Abstract
Ionotropic glutamate receptors, which underlie a majority of excitatory synaptic transmission in the CNS, associate with transmembrane proteins that modify their intracellular trafficking and channel gating. Significant advances have been made in our understanding of AMPA-type glutamate receptor (AMPAR) regulation by transmembrane AMPAR regulatory proteins. Less is known about the functional influence of cornichons—unrelated AMPAR-interacting proteins, identified by proteomic analysis. Here we confirm that cornichon homologs 2 and 3 (CNIH-2 and CNIH-3), but not CNIH-1, slow the deactivation and desensitization of both GluA2-containing calcium-impermeable and GluA2-lacking calcium-permeable (CP) AMPARs expressed in tsA201 cells. CNIH-2 and -3 also enhanced the glutamate sensitivity, single-channel conductance, and calcium permeability of CP-AMPARs while decreasing their block by intracellular polyamines. We examined the potential effects of CNIHs on native AMPARs by recording from rat optic nerve oligodendrocyte precursor cells (OPCs), known to express a significant population of CP-AMPARs. These glial cells exhibited surface labeling with an anti-CNIH-2/3 antibody. Two features of their AMPAR-mediated currents—the relative efficacy of the partial agonist kainate (IKA/IGlu ratio 0.4) and a greater than fivefold potentiation of kainate responses by cyclothiazide—suggest AMPAR association with CNIHs. Additionally, overexpression of CNIH-3 in OPCs markedly slowed AMPAR desensitization. Together, our experiments support the view that CNIHs are capable of altering key properties of AMPARs and suggest that they may do so in glia.
Introduction
Throughout the CNS, AMPARs mediate rapid excitatory signaling between neurons and between neurons and glia. AMPARs are homotetrameric or heterotetrameric assemblies of the pore-forming subunits GluA1–4, whose properties depend critically on their subunit composition and on the nature of alternatively spliced or posttranscriptionally edited variants (Traynelis et al., 2010). The GluA2 subunit is particularly important, as editing at its Q/R site in the pore profoundly affects calcium permeability of the receptors. Thus, AMPARs lacking GluA2 are permeable to calcium (Geiger et al., 1995), have a large single-channel conductance (Swanson et al., 1997), and exhibit characteristic voltage-dependent block by endogenous intracellular polyamines (Bowie and Mayer, 1995; Kamboj et al., 1995; Koh et al., 1995).
The properties of both calcium-impermeable (CI) and calcium-permeable (CP) AMPARs are strongly influenced by their interaction with transmembrane AMPAR regulatory proteins (TARPs). Six TARP isoforms have been identified—γ-2 (stargazin), γ-3, γ-4, γ-5, γ-7, and γ-8—that differentially modulate the trafficking, gating, and pharmacology of AMPARs (Tomita et al., 2003; Fukaya et al., 2005; Cho et al., 2007; Milstein et al., 2007; Soto et al., 2007, 2009; Kato et al., 2008, 2010a). Recently, cornichon homologs 2 and 3 (CNIH-2 and CNIH-3) were identified by proteomic analysis as AMPAR-interacting proteins and were suggested to form part of the AMPAR assembly at the cell surface of various neurons and glia (Schwenk et al., 2009). Coexpression of recombinant AMPARs with CNIH proteins, as with TARPs, increases the surface expression of receptors and slows their deactivation and desensitization (Schwenk et al., 2009; Kato et al., 2010b; Shi et al., 2010; Gill et al., 2011). However, the status of CNIHs as bona fide AMPAR auxiliary subunits has been the subject of debate (Jackson and Nicoll, 2009, 2011; Tigaret and Choquet, 2009; Brockie and Maricq, 2010; Shi et al., 2010).
Here we have compared the effects of CNIH-1, CNIH-2, and CNIH-3 with those of stargazin (TARP γ-2) on both GluA2-lacking CP-AMPARs and GluA2-containing CI-AMPARs. We found that CNIH-2 and -3 markedly increased single-channel conductance of CP-AMPARs and slowed the desensitization and deactivation of both CI- and CP-AMPARs. Furthermore, in the presence of CNIH-2 or -3, CP-AMPARs displayed increased calcium permeability, decreased block by intracellular polyamines, and enhanced glutamate potency. Thus, for recombinant CP-AMPARs, interaction with CNIHs would be expected to facilitate AMPAR-mediated calcium entry. We examined the potential interaction of CNIHs and native CP-AMPARs in rat optic nerve oligodendrocyte precursor cells (OPCs), glial cells known to express CP-AMPARs (Bergles et al., 2000). OPCs exhibited surface immunolabeling with an antibody to CNIH-2/3, consistent with the presence of cornichon proteins in the cell membrane. In whole-cell recordings from OPCs, the relative amplitude of responses elicited by glutamate and the partial agonist kainate, together with the marked potentiation of kainate responses by the positive allosteric modulator cyclothiazide (CTZ), also suggested the incorporation of CNIHs in functional surface AMPARs. Additionally, the overexpression of CNIH-3 in OPCs markedly slowed AMPAR desensitization. Our data suggest that the presence of CNIHs can influence key properties of AMPARs and that they may serve this function in OPCs.
