Kainate Binding Proteins Possess Functional Ion Channel Domains

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Volume 17, Number 20, Issue of October 15, 1997 pp. 7634-7643
Copyright ©1997 Society for Neuroscience

Kainate Binding Proteins Possess Functional Ion Channel Domains

Carmen Villmann, Leonard Bull, and Michael Hollmann
Glutamate Receptor Laboratory, Max-Planck-Institute for Experimental Medicine, D-37075 Göttingen, Germany

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Kainate binding proteins (KBPs) are highly homologous to ionotropic glutamate receptors; however, no ion channel functionhas been demonstrated for these proteins. To investigate possiblereasons for the apparent lack of ion channel function we transplantedthe ion channel domains of five KBPs into glutamate receptorsGluR 6 and GluR1. In each case we obtained functional chimericreceptors in which glutamatergic agonists were able to open theKBP-derived ion channel with EC₅₀ values identical to those ofthe subunit contributing the ligand binding domain. Maximal currentamplitudes were significantly smaller than those of the parentclones, however. We also show that the KBP ion channels are highlypermeable for calcium and have certain pharmacological propertiesthat are distinct from all other glutamate receptor (GluR) subunits.Thus, all five known KBPs, in addition to their well characterizedfunctional ligand binding sites, have functional ion permeationpathways. Our data suggest that the lack of ion channel functionin wild-type KBPs results from a failure to translate ligand bindinginto channel opening. We interpret our findings to indicate therequirement for a modulatory protein or an additional subunitserving to alter the structure of the KBP subunit complex suchthat signal transduction is enabled from the ligand binding siteto the intrinsically functional ion pore.
Key words: kainate binding proteins; KBP; ion pore; domain transplantation; kainate receptors; GluR1; GluR6; calcium permeability; Xenopus oocytes

INTRODUCTION

Ionotropic glutamate receptors (GluRs) are the prevalent excitatory neurotransmitter receptors in the CNS of vertebrates.Three pharmacologically distinct types have been identified throughmolecular cloning: AMPA receptors, kainate (KA) receptors, andNMDA receptors (for review, see Hollmann and Heinemann, 1994).In addition to GluR subunits, which form functional ion channels,several homologous subunits have been characterized that lackapparent intrinsic ion channel function and do not seem to formfunctional heteromeric complexes with other subunits. These includethe kainate binding proteins (KBPs) (Gregor et al., 1989; Wadaet al., 1989; Wo and Oswald, 1994, Ishimaru et al., 1996; forreview, see Henley, 1994) and several orphan receptors (Hollmannand Heinemann, 1994).

The KBPs are ~50 kDa proteins that bind kainate receptor agonists such as Glu, KA, and domoate (Dom) (Wada et al., 1989);however, the physiological role of these proteins remains enigmatic(Henley, 1994). In the KBP subfamily, five different genes havebeen identified from five different species: one subunit eachfrom the frog Rana pipiens [KBP(Rp)], the chicken Gallus domesticus[KBP(Gd)], the toad Xenopus laevis [KBP(Xl)], and the duck Anasdomesticus [KBP(Ad)], and two different subunits from the goldfishCarassius auratus [KBP(Ca) $alpha$ and KBP(Ca) $beta$ ]. KBP(Gd) and KBP(Ad)are 92.8% identical at the amino acid level, indicating that theyrepresent the same gene. The other subunits share between 49.8and 67.9% sequence identity and thus are derived from differentgenes. Notably, no KBPs have been discovered in mammals.

There is significant sequence homology (35-40%) between KBPs and other GluRs, particularly the KA receptors. In addition,their transmembrane topology is believed to be identical to thatof other GluRs (Hollmann et al., 1994; Wo and Oswald, 1994). Themost compelling structural difference between KBPs and other GluRsis their short N-terminal domains (128-148 amino acids as opposedto ~520 for other GluR subunits), which is characteristic forall KBPs (see Fig. 1).
Fig. 1. Bar graph representation of the structural features of receptor subunits used for ion pore transplantation. KBPs of Rana pipiens(Rp), Gallus domesticus (Gd), Carassius auratus (Ca, two subunits, $alpha$ and $beta$ ), and Xenopus laevis (Xl) are compared with the AMPA receptorGluR1 and the KA receptor GluR6. The chimera GluR6N-KBP(Rp)C isa construct with an N-terminal transplantation between GluR6 (N-terminalpart) and KBP(Rp) (C-terminal part); the black circle marks thejunction between the two domains. Chimera GluR6-Rp-R6-Rp (bottombar) is derived from GluR6N-KBP(Rp)C by exchanging the pore domainfor that of GluR6(Q). The predicted signal peptides, the threetransmembrane domains (TMD A, TMD B, TMD C) and the pore loopdomains (the "TMD II" of previous topology models) are indicatedby black rectangles.
[View Larger Version of this Image (21K GIF file)]

To gain insight into the biological role of KBPs we set out to determine whether KBPs could potentially form functional ionchannels. We chose a domain transplantation strategy that involvedengineering of the ion channel domain of KBPs into functionalGluR subunits. This approach was based on recent suggestions thatGluRs may be modular proteins made up of building blocks derivedfrom different precursor proteins (Seeburg et al., 1995; Wo andOswald, 1995; Hollmann, 1996), a design that should allow domainexchange among subunits.

The domain transplantation experiments described in this study identified the putative ion channel domains of all five KBPgenes [KBP(Rp), KBP(Gd), KBP(Ca) $alpha$ , KBP(Ca) $beta$ , and KBP(Xl)] as sequencescapable of forming functional cation conduction pathways withdistinct pharmacological properties. Moreover, these domains arecapable of coupling to glutamatergic ligand binding sites, andthey permit the flow of calcium ions.

