensitivity is a common notable feature of ASIC channels. However, according to numerous previous observations, acid-evoked responses of rat taste cells were barely suppressed by amiloride, so it has been highly controversial whether an amiloride-sensitive sour-taste transduction pathway really exists in the rat. Amiloride inhibited gustatory neural responses to hydrogen chloride in the hamster and rat, but its inhibitory effect was restricted to acid-evoked responses in sodium-selective nerve fibers (N-best fibers), which primarily carry information for salty taste (Ninomiya and Funakoshi, 1988
To solve this riddle, we investigated the amiloride sensitivity of the ASIC2a/ASIC2b channel in various pH conditions and found that it dramatically decreased at a pH of
According to imaging experiments, extracellular application of acids generates intracellular pH decreases in rat taste cells (Lyall et al., 1997
FOOTNOTES Received Dec. 17, 2002; revised Feb. 11, 2003; accepted Feb. 20, 2003.
This work was supported by research grants from the Japan Society for the Promotion of Science (to S.U. and S.S.).
Correspondence should be addressed to Dr. Shinya Ugawa, Department of Anatomy II, Nagoya City University Medical School, 1 Kawasumi, Mizuho-cho, Mizuho-ku, Nagoya 467-8601, Japan. E-mail: ugawa{at}med.nagoya-cu.ac.jp.
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