Materials and Methods
Cell culture.
tsA201 cells were maintained as described previously (Soto et al., 2007) and transfected using Lipofectamine 2000 (Invitrogen). DNA for GluA1(i) or GluA2(i)(Q), or both GluA1(i) and GluA2(i)(R), was transfected either alone or with CNIH-1, CNIH-2, CNIH-3, or γ-2. Coexpression of GFP was used to identify transfected cells. After 24 h, cells were transferred to coverslips, and electrophysiological recordings were made 24–72 h later. Some transfections were maintained in the presence of 50 μm NBQX to limit cytotoxic effects.
Electrophysiology.
Solutions and procedures were as described previously (Soto et al., 2007). For outside-out patch and whole-cell recording, the “external” solution contained the following (in mm): 145 NaCl, 2.5 KCl, 1 CaCl2, 1 MgCl2, 10 glucose, and 10 HEPES, pH 7.3, with NaOH. For fast application experiments, glutamate was used at a concentration of 10 mm [nonstationary fluctuation analysis (NSFA) and I–V measurements] or 1 mm (measurement of deactivation). Jump experiments were performed at −60 mV. Steady state single-channel recordings were performed in 10 mm glutamate at −80 mV. The “internal” (pipette) solution contained the following (in mm): 145 CsCl, 2.5 NaCl, 1 Cs-EGTA, 4 MgATP, 0.1 spermine tetrahydrochloride, and 10 HEPES, pH 7.3, with CsOH. Rapid solution switching was achieved by piezoelectric translation of a theta-barrel application tool. Fast exchange (10–90% rise time <200 μs) was confirmed by averaging liquid junction currents at the end of each experiment for both 1 and 100 ms steps. Measurement of relative calcium permeability was carried out as described previously (Soto et al., 2007). Ramps from −80 to +60 mV were applied in “low” and “high” Ca2+ solutions as follows (in mm): low Ca2+: 145 NaCl, 2.5 KCl, 1 CaCl2, 1 MgCl2, 10 HEPES, pH 7.3, with NaOH; high Ca2+: 30 CaCl2, 110 N-methyl-d-glucamine, 5 HEPES, 50 sucrose, pH 7.3, with HCl. Control ramps were recorded in each Ca2+ solution, then in the same solutions containing 1 mm glutamate and 50 μm CTZ (Tocris Bioscience). Further control ramps were recorded on return to low Ca2+. The I–V relationships of control ramps were subtracted from the agonist-evoked currents. In these experiments, the pipette solution contained either 100 μm or no added spermine. As no differences in the reversal potentials were observed, the data were pooled. The relative Ca2+ permeability, PCa/PNa, was determined from the reversal potentials in low Ca2+ and in high Ca2+ extracellular solutions using the equation where aNa and aCa represent the activities of Na+ and Ca2+ in the extracellular solutions (108.7 and 16.5, calculated from activity coefficients of 0.75 and 0.55, respectively) (Geiger et al., 1995), and R, T, and F have their conventional meanings. Recording pipettes were pulled from borosilicate glass capillaries (Harvard Apparatus) coated with Sylgard 184 resin (Dow Corning) and fire polished to a final pipette resistance of 4–7 MΩ (whole-cell recording) and 10–15 MΩ (outside-out patches). Pipettes contained standard “intracellular solution” (Soto et al., 2007) supplemented with 100 μm spermine. For whole-cell recordings, series resistance was maintained between 5 and 16 MΩ and was compensated by 75% (Axopatch 200A). Residual series resistance errors were corrected off-line. Whole-cell input capacitances were 9–18 pF. Voltage ramps were performed every 5 s between −70 mV and +60 mV (100 mV/s) following a 500 ms hold at −70 mV. The average current for the −70 mV period was used to generate the steady state dose–response curves (CTZ was not used). Currents were filtered at 1 kHz and sampled at 2 kHz. Records from outside-out patches were filtered at 10 kHz and sampled at 50 kHz.