MATERIALS AND METHODS
Mutagenesis. To allow easy exchange of ion pores between subunits, unique restriction sites were introduced into both donorand acceptor subunits by PCR-based mutagenesis. Homologous positionswithin each sequence were chosen to engineer an EcoRI site downstreamof the pore region at amino acids 211-213 (RII) in KBP(Rp) (thecDNA clone was kindly provided by Drs. K. Wada and R. Wenthold,National Institutes of Health) and at the corresponding aminoacids in GluR6(Q) (603-605, RIV) and GluR1 (595-597, RIV). Numberingstarts with the first codon of the mature protein. Upstream ofthe pore region an Nru I site was introduced at amino acids 163-165(FLV) in KBP(Rp), at amino acids 548-560 (FVI) in GluR6(Q), andat amino acids 537-539 (FLV) in GluR1 (see Fig. 2). The siteswere chosen such that the entire pore region including both adjacentintracellular loops (L1 and L2) (Hollmann et al., 1994) was transplanted.The resulting constructs were named "x-PCS," where "x" standsfor the clone modified and "PCS" means "pore cassette sites".Mutagenetic oligonucleotide primers of 21-36 bp length were obtainedfrom Eurogentec (Seraing, Belgium). A fragment containing bothnewly generated restriction sites was synthesized in a first roundof PCR. The purified fragment was extended C-terminally in a secondPCR using wild-type DNA as the template and a tailed primer bindingdownstream of the gene within the vector sequence. The vectorused throughout this study was pSGEM, a modified version of pGEMHEin which we replaced the original multiple cloning site by thepBluescript (Stratagene, Heidelberg, Germany) polylinker; furthermore,two additional sites for template linearization (the eight-cuttersPacI and SfiI) were inserted between the existing SphI and NheIsites. The original pGEMHE vector was kindly provided by EmilyLiman and the late Peter Hess (Harvard Medical School). In a thirdround of PCR the second-round fragment was N-terminally extendedusing primers binding to the T7 promoter of pSGEM and the tailsequence generated in the second round of PCR, respectively, sothat only the mutated strand will be amplified.
Fig. 2. Amino acid sequence alignment of the transplanted ion pore regions (the sequence between the end of TMD A and the start ofTMD B) of the five KBPs (see legend to Fig. 1), GluR1, and GluR6(Q).Flanking the sequences to be exchanged are three amino acids shownin bold that were mutated to obtain the consensus sequences FAIand RIL shown at the bottom, thereby introducing unique restrictionsites as indicated. The Q/R editing site of AMPA and KA receptorsis marked by an arrow.
[View Larger Version of this Image (31K GIF file)]

PCRs were set up as follows: 1 ng of template DNA, 200 mM Tris-HCl, pH 8.8, 100 mM KCl, 100 mM (NH₄)₂SO₄, 20 mM MgSO₄, 1%Triton X-100, 1 mg/ml bovine serum albumin, 50 µM each dATP, dCTP,dTTP, and dGTP, 100 pmol of each primer, and 2 U Pfu polymerase(Stratagene). PCR conditions were 5 min/95°C for denaturation,5 min/50°C for annealing, 5 min/72°C for elongation in the firstcycle, followed by 28 cycles of 1 min/95°C, 2 min/50°C, and 2.5min/72°C. The last cycle ended with a 10 min/72°C amplificationstep.

The final PCR fragments were cut with suitable restriction sites as close as possible to the region to be transplanted andwere reinserted into the respective wild-type clones to minimizeany PCR-generated sequence. The following cloning cassettes wereused for shuttling: EcoRV-AccI [nucleotide (nt) 1685-1950] forGluR6(Q), BglII-BglII (nt 1810-2220) for GluR1, and AflIII-XcmI (nt 455-720) for KBP(Rp). The resulting mutants were designatedGluR6(Q)-PCS, GluR1-PCS, and KBP(Rp)-PCS, respectively, and wereused as recipient clones of the pore regions to be transplanted.Next, PCR-amplified fragments of the pore domains of GluR6(Q),KBP(Rp), KBP(Ca) $alpha$ , KBP(Ca) $beta$ , KBP(Gd), and KBP(Xl) were generatedto include the required flanking EcoRI and Nru I sites, usingthe appropriate mutagenetic primers. These fragments were digestedwith EcoRI and Nru I and ligated into the appropriate recipientclones, GluR1-PCS, GluR6(Q)-PCS, or KBP(Rp)-PCS, which had beenprepared for ligation by digestion with EcoRI and Nru I. The originalcDNA clones of the KBPs were used as starting material. Clonesof these KBPs were generously provided by Dr. R. Oswald (CornellUniversity) (KBP(Ca) $alpha$ and KBP(Ca) $beta$ ) and Dr. V. Teichberg (WeizmannInstitute) (KBP(Gd)). For the recently cloned KBP(Xl) (Ishimaruet al., 1996), a cDNA clone was not available to us. We thereforeused an 865 bp PCR-generated fragment (nt 241-1105) amplifiedfrom Xenopus cDNA that had been reverse-transcribed from totalbrain mRNA isolated from 10 female Xenopus laevis.

All mutant clones were sequenced across the PCR-generated fragment with the Sequenase 2.0 sequencing kit (United States Biochemicals,Braunschweig, Germany), which uses the dideoxynucleotide chaintermination method (Sanger et al., 1977). Sequence data were analyzedwith the University of Wisconsin software package (Devereux etal., 1984).

cRNA synthesis. Template DNA was linearized with NheI. cRNA was synthesized from 1 µg of linearized DNA using an in vitrotranscription kit (Stratagene) with a modified protocol that uses800 µM each nucleotide (except GTP, 200 µM), 800 µM ^m7GpppG (Pharmacia, Freiburg, Germany) for capping, and an extendedreaction time of 3 hr with T7 polymerase. Trace labeling was performedwith [³²P]UTP to allow calculation of yields and transcript quality checkby agarose gel electrophoresis.