Data analysis.
NSFA and Boltzmann fitting were carried out as described previously (Soto et al., 2007). EC50 values (peak or steady state) were derived by fitting the Hill equation: where Imax is the peak of the fit, EC50 is the concentration producing the half-maximal response and nH is the Hill coefficient. Imax values derived from fits to individual experiments were used to rescale each dataset. The rescaled values were then averaged and refit for each receptor combination. The final fits were weighted according to the SD of the averages.
Single-channel records were filtered off-line at 2 kHz (8-pole low-pass digital Clampfit 10, Bessel) before analysis and idealized using a 50% threshold method (Clampfit 10, Bessel). Events briefer than two filter rise times were excluded from the analysis. To estimate the channel chord conductance, current amplitude histograms were constructed and fitted to the sum of Gaussian components. Open time histograms were fitted with mixtures of exponential functions to obtain mean open times. Bursts were defined as openings or groups of openings separated from each other by shut times greater than a critical shut time (tcrit). These values were calculated as the lowest frequency shut time bin (10 bins/decade) that clearly separated the “brief” shut time component from the “long” shut time component in the Sigworth-Sine transformed shut time distributions. Using this criterion, tcrit values were consistently 8 to 10 ms for all patches. Mean burst duration and number of bursts were estimated using Scilab 5.2 (www.scilab.org).
OPC cultures.
Optic nerve OPCs were prepared using the method of Shi et al. (1998). Briefly, optic nerves were obtained from postnatal day 7 (P7) male and female rats in accordance with the UK Animals (Scientific Procedures) Act 1986. Tissue was diced, digested in trypsin 0.05% EDTA, then gently dissociated for 30 min at 37°C. Dissociated tissue was sequentially immunopanned on Ran-2 (T1B-119; LGC Standards), anti-galactocerebrosidase (GalC) (AB142; Millipore), and then O4 antibody plates (MAB1326; R&D Systems) to select GalC− O4+ OPCs (Zonouzi et al., 2011). Purified OPCs were transferred to poly-l-lysine-coated 24-well tissue culture plates containing proliferation medium. All cells were cultured at 37°C, 5% CO2, in DMEM (Invitrogen) containing Sato medium, as follows: human transferrin (100 μg/ml), bovine serum albumin (100 μg/ml), putrescine (16 μg/ml), progesterone (60 ng/ml), sodium selenite (40 ng/ml), N-acetyl-l-cysteine (6.3 μg/ml), bovine insulin (5 μg/ml) (Sigma), glutamine (2 mm), sodium pyruvate (1 mm), and penicillin-streptomycin (100 U each) (Sigma). Proliferation medium also contained OPC mitogens PDGF-AA and bFGF (both 10 ng/ml) (R&D Systems). OPCs were transfected with CNIH-3 and GFP DNA using Ca2+ phosphate, and recordings were made from labeled cells 24 h later.
Immunocytochemistry.
OPC cultures on poly-l-lysine-coated coverslips were fixed with 4% PFA for 10 min at 25°C and washed with 1× PBS. Cells were then incubated with in 1× PBS containing 250 mg of BSA (Sigma) and 10% horse serum (Invitrogen) and (where stated) permeabilized with 0.5% Triton for 20 min. Cells were labeled with primary antibodies for 1 h at 25°C: anti-O4 (mouse, MAB345, 1:100; Millipore) and anti-CNIH-2/3 antibody (3.5 μg/ml; a gift from Bernd Fakler, University of Freiburg, Freiburg, Germany). Secondary antibodies—goat anti-rabbit Alexa-568 (A-11011, 1:1000; Invitrogen) and goat anti-mouse Alexa-488 (A-21042, 1:1000; Invitrogen)—were applied for 1 h at 25°C. Coverslips were mounted using anti-fade medium (Invitrogen).
Statistical analysis.
All group data were compared using a nonparametric Kruskal–Wallis rank-sum test followed by pairwise Wilcoxon rank-sum tests with Holm's sequential Bonferroni correction for multiple comparisons (R, version 2.9.2; The R Foundation for Statistical Computing; http://www.R-project.org). Single comparisons were made using Wilcoxon rank-sum test. For all data, differences were considered significant at p < 0.05.