Electrophysiological measurements in Xenopus oocytes. Oocytes of stages V-VI were surgically removed from the ovaries of Xenopuslaevis anesthetized with 3-aminobenzoic acid ethylester (2.3 gm/l).The oocytes were incubated in calcium-free Barth's solution (seebelow) containing 815 U/ml (=2.8 mg/ml) collagenase and 2200 U/ml(=0.15 mg/ml) trypsin for 2.75 hr while they were gently shakento remove the follicular cell layer. Oocytes were washed fiveto six times in Barth's solution (88 mM NaCl, 1.1 mM KCl, 2.4mM NaHCO₃, 0.3 mM Ca(NO)₃, 0.3 mM CaCl₂, 0.8 mM MgSO₄, 15 mM HEPES-NaOH,pH 7.6). After selection the oocytes were kept in Barth's solutioncontaining 63 µg/ml penicillin, 40 µg/ml streptomycin, and 100µg/ml gentamycin; 10 ng (=50 nl) of cRNA was injected into theoocytes using a 10 µl Drummond microdispenser. Two-electrode voltage-clamprecordings were performed with a TurboTec 10CD amplifier (npi,Tamm, Germany) 4-8 d after cRNA injection by superfusion of theoocyte with glutamatergic agonists (1-300 µM) prepared in normalfrog Ringer's solution (NFR) (115 mM NaCl, 2.5 mM KCl, 1.5 mMCaCl₂, 10 mM HEPES-NaOH, pH 7.2). Voltage electrodes were filledwith 3 M KCl and had resistances of ~4 M $Omega$ ; current electrodeswere filled with 3 M CsCl and had resistances of ~0.5-1.5 M $Omega$ .Oocytes were held at $-$ 70mV. All measurements of clones based onthe KA receptor GluR6 were performed after preincubation of theoocyte with 1 mg/ml concanavalin A (ConA) for 8 min. This treatmenteliminates desensitization of KA receptors, particularly GluR6(Egebjerg et al., 1991). Agonists were applied for 10 sec by superfusionof the oocyte at a flow rate of 10-14 ml/min. Current-voltage(I-V) relationships were determined with a 2 sec voltage rampand analyzed using the PulseFit 7.62 program (HEKA Electronics,Lambrecht, Germany). To determine the EC₅₀ values for KA and Glu,8-10 different agonist concentrations were applied to the sameoocyte, and steady-state values of the evoked currents were measured.Data from each oocyte were fitted separately, and EC₅₀ valuesobtained this way from three to five oocytes were averaged. Calciumpermeability tests were performed in low or high "Ca-Ringer" lackingany other permeable cation. Both 10 mM Ca-Ringer (10 mM HEPES,10 mM CaCl₂, 105.2 mM N-methyl-D-glucamine, pH 7.2, adjusted withconcentrated HCl) and 80 mM Ca-Ringer (80 mM CaCl₂, 10 mM HEPES,pH 7.2, adjusted with N-methyl-D-glucamine) were used.

Gel electrophoresis and immunoblotting. Batches of 12 oocytes were used for membrane preparations 6-8 d after cRNA injection,following a previously described protocol (Hollmann et al., 1994).For experiments in which only those proteins inserted into theplasma membrane were to be analyzed, membrane preparations wereperformed after biotinyl-ConA labeling of glycosylated surfaceproteins and streptavidin-Sepharose-mediated precipitation oflabeled proteins. Briefly, the oocytes were incubated in 10 µMbiotinyl-ConA (Sigma, Munich, Germany) in NFR for 30 min at roomtemperature (RT). After five washes for 10 min each in NFR, oocyteswere homogenized with a Teflon pestle in 240 µl H-buffer (100mM NaCl, 20 mM Tris-HCl, pH 7.4, 1% Triton X-100, 1 mM phenylmethylsulfonylfluoride plus a cocktail of additional proteinase inhibitors:2.5 µg/ml leupeptin, 20 µg/ml aprotinin, 2.5 µg/ml pepstatin,and 20 µg/ml benzamidine hydrochloride) and kept on ice for 15min. After centrifugation for 60 sec at 16,000 × g, the supernatantswere supplemented with 20 µM washed streptavidin-Sepharose beads(Sigma) and incubated for 3 hr at 4°C on a rotator. The streptavidin-Sepharosebeads were pelleted by a 60 sec spin and washed three times withH-buffer, and the final pellets were boiled in 40 µl/oocyte SDS-PAGEloading buffer (0.8 M $beta$ -mercaptoethanol, 6% SDS, 20% glycerol,25 mM Tris-HCl, pH 6.8, 0.1% bromphenol blue).

Samples were run on 20 cm discontinuous SDS-PAGE gels (Laemmli, 1970) (5% stacking gel, 7.5% separating gel; running time2.5 hr at 4°C). Prestained protein markers (Bio-Rad, Munich, Germany)were used to monitor separation on the gel as well as to identifythe position of immunoreactive bands on blots. The gel was blotted(Towbin et al., 1979) onto Hybond ECL nitrocellulose membranes(Amersham, Braunschweig, Germany) at a constant current of 200mA for 16 hr at 4°C. Filters were blocked for 2 hr at RT withblocking buffer [1× Roti-block (Roth, Karlsruhe, Germany) in 140mM NaCl, 0.1% Triton X-100, 20 mM Tris-HCl, pH 7.6] and probedovernight at 4°C with affinity-purified rabbit antisera directedagainst the C termini of GluR6 (peptide sequence TFNDRRLPGKETMA)(Wenthold et al., 1994) or KBP(Rp) (peptide sequence KSPTSNSCDEVKA).Both antibodies were kindly provided by Dr. Robert Wenthold. Incubationswere performed in 0.1× Roti-block, 0.1% Triton X-100, 140 mM NaCl,20 mM Tris-HCl, pH 7.6. Peroxidase-labeled donkey anti-rabbitIgG (Dianova, Hamburg, Germany) was used as secondary antibody.Immunoreactive bands were visualized by the chemoluminescencemethod (ECL detection kit, Amersham).

Reagents. Restriction enzymes were purchased from Boehringer Mannheim (Mannheim, Germany), Promega (Mannheim, Germany), andNew England Biolabs (Schwalbach, Germany). All nucleotides werefrom Pharmacia (Freiburg, Germany). Unless noted otherwise, allchemicals were from Sigma.