Results
Cornichons slow desensitization and deactivation of CP- and CI-AMPARs
Recent studies of heterologously expressed recombinant AMPARs have shown that CNIH-2 and -3 can markedly slow receptor deactivation and desensitization (Schwenk et al., 2009; Kato et al., 2010a; Shi et al., 2010). We extended these observations by examining the influence of three CNIH family members (CNIH-1, -2, and -3) on multiple properties of both CI and CP-AMPARs. First, using rapid application of glutamate (10 mm) onto outside-out membrane patches from tsA201 cells, we confirmed that both CNIH-2 and -3 produced an approximately twofold slowing in the desensitization of homomeric GluA1 CP-AMPARs (increased τw, des; Fig. 1a,b). This effect on desensitization was qualitatively similar to that seen with the TARP γ-2 (Fig. 1b), but for CNIH-2 the extent of slowing was significantly greater than that produced by γ-2 (Table 1). CNIH-1, which has been shown not to interact with AMPARs (Schwenk et al., 2009), was without effect (Fig. 1b). In addition, we found that CNIH-2 and -3 slowed the deactivation (increased τw, deact) of homomeric GluA1 AMPARs (Table 1). CNIH-3 also slowed the deactivation and desensitization of GluA1/A2 heteromers (Fig. 1c, Table 1) and of homomeric GluA2(Q) receptors (Fig. 1d), with the latter the most markedly affected; τdeact GluA2(Q) was increased more than 10-fold by CNIH-3 (Table 1). This suggests subunit selective effects of the CNIHs. The slowing of desensitization by CNIH-2 and -3 was accompanied, in GluA2-containing receptors, by an increase in the steady state current (Table 1).
Cornichons increase channel conductance of CP- but not CI-AMPARs
To determine whether other functionally important AMPAR properties are regulated by cornichons, we examined their influence on channel gating, glutamate sensitivity, and calcium permeability. Although an effect of CNIH-2 on channel conductance of homomeric GluA1 receptors has recently been described (Shi et al., 2010), the effects of other cornichons have not been determined. We first estimated the single-channel conductance and peak open probability of agonist-bound channels (Po, peak) using NSFA of macroscopic current responses. As expected, CNIH-2 increased the weighted mean single-channel conductance of homomeric GluA1 receptors (∼1.5-fold). A similar effect was seen with CNIH-3, and for both cornichons the effects were comparable to the increase seen with TARP γ-2 (Fig. 1b, Table 2). Again, CNIH-1 was without effect. None of the coexpressed CNIH proteins altered Po, peak (Table 2).
The cornichon-induced change in channel conductance inferred from macroscopic currents was confirmed in separate recordings in which we analyzed directly resolved single-channel openings. Thus, when CNIH-3 was coexpressed with GluA1, steady state single-channel currents evoked by 10 mm glutamate (−80 mV) (Fig. 1e) displayed markedly increased chord conductance (from 14.3 ± 2.2 to 22.3 ± 1.3 pS; n = 5 and 7, respectively; p = 0.030), mean burst duration (from 5.2 ± 1.0 to 30.5 ± 13.3 ms; p = 0.030), and mean open time (from 1.4 ± 0.1 to 5.7 ± 2.0 ms; p = 0.010) (Fig. 1f). Effects on conductance were not restricted to homomeric GluA1 AMPARs. Both CNIH-2 and -3 also increased the conductance of homomeric GluA2(Q) receptors (Fig. 1d, Table 2). However, unlike TARP γ-2, neither CNIH-2 nor CNIH-3 affected the conductance of heteromeric GluA1/2 CI-AMPARs (Fig. 1c). This latter observation reveals a distinction between cornichons and TARPs in their regulation of channel properties and points to the possibility of a selective effect of cornichons on the conductance of CP-AMPARs.
Cornichons are less effective than TARP γ-2 in decreasing polyamine block of CP-AMPARs
TARPs decrease the block of CP-AMPARs by intracellular polyamines at positive and negative membrane potentials, reducing the characteristic inward rectification (Soto et al., 2007). We compared the polyamine block of CP-AMPARs (homomeric GluA1) when coassembled either with cornichon proteins or γ-2, by examining currents generated by fast application of glutamate to outside-out membrane patches (−100 mV to +60 mV). Conductance-voltage (G–V) plots were constructed from currents recorded in the negative voltage range (Fig. 2a) and fitted with Boltzmann functions (Fig. 2b). While both CNIH-2 and -3 caused clear rightward shifts in the fitted curves (depolarization in V1/2), the change was significantly less marked than with γ-2 (Fig. 2d, Table 2). The rectification index (RI+60/–80; ratio of peak current at +60 and −80 mV) increased in the presence of CNIH-2 and -3; however, this was significantly less that the change in RI seen with the coexpression of γ-2 (Fig. 2c, Table 2). Thus, using either measure to quantify relief of spermine block, CNIH-2 and -3 were less effective than γ-2. This result differs from that of Shi et al. (2010), who observed equivalent effects of TARP γ-2 and cornichons on polyamine block.