RESULTS

N-terminal elongation of KBPs
The most obvious structural difference between functional members of the GluR family and the nonfunctional KBPs is the shortN-terminal domain of the latter (Fig. 1). To test whether an extendedN-terminal domain would render KBPs functional, we engineeredthe N-terminal sequence of the KA receptor GluR6 (comprising aminoacids 1-399) onto the KBP from Rana pipiens. Amino acid 22 (alysine) of wild-type KBP(Rp) was used as the N-terminal pointof connection to create the chimera GluR6N-KBP(Rp)C (Fig. 1).Unfortunately, this chimera was not functional on expression inXenopus oocytes (data not shown), although the protein was expressedand inserted into the oocyte plasma membrane (see Fig. 4C). Coexpressionof wild-type GluR6(Q) did not enhance expression levels (see Fig.4C, right lane) and did not produce any alterations of the functionalproperties found for GluR6(Q) alone (data not shown).
Fig. 4. Western blots demonstrating protein expression of chimeric receptors. A, GluR6(Q) wild-type compared with pore transplantationchimeras of GluR6. B, KBP(Rp) wild-type compared with pore transplantationchimeras of KBP(Rp). C, N-terminus transplantation chimeras betweenGluR6 and KBP(Rp). Total oocyte proteins (T, 1 oocyte/lane), streptavidin-precipitatedbiotinyl-ConA-labeled plasma membrane proteins (P, 10 oocytes/lane),and nonbiotinylated controls (P $-$ , 10 oocytes/lane) were separatedelectrophoretically, blotted, and probed with affinity-purifiedantibodies generated to the C-terminal peptide of GluR6 (A) orthe C-terminal peptide of KBP(Rp) (B, C). Arrows point to theposition of the ~120 kDa GluR6 wild-type and pore transplantationmutant proteins in A, to the position of the ~48 kDa KBP in B,and to the position of the ~118 kDa N-terminal transplantationchimeras between GluR6 and KBP in C. Note that in A an unidentifiedband cross-reacting with the GluR6 antibody (marked by an asterisk)is present in all control precipitations and even in uninjectedoocytes (panels P, P $-$ ). This band is absent from the total oocyteprotein (panel T) because only a single oocyte was loaded in thatcase as opposed to 10 oocytes for panels P and P $-$ . Note also thatspecific bands (arrows) are either totally absent (B, C) or onlyvery weak (A) in precipitation control samples (P $-$ ) that werenot biotinyl-ConA-labeled. This demonstrates that the immunoreactiveprotein identified in panel P is actually residing in the plasmamembrane. KBP(Rp)-PGluR1 in B runs at a slightly larger molecularweight than expected. This erratic running behavior is not attributableto a sequence problem in the construct but likely reflects a conformationalpeculiarity of this particular construct.
[View Larger Version of this Image (26K GIF file)]

Transplantation of KBP ion pores into functional channels
Another domain critically involved in channel function is obviously the ligand binding site. This domain, however, has alreadybeen well established as a functional site on all cloned KBPsthrough agonist binding experiments with ³H-KA (Gregor et al., 1989; Wada et al., 1989; Wo and Oswald, 1994,Ishimaru et al., 1996). An equally important domain that has notreceived nearly as much attention is the ion channel domain itself.If this domain was intrinsically defective or nonfunctional, obviouslyno ionic currents would be possible even after binding of theproper ligand. We therefore transplanted the putative ion channeldomain of KBP(Rp) into functional GluR subunits to test the intrinsicfunctionality of the channel domain in the context of proven functionalsubunits. We chose the AMPA receptor GluR1 (45.9% sequence identityat the amino acid level) and the KA receptor subunit GluR6, whichis the most closely related subunit (51.5% sequence identity),as donors for the ligand binding site. The excision points ofthe transplanted ion channel domain from KBP(Rp) and the correspondinginsertion points in GluR1 and GluR6 were chosen such that theentire hairpin loop comprising the putative channel-lining segmentcould be transplanted together with the flanking intracellularloops L1 and L2 as defined in Hollmann et al. (1994). The transplantedsequence starts at the C-terminal end of transmembrane domain(TMD) A and runs up to the N-terminal end of TMD B. To facilitateion pore exchange between various receptor subunits, we insertedunique restriction enzyme sites at the starting points and endpoint of the region to be transplanted. The resulting constructsmade from GluR1, GluR6, and KBP(Rp) were named GluR1-PCS, GluR6-PCS,and KBP(Rp)-PCS, respectively (Fig. 2) (also see Materials andMethods). They served as the parent constructs for all ion channeltransplantations performed for this study.

Both chimeric constructs, GluR1-PKBP(Rp) and GluR6-PKBP(Rp), gave functional ion channels that could be activated by KA, Glu,and Dom (Fig. 3B,D). Maximal current amplitudes of GluR1-PKBP(Rp)(6.3 ± 0.4 nA for KA currents; n = 7) and GluR6-PKBP(Rp) (9.03± 0.2 nA; n = 39) were rather small compared with those of wild-typeGluR1 (3157 ± 711 nA for KA currents; n = 4) and wild-type GluR6(14550 ± 1892 nA; n = 4), respectively (~1%). They could be reproduciblymeasured in every oocyte tested, however, provided that currentdesensitization was minimized by ConA pretreatment of oocytesexpressing GluR1-PKBP(Rp) and GluR6-PKBP(Rp) (see Materials andMethods). Additionally, cyclothiazide was coapplied for recordingsof GluR1-PKBP(Rp), because this compound specifically blocks desensitizationat AMPA receptors (Partin et al., 1993). Interestingly, despitethe pronounced difference between wild-type GluR1 and GluR6 inmaximal current amplitudes (the ratio found was 1:~4.6), the twochimeras GluR1-PKBP(Rp) and GluR6-PKBP(Rp) had similar currents(a ratio of 1:~1.4), indicating that the transplanted KBP porerather than the sequence background of the ligand binding sitedonor subunit determined the maximal currents.
Fig. 3. Sample current traces of the receptor constructs GluR1-PCS (A) and GluR6(Q)-PCS (C), which had been engineered for easy poretransplantation (see Materials and Methods), and of chimeric receptorsharboring the ion pore domains of various KBPs (B, D-H). Agonistsused were kainate (KA, 100 µM in C-H; 300 µM in A, B), glutamate(GLU, 300 µM), and domoate (DOM, 10 µM). To minimize desensitization,all clones were treated with 10 µM ConA before recording; in addition,for GluR1-derived clones (A, B), 100 µM cyclothiazide was coappliedwith the agonist.
[View Larger Version of this Image (22K GIF file)]

To test whether the ion channel domains of other KBPs were similarly capable of conducting currents, we engineered the respectivedomains of KBP(Xl) (Ishimaru et al., 1996), KBP(Ca) $alpha$ and KBP(Ca) $beta$ (Wo and Oswald, 1994), and KBP(Gd) (Gregor et al., 1989) intoGluR6 using the same strategy as described above for KBP(Rp) (fordetails, see Materials and Methods). All chimeras containing KBPion channel transplants were expressed at the protein level (Fig.4A, panel T) and were inserted into the plasma membrane (Fig.4A, panel P), and all were functional (Fig. 3E-H). GluR6-PKBP(Ca) $alpha$ gave the largest maximal amplitudes (Table 1), which were inthe range of 7% of wild-type GluR6(Q) or 17% of GluR6(Q)-PCS (seeMaterials and Methods) for both Glu- and KA-evoked currents.

Table 1. EC₅₀ values of GluR6 and chimeras containing ion pores from KBPs of different species

Clone EC₅₀ KA n_H I_max [nA] n EC₅₀ GLU n_H I_max [nA] n

GluR6(Q) wild type 1.74 ± 0.72 1.09 ± 0.11 6224 ± 1487 3 34.4 ± 6.2 1.2 ± 0.12 9898 ± 2042 3

GluR6(Q)-PCS 2.2 ± 0.06 0.97 ± 0.06 667 ± 179 4 59.9 ± 4.8 1.2 ± 0.06 695 ± 132 3

GluR6-PKBP(Rp) 2.4 ± 0.15 1.4 ± 0.1 8.02 ± 1.13 4 35.7 ± 7.35 1.78 ± 0.2 6.47 ± 1.9 5

GluR6-PKBP(Gd) 6.0 ± 1.4 0.93 ± 0.08 6.0 ± 0.7 5 47.2 ± 1.6 1.35 ± 0.02 10.61 ± 1.2 3

GluR6-PKBP(Ca) $alpha$ 2.16 ± 0.05 1.64 ± 0.26 55.9 ± 16.2 4 49.9 ± 2.8 1.47 ± 0.04 58.7 ± 10.8 4

GluR6-PKBP(Ca) $beta$ 2.9 ± 0.8 1.06 ± 0.1 11.03 ± 3.4 4 35.6 ± 2.3 1.26 ± 0.1 18.4 ± 5.5 4

GluR6-PKBP(XI) 2.25 ± 0.53 0.95 ± 0.04 7.9 ± 2.25 4 44.4 ± 7.5 1.1 ± 0.17 8.1 ± 1.12 3

Half-maximal efficient concentrations (EC₅₀) for kainate (KA) and glutamate (Glu), Hill coefficients (n_H), as well as maximalcurrent amplitudes (I_max) are listed ± SEM; n, number of oocytestested. PCS, Clone-engineered for easy pore cassette exchange(containing unique restriction sites flanking the pore; see Materialsand Methods for details). GluR6-PKBP(Nn), GluR6 containing thepore domain of a KBP; "Nn" stands for the abbreviation of theLatin names of the species from which the KBP ion pore originated(Rp = Rana pipiens; Gd = Gallus domesticus; Ca = Carassius auratus,genes $alpha$ and $beta$ ; XI = Xenopus laevis).