Regulation of AMPAR calcium permeability
To determine whether the CNIH-2-induced change in spermine sensitivity was accompanied by a change in the relative permeability of Ca2+ (PCa/PNa), we compared the reversal potential of glutamate-evoked currents in solutions containing 1 or 30 mm Ca2+ (low-Ca2+ or high-Ca2+). Switching from low- to high-Ca2+ shifted the reversal potentials for homomeric GluA1 receptors toward more negative values. By contrast, when GluA1 receptors were coexpressed with CNIH-2 or γ-2, the same manipulation shifted the reversal potential to positive membrane potential values (Fig. 2e,f). From these Erev shifts, we calculated that PCa/PNa increased from 2.7 ± 0.3 with GluA1 alone (n = 9) to 5.1 ± 0.7 in the presence of CNIH-2 (n = 9, p = 0.049) and to 4.7 ± 0.4 in the presence of γ-2 (n = 8, p = 0.0017) (Fig. 3b). As expected, we saw no significant change in PCa/PNa when CNIH-1 was coexpressed with GluA1 (2.3 ± 0.2, n = 9, p = 0.57).
CNIH-2 enhances glutamate potency
We next asked whether CNIH-2, like γ-2 (Yamazaki et al., 2004; Priel et al., 2005; Tomita et al., 2005b; Kato and Bredt, 2007; Kott et al., 2007), modified glutamate potency, a measure that reflects both receptor affinity and gating. Using rapid application of glutamate (0.03–10 mm) onto excised patches, we constructed concentration–response curves for the peak current (Fig. 3a,b). For homomeric GluA1 receptors, the glutamate EC50, peak decreased from 1.55 ± 0.22 mm to 0.92 ± 0.07 mm in the presence of CNIH-2 (both n = 7, p = 0.033) and to 0.45 ± 0.09 mm with γ-2 (n = 3, p = 0.033) (Fig. 3c). The measurement of peak responses to rapid glutamate application provides information most relevant to direct synaptic responses. AMPARs in neurons or glia that are not in close apposition to release sites may be exposed to glutamate concentration transients of relatively slow time course. Thus, during transmitter spillover, the glutamate transient that activates extrasynaptic AMPARs reaches a relatively low concentration that lasts for many milliseconds (Bergles et al., 1999; Szapiro and Barbour, 2007). Additionally, activation of AMPARs within the endoplasmic reticulum, where glutamate activates gating movements that are suggested to be critical for AMPAR biogenesis (Penn et al., 2008; Coleman et al., 2009), may well occur under near-equilibrium conditions. We therefore examined whole-cell responses to bath-applied glutamate (0.001–1 mm) to obtain steady state responses (Fig. 3d,e). CNIH-2 lowered EC50, steady state from 19.8 ± 2.7 μm (n = 4) to 9.4 ± 1.4 μm (n = 4, p = 0.029) and greatly increased current density (Fig. 3e). Thus, CNIH-2 produced statistically significant, albeit modest, enhancement of CP-AMPAR activation, in response to both rapid glutamate transients and sustained glutamate application.
Although we have shown, with heterologous expression, that cornichons can influence key aspects of AMPAR function, including glutamate potency, channel kinetics, channel conductance, polyamine block, and calcium permeability, a question remains as to the physiological relevance of such changes. For hippocampal neurons at least, there is evidence for the incorporation of cornichons within synaptic AMPARs, either alone (Schwenk et al., 2009) or in combination with TARP γ-8 (Kato et al., 2010b; Gill et al., 2011). But there is no general consensus on this point. Thus, Shi et al. (2010) reported that neuronal overexpression of epitope-tagged CNIH-2 led to high protein density in the Golgi apparatus, but not at the cell surface, leading them to conclude that cornichons act as endoplasmic reticulum (ER) chaperones (Brockie and Maricq, 2010; Shi et al., 2010). While the study of Schwenk et al. (2009) identified CNIH-2/3 immunoreactivity in various glial cells (including Bergmann glia and hippocampal astrocytes), the issue of whether cornichon association modifies surface AMPARs in glia has not been addressed. We chose to examine this question in OPCs. These immature glia, which give rise to oligodendrocytes responsible for axonal myelination, express both CP- and CI-AMPARs (De Biase et al., 2010) and can be prepared from optic nerve as pure cultures (Shi et al., 1998).