We recorded dose-response curves for KA- and Glu-evoked currents of wild-type GluR6(Q), GluR6(Q)-PCS, and the five chimerasharboring KBP ion pores. The mutant GluR6(Q)-PCS, which carriesthe engineered sites for ion channel exchange but has the originalion channel domain of GluR6(Q), displays a small (1.7-fold) decreasein Glu affinity compared with wild-type GluR6(Q), whereas theaffinity for KA is unchanged (Table 1). When we analyzed thechimeras we did not find significant differences in the EC₅₀ valuesof KA-evoked currents compared with GluR6(Q)-PCS (Fig. 5A,B),except for GluR6-PKBP(Gd), in which we measured a modest increasein the EC₅₀ (approximately threefold) (Table 1). For Glu-evokedcurrents we observed no major changes in the EC₅₀ values (Fig.5C,D), with none of the EC₅₀ deviating by more than a factor of1.7 from the agonist affinity of GluR6(Q)-PCS (Table 1). Moreover,those chimeras deviating most from GluR6(Q)-PCS had EC₅₀ valuesclose to that of wild-type GluR6(Q). Therefore, construction ofthe chimeras had little effect on the affinities for any of theagonists and thus evidently had no major impact on the ligandbinding site.
Fig. 5. Comparison of dose-response curves of GluR6(Q)-PCS and chimeric GluR6 receptors harboring the ion pore domains of KBP(Ca) $alpha$ (A, C), KBP(Ca) $beta$ (A, C), KBP(Rp) (B, D), KBP(Gd) (B, D), or KBP(Xl)(B, D). Note lack of significant changes in EC₅₀ values with eitherKA (A, B) or Glu (C, D) as the agonist. Each data point representsthe average of three to five oocytes ± SEM, as indicated. SeeMaterials and Methods for details. For EC₅₀ values and maximalcurrents, see Table 1.
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Channel properties of KBP-GluR6 chimeras
The wild-type GluR6(Q) is characterized by an inwardly rectifying I-V relationship (Egebjerg and Heinemann, 1993), indicatingthat outward currents are blocked, presumably by endogenous compoundssuch as spermine (Bowie and Mayer, 1995). This block of outwardcurrent is determined mainly by the so-called Q/R-site, whereeither a glutamine (Q) or an arginine (R) residue is found tobe located at the presumably most narrow position of the ion channel.The amino acid present at this site is determined by RNA editing(Seeburg, 1996). We recorded I-V curves of GluR6(Q)-PCS and thefive chimeras (Fig. 6A,B) and determined that all of them hadinwardly rectifying I-V relations. Thus, the ion channel of KBPsis susceptible to block of outward current just like the AMPAand KA receptor channels; however, the five chimeras, unlike GluR6(Q)and GluR6(Q)-PCS, did show a small but significant current atpositive membrane potentials (Fig. 6A,B). This small outward currentis not attributable to the activation of calcium-dependent chloridechannels, which are endogenous to the oocyte (and which have linearI-V relations), because they persist even in a buffer in whichcalcium has been replaced by magnesium (Fig. 6C, trace 2). Wespeculated that this outward current might be attributable tothe fact that in all KBPs cloned so far a leucine is located atthe site equivalent to the Q/R editing site of GluR6. We thereforemutated the glutamine at the Q/R-site of GluR6(Q) to a leucineresidue and tested this mutant for outward current. As expected,GluR6(Q590L) had an inwardly rectifying I-V and indeed showedsmall but significant outward currents at positive holding potentials,just like the chimeras (Fig. 6C, trace 4). This outward currentdid not persist in calcium-free NFR (Fig. 6C, trace 3), however,indicating that the leucine residue at the Q/R-site by itselfcannot be the sole determinant of the outward current at positivemembrane potentials. To investigate this further we constructeda mutant chimera, GluR6-PKBP(Rp)L583Q, which carries the KBP poreregion transplanted into GluR6 but has a glutamine instead ofa leucine residue at the Q/R site. This clone is functional, hasa rectifying I-V curve, and shows distinct outward currents atpositive membrane potentials (Fig. 6C, trace 5). Thus, determinantsof the pore domain of KBPs other than the leucine at the Q/R siteare responsible for the slight outward rectification observedon top of a basically inwardly rectifying I-V relation.
Fig. 6. Comparison of I-V curves of GluR6(Q)-PCS and chimeric GluR6 receptors. Note that transplantation mutants harboring the ionpore domains of KBP(Ca) $alpha$ (A), KBP(Ca) $beta$ (A), KBP(Rp) (B), KBP(Gd)(B), or KBP(Xl) (B) are all inwardly rectifying and not significantlydifferent from GluR6(Q)-PCS. C, Comparison of I-V curves of GluR6-PKBP(Ca) $alpha$ and GluR6(Q590L) in NFR and calcium-free, magnesium-substitutedNFR (MgR), and I-V of the mutant chimera GluR6-PKBP(Rp)L583Q.Note that lack of outward rectification is observed only in GluR6(Q590L)in MgR. At least three oocytes were measured for each chimeraand gave identical curves.
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The Q/R-site not only determines the rectification properties of GluRs but also has a major impact on calcium permeability.AMPA receptors carrying an edited arginine residue at this position(such as GluR2) are virtually impermeable to calcium, whereasunedited subunits carrying a glutamine residue are calcium permeable(Hume et al., 1991). Similarly, for KA receptors, "Q" editingvariants have a higher calcium permeability than "R" variants,although the latter are not entirely calcium impermeable (Egebjergand Heinemann, 1993). Despite the large number of Q/R site mutantsreported in the literature, no data are available on a GluR subunitcarrying a leucine residue at this position. Consequently, itis difficult to predict whether the presence of a leucine residueat the Q/R site might allow calcium permeability of the ion channel.We therefore tested GluR6(Q)-PCS and GluR6-PKBP(Ca) $alpha$ for calciumpermeability using a sodium- and potassium-free modified NFR thatcontains Ca²⁺ as the sole cation capable of permeating the ion channel on agonist-mediatedchannel opening (Hollmann et al., 1991). For GluR6(Q)-PCS we foundabout the same permeability for Ca²⁺ as is seen in wild-type GluR6(Q). KA (300 µM) in 10 mM Ca-Ringerevoked ~60% of the control current seen in NFR, and in 80 mM Ca-Ringeralmost as much current can be recorded as in NFR (data not shown).GluR6-PKBP(Ca) $alpha$ was selected for analysis of calcium permeabilityof KBP pores because this chimera yields the largest currentsof the five chimeras. In 10 mM Ca-Ringer, GluR6-PKBP(Ca) $alpha$ gave5% of the current evoked by 300 µM KA in NFR, and in 80 mM Ca-Ringerit yielded 75% of the control current (Fig. 7). Thus, the KBP(Ca) $alpha$ ion channel domain is capable of fluxing Ca²⁺ ions to a considerable degree, although not quite to the extentof wild-type GluR6(Q) and GluR6(Q)-PCS. We also tested the poreof KBP(Xl) and found it to flux calcium to a similar degree (datanot shown). Thus, the leucine residue at the Q/R site of the poreevidently is compatible with calcium permeating the ion channel.In keeping with these results, we determined that the mutant GluR6(Q590L),which contains a leucine residue at the Q/R site, is also permeablefor calcium (data not shown).
Fig. 7. The ion pore of KBP(Ca) $alpha$ is permeable to calcium. KA-evoked currents were compared in normal frog Ringer's solution (NFR,A) and Ca-Ringer containing either 80 mM (B) or 10 mM (C) calciumbut no other cations. Note distinct currents in the absence ofsodium and potassium (B, C). At least three oocytes were measuredunder each condition and gave identical results.
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The KBP pore domains, just like the pores of GluR6, are not blocked by NMDA receptor channel blockers such as magnesium (Fig.6C, trace 2) or MK-801. We tested this for GluR6-PKBP(Rp), GluR6-PKBP(Ca) $alpha$ ,and GluR6-PKBP(Gd) (Fig. 8A). The KBP pore domains, however, areblocked by zinc, which is a channel blocker at both NMDA and non-NMDAreceptors (Westbrook and Mayer, 1987; Rassendren et al., 1990).We found that 100 µM zinc blocked 30% of KA-evoked (100 µM) currentsat GluR6(Q) as well as GluR6-PKBP(Rp), GluR6-PKBP(Ca) $alpha$ , and GluR6-PKBP(Ca) $beta$ .No block was seen with 1 µM zinc (data not shown). Interestingly,the KBP pore domains are not affected by philanthotoxin (PhTx),a wasp toxin (Fig. 8B), or by N-(4-hydroxyphenylpropanoyl)-spermine,a synthetic analog of wasp and spider toxins (data not shown).PhTx and spider toxins are known to efficiently block all NMDAreceptors and all non-NMDA receptors with rectifying I-V relations(Blaschke et al., 1993; Herlitze et al., 1993; Washburn and Dingledine,1996). We tested GluR6-PKBP(Rp), GluR6-PKBP(Ca) $alpha$ , GluR6-PKBP(Ca) $beta$ ,and GluR6-PKBP(Gd) and found no effect of the toxin or its syntheticanalog. The toxin block had previously been shown to be determinedby the amino acid located at the Q/R/N site, with "Q" and "N"versions being blocked and "R" versions not being blocked. Ourdata suggested that a leucine residue might also unexpectedlyprevent channel block, althoug it does not carry the positivecharge of an arginine residue. To verify this we tested the mutantGluR6(Q590L) for PhTx block and indeed found that the channel,which now has a leucine residue at the Q/R site, is no longersignificantly affected by the toxin (Fig. 8B). To obtain furtherevidence we used our mutant GluR6-PKBP(Rp)L583Q, which tests the"reverse" situation in which the leucine has been converted intoa glutamine. As expected, this mutant could now be blocked byPhTx (data not shown).
Fig. 8. Effects of MK-801 and PhTx on KBP ion channel domains transplanted into GluR6. A, Absence of block by MK-801. MK-801 (1 µM)was coapplied with 100 µM KA for 20-30 sec. After a washout period,100 µM KA was applied alone. Note lack of block of GluR6(Q) andthree ion pore transplantation chimeras during coapplication ofagonist and MK-801, and unaltered size of agonist-evoked responseafter washout. MK-801 (1 µM) did block NMDA receptors in controloocytes (data not shown). B, Absence of block by PhTx. KA (100µM) was applied for 50-60 sec, followed by a brief wash and anotherapplication of 100 µM KA followed within 2 sec by additional applicationof the open channel blocker PhTx (0.5 µM). Note lack of blockof two ion pore transplantation chimeras and mutant GluR6(Q590L),whereas GluR6(Q) is rapidly and efficiently blocked. Three tofour oocytes were measured in each case and gave identical results.
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Transplantation of functional ion pores into KBPs
We have demonstrated that the ion channel domains of KBPs are functional in the sequence background of both the KA receptorGluR6 and the AMPA receptor GluR1 but not in their own (KBP) sequencebackground. This suggested that most likely communication betweenthe ligand binding site and the ion channel domain is disruptedin homomeric KBPs. If this is indeed the case, a functional channeldomain such as that of GluR1 or GluR6 when inserted into a KBPshould not be able to rescue function but rather should producenonfunctional chimeric receptors. To test this we engineered theappropriate "reverse" chimeras, transplanting the ion channeldomains of GluR6 and GluR1 into KBP(Rp). These chimeras when expressedin Xenopus oocytes did not produce any measurable currents onactivation with the glutamatergic agonists Glu, KA, or Dom, althoughthe chimeric proteins were clearly synthesized and inserted intothe plasma membrane (Fig. 4B). We also attempted to rescue functionof the N-terminally elongated KBP construct GluR6N-KBP(Rp)C bytransplanting the pore domain of GluR6 into this clone, creatingthe chimera GluR6-Rp-R6-Rp (Fig. 1, bottom bar graph). This constructwas also nonfunctional, although it was expressed and transportedto the plasma membrane (Fig. 4C).