CNIHs are present at the surface of OPCs
We first examined the labeling of OPCs with an anti-CNIH antibody, used previously to identify cornichon expression in native tissue. This antibody recognizes both CNIH-2 and -3 (Schwenk et al., 2009) and, in our hands, labeled tsA201 cells transfected with CNIH-2 but not untransfected cells (data not shown). OPCs in culture were identified with an antibody to O4, a specific marker protein (Fig. 4). When permeabilized, OPCs displayed a high level of labeling with the CNIH-2/3 antibody, in both the soma and fine processes (Fig. 4a). Nonpermeabilized OPCs also exhibited intense surface labeling for CNIH-2/3, consistent with the presence of cornichon proteins in the cell membrane (Fig. 4b).
Functional properties of OPC AMPARs are influenced by CNIHs
To determine whether cornichons in the surface membrane of OPCs were likely to be associated with AMPARs that might be influencing their functional properties, we examined the kinetic behavior, rectification, and channel conductance of AMPARs in control cells and in cells overexpressing CNIH-3. Untreated OPCs exhibited I–V relationships with moderate inward rectification (Fig. 4c,d), consistent with the presence of a mixed population of CP- and CI-AMPARs. The relatively high channel conductance, estimated from NSFA (35.4 ± 4.2 pS, n = 7), suggested that in these untreated OPCs, AMPARs are normally associated with auxiliary subunits. Overexpression of CNIH-3 did not significantly alter the rectification of AMPAR currents (RI+60/−80 control 0.29 ± 0.04; + CNIH-3 0.30 ± 0.06; n = 3 each; p = 1.0) or channel conductance (+ CNIH-3 28.3 ± 2.2 pS; n = 8; p = 0.093), suggesting that the relative proportions of CP- and CI-AMPAR subunits were not greatly affected. However, the weighted mean time constant of desensitization (τdes) was increased from 6.2 ± 0.8 ms to 10.0 ± 0.8 ms (n = 9 and 11; p = 0.0034) (Fig. 4g). The effects of CNIH-3 on rectification, weighted-mean single-channel conductance, and τdes are compared in Figure 4h.
We next compared the effects of CNIH-3 on the desensitization of AMPARs in OPCs with the effects of CNIH-2, CNIH-3, and TARP γ-2 on the desensitization of recombinant AMPARs. Specifically, we examined the kinetics and relative proportions of the fast and slow components of desensitization (Fig. 5). For homomeric GluA1 CP-AMPARs, CNIH-2 and -3 preferentially slowed the fast component (τfast; Fig. 5a–c). For GluA1/A2 CI-AMPARs, CNIH-2 and -3 slowed both the fast and the slow components (τfast and τslow; Fig. 5d–f). This contrasts with the effect of TARP γ-2, which for both CP- and CI-AMPARs primarily decreased the relative proportion of the fast component of desensitization (Fig. 5a–f). In OPCs, the overexpression of CNIH-3 slowed τfast and τslow to similar extents, without changing their relative contribution (Fig. 5g–i). It is of note that in untreated OPCs, both components of desensitization appeared slower than would be expected for a mixed population of CP- and CI-AMPARs associated solely with TARP γ-2.
In an attempt to identify the potential contribution of cornichons to AMPARs in OPCs, we examined the relative amplitude of AMPAR-mediated currents elicited by kainate (IKA) and glutamate (IGlu) (1 mm each plus 100 μm CTZ). Previous studies have shown that AMPAR auxiliary subunits differentially increase the efficacy of the partial agonist kainate, thereby altering, to varying extents, the IKA/IGlu ratio (Tomita et al., 2005a; Turetsky et al., 2005; Shi et al., 2010). For GluA1 receptors, the effect of CNIH-3 was modest, with an approximately four-fold shift in the ratio (from 0.026 ± 0.004 to 0.10 ± 0.03; n = 4 and 5, respectively). This effect of CNIH-3 was significantly less (p = 0.029) than the 16-fold shift produced by γ-2 (to 0.43 ± 0.03, n = 7). With the coexpression of both CNIH-3 and γ-2, the IKA/IGlu ratio was similar to that with γ-2 alone (0.42 ± 0.08, n = 5; p = 0.52). For AMPARs in untreated OPCs, the IKA/IGlu ratio was 0.42 ± 0.04 (n = 6), similar to that of recombinant receptors in the presence of TARP or both TARP and cornichon.