Thus, even with a highly functional ion channel domain such as that of GluR6(Q), these receptor subunits failed to translateligand binding into channel opening, supporting our conclusionthat the gating mechanism rather than the ion pore is dysfunctionalin homomeric KBPs.

DISCUSSION

N-terminal elongation does not rescue KBP function
N-terminal domains have been swapped between GluR6 and NMDAR1 GluR subunits without loss of function (Stern-Bach et al., 1994).Because even a remotely related subunit such as NMDAR1 (only 34.1%sequence identity with GluR6) evidently can serve as the donorof an N-terminal domain, it was not unreasonable to expect thatthe much more closely related KBP(Rp) (40.0% sequence identity)might be functionally rescued by a grafted N-terminal domain fromGluR6; however, the N-terminal transplant did not render KBP(Rp)functional. The failure to produce a functional chimera indicatesthat the short N-terminal domain in KBPs is not likely the reasonfor lack of channel function.

Transplanted KBP ion pores are functional
The overall distribution of hydrophobic domains in KBPs is similar to that of functional GluRs (Fig. 1), and even the genestructure that has been elaborated for KBP(Gd) (Eshhar et al.,1992; Gregor et al., 1992) is quite similar. Furthermore, thetopology that has been shown for KBP(Ca) $alpha$ and KBP(Ca) $beta$ based onN-glycosylation studies (Wo and Oswald, 1994) is identical tothat proposed for GluR1 (Hollmann et al., 1994), GluR3 (Bennettet al., 1995), and NMDAR1 (Wood et al., 1995). The obvious structuralresemblance between KBPs and other GluRs suggested that domainsfrom KBP subunits could potentially be exchanged for equivalentdomains of functional GluRs, and vice versa. Indeed, when we insertedthe hypothetical ion pore domains of KBPs in GluR1 or GluR6 weobtained functional chimeras, although maximal current amplitudesreached only 1-10% of the currents found in the parent clones.The domains transplanted consisted of the entire region betweenTMDs A and B (Fig. 2) rather than just the hydrophobic stretchthat is thought to loop into the membrane to form the ion pore(Hollmann et al., 1994). This design was chosen because recentcysteine scanning mutagenesis data (Kuner et al., 1996) suggestedthat the sequences flanking the pore loop participate to someextent in establishing the structure of the pore.

Chimeras containing pores from KBPs had pharmacological characteristics and agonist affinities virtually indistinguishablefrom those of the ligand binding site donor subunit, demonstratingthat the properties of the extracellular ligand binding site ofGluRs are not dependent on the pore structure to which that siteis connected. This conclusion is consistent with the work of Keinänenand colleagues, who reported construction of a functional solubleligand binding site solely derived from the two extracellularhalves of the ligand binding domain, without any pore structurein between (Kuusinen et al., 1995; Arvola and Keinänen, 1996).

KBP ion pores have distinct properties
The properties of the pore domains of the five known KBPs tested as domain transplants in GluR6 are very similar. This isnot unexpected given the high amino acid sequence homology ofthese regions (56-76% among the five KBPs), and in particularthe presence of a leucine residue in all five genes at a positionthat is homologous to the Q/R/N editing site in AMPA, KA, andNMDA receptors. All five pore domains have rectifying I-V valuesas might be predicted from the absence of an arginine residueat the Q/R/N editing site (Hume et al., 1991), and they all arepresumably permeable to calcium, although we verified this onlyfor GluR6-PKBP(Ca) $alpha$ and GluR6-PKBP(Xl). The KBP pore domains arenot blocked by NMDA receptor channel blockers, such as magnesiumor MK-801, but are inhibited by zinc, which at high concentrations(>100 µM) does not discriminate between NMDA and non-NMDA receptors(Westbrook and Mayer, 1987; Rassendren et al., 1990). Interestingly,the KBP pore domains are not affected by the wasp toxin PhTx,other spider toxins, or their synthetic analogs, and we showedthat this property is linked to the presence of a peculiar leucineresidue at the Q/R/N site that is unique to KBPs. Thus, the propertiesof the KBP ion pore as reflected in the channel properties ofthe GluR6-KBP chimeras are distinct from those of AMPA, KA, andNMDA receptors, although they somewhat resemble properties oftypical KA receptors.