Next, we examined the degree to which CTZ (100 μm) potentiated currents evoked by kainate (1 mm, −60 mV). With homomeric GluA1 receptors, IKA was increased ∼12-fold by CTZ (to 1294 ± 260% of control, n = 5). GluA1 receptors coexpressed with CNIH-3 were similarly potentiated (1234 ± 385%, n = 3; p = 1.00). By contrast, following coexpression with TARP γ-2 or with both γ-2 and CNIH-3, CTZ produced a much lesser effect (196 ± 18 and 326 ± 42% of control, respectively; n = 5 and 4; p = 0.037 and 0.040). This result is consistent with recent findings showing that CTZ potentiation of IKA is reduced for heteromeric GluA1/2/CNIH-2 receptors when coexpressed with TARP γ-8 (Kato et al., 2010b). In control OPCs, the CTZ potentiation (458 ± 55%, n = 7) was significantly greater than that seen with GluA1 plus γ-2 alone (p = 0.047) and closest to that seen with GluA1/γ-2/CNIH-3 coexpression (p = 0.47), providing suggestive evidence that the receptors in OPCs may be associated with both TARP and cornichon.
Finally, as we have recently shown that the prevalence of CP-AMPARs in OPCs can be dynamically regulated in a TARP-dependent manner by the activation of Group 1 mGluRs and purinergic receptors (Zonouzi et al., 2011), we asked whether such changes in AMPAR expression might be accompanied by changes in CNIH association. After treatment of OPCs with ATP (1 mm for 10 min at 37°C) (Zonouzi et al., 2011), which promotes a switch toward CI-AMPARs, the CTZ potentiation of IKA (396 ± 42%, n = 5) remained similar to GluA1/γ-2/CNIH-3 (p = 0.66) and different from GluA1 plus γ-2 alone (p = 0.049).
Discussion
CNIHs and TARPs similarly modify AMPAR gating but have different effects on pharmacology
In this study, we have recorded macroscopic and single-channel currents to examine the effects of CNIHs on the properties of recombinant and native AMPARs, concentrating on the behavior of CP-AMPARs. Our data indicate that CNIH-2 and -3 slow the kinetics of CP-AMPARs, increase their glutamate sensitivity, increase their single-channel conductance, and increase calcium-permeability while reducing their block by intracellular polyamines. Thus, CNIH association would be expected to enhance the activation of and calcium flux through CP-AMPARs. These effects of CNIHs are largely comparable to those described previously for TARPs. However, more detailed kinetic analysis suggests that the TARPs and CNIHs differ in the means by which they slow desensitization: CNIHs decrease the rate of both the slow and the fast components, while γ-2 increases the proportion of the slower component.
A clear difference between CNIHs and TARPs is seen in their effects on kainate efficacy, which are greater for the TARPs than the CNIHs. Our data demonstrate that additional expression of CNIH-3 does not change the IKA/IGlu ratio of GluA1/γ-2 assemblies but does increase the CTZ sensitivity of IKA, indicating that CNIHs can interact with and modify the AMPAR/TARP complex. These effects are similar to those seen with coexpression of CNIH-2 with GluA1 and γ-8 (Kato et al., 2010b) or with a GluA1-γ-8 chimera (Shi et al., 2010). Thus, detailed kinetic analysis and examination of kainate pharmacology can be used to evaluate the TARP/CNIH content of native receptors.
CNIHs are expressed at the surface of glial cells
The functional importance of CNIHs in neurons has been the subject of controversy. Initial suggestions that CNIHs and TARPs were not found in the same receptor complexes (Schwenk et al., 2009) and failed to traffic to the neuronal surface (Shi et al., 2010) led to the hypothesis that CNIHs were simply responsible for biosynthetic trafficking of AMPARs intracellularly. This would represent conservation of the role performed by CNIH homologs in Drosophila and yeast (Cni and Erv14p), which participate in protein maturation by facilitating the export of nascent protein from the ER to the Golgi apparatus in CopII vesicles (Bokel et al., 2006; Castillon et al., 2009). By contrast, data from Kato et al. (2010b) suggested that CNIH-2 could functionally interact with AMPARs containing TARP γ-8, both in the hippocampus and in cerebellar granule neurons from stargazer mice transfected with γ-8. Recent evidence suggests that in hippocampal and cerebellar neurons the presence of CNIH-2 can alter AMPAR/TARP stoichiometry, although it associates with surface AMPARs only in the presence of specific TARPs (Gill et al., 2011). Thus, it now seems clear that CNIHs can interact with neuronal AMPARs in the presence of TARPs to modulate receptor function.
Although CNIH2/3 isoforms have previously been identified in Bergmann glia by immunocytochemistry (Schwenk et al., 2009), we have demonstrated, for the first time, that they have functional effects on AMPARs in glial cells. We have shown that CNIH-2/3 immunoreactivity is present at the surface of OPCs and that, when overexpressed, CNIH-3 can modulate the kinetic and pharmacological properties of AMPARs. While some of the pharmacological aspects of OPC AMPAR responses could be attributed to CNIH coassembly, this does not conclusively demonstrate that CNIHs are elements of AMPAR signaling in OPCs. Nevertheless, taken at face value, our data suggest that surface AMPARs in OPCs may not normally be saturated with CNIHs. The incorporation of CNIHs in AMPAR subunit assemblies may occur at the expense of TARP components (Gill et al., 2011, 2012) or may simply lead to receptors with additional auxiliary subunits. OPCs express several TARP isoforms (Cahoy et al., 2008), and we have shown recently that γ-2 is important for both constitutive trafficking and mGluR-mediated insertion of GluA2-lacking CP-AMPARs in these cells (Zonouzi et al., 2011). The additional presence of mRNA for γ-3, γ-4, and γ-5 (Zonouzi et al., 2011) and CNIH-2/3 protein (Fig. 4), together with a mixed population of CP- and CI-AMPARs (Fig. 4), suggests the potential for significant AMPAR heterogeneity in OPCs. The IKA/IGlu ratio we obtained in OPCs is consistent with the presence of Type I TARPs (either with or without CNIHs). However, the presence of receptors containing CNIH-2/3 is suggested by the degree of potentiation of IKA by CTZ, which is larger than would be expected for AMPARs associated with TARP alone. Furthermore, both the slow and fast time constants of AMPAR desensitization in OPCs are slower than those expected for CNIH-free receptors (Fig. 5). Thus, our electrophysiological data are in line with the emerging view that TARPs and CNIHs not only interact with the same AMPARs at the cell surface but that their precise stoichiometries dictate the properties of AMPAR populations (Gill et al., 2011, 2012).
CNIHs and OPC AMPAR plasticity
In OPCs, the prevalence of CP-AMPARs can be dynamically regulated, in a TARP-dependent manner, by activation of metabotropic glutamate and purinergic receptors (Zonouzi et al., 2011). In the present study, we found that following exposure to ATP (which induces a switch to CI-AMPARs) the kainate pharmacology of the receptors was unchanged, suggesting the dual presence of TARPs and CNIHs, both before and after plasticity. It is tempting to speculate that synaptic plasticity in neurons expressing CNIHs, such as hippocampal CA1 neurons, may also involve the trafficking of CNIH-containing receptors. The exact mechanisms underlying AMPAR plasticity in OPCs are not yet fully understood, but it is likely that new cell surface receptors originate from intracellular pools or from the extrasynaptic membrane (Shi et al., 1999; Bats et al., 2007). While modification of TARPs by phosphorylation can facilitate AMPAR cell surface trafficking and lateral diffusion in the membrane (Tomita et al., 2005a; Bats et al., 2007; Opazo et al., 2010; Sumioka et al., 2010) a direct role of CNIHs in plasticity has not been described. It is possible that CNIHs are passive in this regard, with post-Golgi receptor trafficking being dictated by the TARPs. However, it is also possible that CNIHs play a specific role in plasticity, either by directly dictating receptor trafficking or by influencing this indirectly by modifying TARP stoichiometry. Further studies are required to resolve these issues. During development, OPCs receive glutamatergic inputs from neurons (Bergles et al., 2000), which influence oligodendrocyte migration (Gudz et al., 2006). The means by which AMPARs in OPCs are trafficked and targeted to these “synaptic” sites is unresolved, but CNIH-2/3, by enhancing steady state currents, assisting receptor biogenesis, or facilitating AMPAR plastic changes, may influence the processes responsible for establishing such connections.
Footnotes
The authors declare no competing financial interests.
This work was supported by programme grants from the Wellcome Trust and the Medical Research Council (S.G.C.-C., M.F.). Cornichon cDNAs and antibody to CNIH-2/3 were gifts from Bernd Fakler (University of Freiburg, Freiburg, Germany), and TARP cDNAs were gifts from Roger Nicoll (University of California, San Francisco, San Francisco, CA). M.Z. was supported by the Medical Research Council studentship programme of the Laboratory of Molecular Cell Biology, University College London. We thank Cécile Bats and Dorota Studniarczyk for discussion.
- Correspondence should be addressed to either Mark Farrant or Stuart G. Cull-Candy, Department of Neuroscience, Physiology and Pharmacology, University College London, Gower Street, London WC1E 6BT, United Kingdom. m.farrant{at}ucl.ac.uk or s.cull-candy{at}ucl.ac.uk