KBPs are defective in gating
If all KBPs have functional agonist binding sites as has been shown previously (Henley, 1994), and if the pores of KBPs inprinciple are capable of conducting currents as our experimentsshowed, why then are these subunits nonfunctional as ligand-gatedion channels? Obviously, homomerically expressed KBP subunitsfail to translate ligand binding into channel opening. Becauseligand binding generally is assumed to cause a conformationalchange in the extracellular domain of the receptors (Mano et al.,1996; Laube et al., 1997), which presumably represents the gatingstep required to open the ion channel, it may be concluded thathomomerically expressed KBPs either fail to generate the appropriateconformational change or fail to communicate it to the pore. Thisconclusion is backed by our observation that the functional poredomains of GluR6 or GluR1, when inserted into KBP(Rp), failedto generate functional ion channels.

KBPs likely lack an essential subunit
It seems unlikely that some secondary modification of the receptor protein such as phosphorylation, which has been shown forKBP(Rp) (Ortega and Teichberg, 1990; Ibarra and Ortega, 1995),or glycosylation is required to "switch on" the interrupted bindingsite-to-ion pore communication in KBPs. Such a mechanism mostlikely would have been detected in one of the various expressionsystems tried for the KBP clones, such as Xenopus oocytes, chinesehamster ovary cells, and human embryonic kidney cells (for review,see Henley, 1994). Rather, it seems likely that an additionalsubunit may be required that interacts with the KBPs to reestablishthe connection between ligand binding site and ion channel. Thismodulatory subunit may be either an accessory protein or anothersubunit of the GluR family. Among GluRs, several cases of homomericallynonfunctional subunits have been observed that are rendered functionalonly on coassembly with another subunit. Examples are the NR2subunits of the NMDA receptor subfamily (Monyer et al., 1992)or the KA2 subunit of the KA receptor subfamily (Herb et al.,1992). Recently it was reported that KBP(Xl) formed functionalion channels of a peculiar, novel pharmacology on coexpressionwith the NMDAR1 subunit of Xenopus laevis. None of the two subunitswas functional by itself, but on coexpression formed channelsthat reportedly were activated by specific agonists for all pharmacologicalsubclasses of GluRs, AMPA, KA, and NMDA, and KBP(Xl) was thereforedubbed "unitary" receptor (Soloviev et al., 1996). This reportis in agreement with our finding that the pore of KBP(Xl) is functional.Other KBPs, however, have not been examined in coexpression experimentswith NMDAR1 subunits from the same species, and our own attemptsto coexpress KBPs with the rat NMDAR1 subunit in Xenopus oocytesdid not yield functional receptors other than typical homomericNMDA receptors (C. Villmann and M. Hollmann, unpublished data).Thus, although it is possible that KBPs from other species mightalso form functional receptors with NMDAR1 subunits, there iscurrently no evidence for this. KBP(Xl) differs from all otherKBPs in binding both KA and AMPA with high affinity (Ishimaruet al., 1996). Therefore, it is possible that this subunit playsa quite different role and indeed has unique properties not sharedby any of the other KBPs.

GluRs are modular proteins
Our data support the view that GluRs are modular proteins with structural features derived from a number of different precursorproteins (Seeburg, 1993; Wo and Oswald, 1995). In particular,the demonstration that pore regions can be transplanted betweendistantly related subunits without killing function strongly supportsthe hypothesis that GluRs indeed might have evolved from bacterialamino acid binding proteins by insertion of a pore domain in betweenthe two ligand binding subdomains (O'Hara et al., 1993; Kuryatovet al., 1994; Stern-Bach et al., 1994).

In summary, we conclude that KBPs in addition to harboring perfectly functional ligand binding sites also have intrinsicallyfunctional ion channel domains that display inward rectification,allow significant calcium permeability, and have distinct pharmacologicalproperties. Our findings suggest that the elusive physiologicalrole of KBPs may indeed be that of Glu-activated ion channels.We speculate that one or more additional subunits or an accessoryprotein may be required to twist the subunits in a heteromericreceptor complex just enough to enable the occupied ligand bindingsite to successfully gate the ion channel. Furthermore, the chimeraconstruction approach presented in this study should prove usefulin analyzing the mechanism of channel gating in GluRs and definingthe molecular pathway involved in signal transduction from theagonist binding site to the ion pore.

FOOTNOTES

Received June 16, 1997; revised July 28, 1997; accepted July 29, 1997.

This work was supported by a Deutsche Forschungsgemeinschaft Heisenberg fellowship to M.H., the Starke-Werner Foundation (L.B.),and a PhD fellowship of the Max-Planck-Society to C.V. We thankDrs. Keiji Wada and Robert Wenthold (National Institute on Deafnessand Other Communication Disorders-National Institutes of Health,Bethesda, MD) for the Rana pipiens KBP cDNA clone [KBP(Rp)], Dr.Robert Oswald (Cornell University, Ithaca, NY) for the GFKAR $alpha$ and GFKAR $beta$ clones [KBP(Ca) $alpha$ and KBP(Ca) $beta$ ], and Dr. Vivian Teichberg(Weizmann Institute, Rehovot, Israel) for the chicken KBP cDNA[KBP(Gd)]. Dr. Robert Wenthold generously donated the affinity-purifiedanti-GluR6 and anti-KBP(Rp) antisera used in this study, and EmilyLiman and the late Peter Hess (Harvard Medical School, Boston,MA) provided the pGEMHE vector.

Correspondence should be addressed to Dr. Michael Hollmann, Glutamate Receptor Laboratory, Max-Planck-Institute for ExperimentalMedicine, Hermann-Rein-Strasse 3, D-37075 Göttingen, Germany.

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Electrophysiological Properties of AMPA Receptors Are Differentially Modulated Depending on the Associated Member of the TARP Family
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C. Schmidt, M. Werner, and M. Hollmann
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N. Decher, A. S. Barth, T. Gonzalez, K. Steinmeyer, and M. C. Sanguinetti
Novel KChIP2 isoforms increase functional diversity of t

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Kainate Binding Proteins Possess Functional Ion Channel Domains

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Volume 17, Number 20, Issue of October 15, 1997 pp. 7634-7643
Copyright ©1997 Society for Neuroscience