Neuronal Inwardly Rectifying K+ Channels Differentially Couple to PDZ Proteins of the PSD-95/SAP90 Family

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The Journal of Neuroscience, January 1, 2000, 20(1):156-162

Neuronal Inwardly Rectifying K⁺ Channels Differentially Couple to PDZ Proteins of the PSD-95/SAP90 Family
Ralf B. Nehring¹, Erhard Wischmeyer¹, Frank Döring¹, Rüdiger W. Veh², Morgan Sheng³, and Andreas Karschin¹
¹ Molecular Neurobiology of Signal Transduction, Max-Planck-Institut for Biophysical Chemistry, 37070 Göttingen, Germany, ² Department of Anatomy, Charité, 10098 Berlin, Germany, and ³ Howard Hughes Medical Institute, Massachusetts General Hospital, Boston, Massachusetts 02114

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Several signaling proteins clustered at the postsynaptic density specialization in neurons harbor a conserved C-terminal PDZdomain recognition sequence (X-S/T-X-V/I) that mediates bindingto members of the PSD-95/SAP90 protein family. This motif is alsopresent in the C termini of some inwardly rectifying K⁺ (Kir) channels. Constitutively active Kir2 channels as well asG protein-gated Kir3 channels, which are fundamental for neuronalexcitability, were analyzed as candidates for binding to PSD-95/SAP90family members. Therefore C termini of Kir2.1(+), Kir2.3(+), Kir2.4( $-$ ),Kir3.1( $-$ ), Kir3.2(+), Kir3.3(+) and Kir3.4( $-$ ) subunits (+, motifpresent; $-$ , motif absent) were used as baits in the yeast two-hybridassay to screen for in vivo interaction with PDZ domains 1-3 ofPSD-95/SAP90. In contrast to Kir2.1 and Kir2.3, all Kir3 fragmentsfailed to bind PSD-95 in this assay, which was supported by thelack of coimmunoprecipitation and colocalization of the entireproteins in mammalian cells. A detailed analysis of interactiondomains demonstrated that the C-terminal motif in Kir3 channelsis insufficient for binding PDZ domains. Kir2.1 and Kir2.3 subunitson the other hand coprecipitate with PSD-95. When coexpressedin a bicistronic internal ribosome entry site expression vectorin HEK-293 cells macroscopic and elementary current analysis revealedthat PSD-95 suppressed the activity of Kir2.3 channels by >50%.This inhibitory action of PSD-95, which predominantly affectsthe single-channel conductance, is likely attributable to a molecularassociation with additional internal interaction sites in theKir2.3protein.

Key words: inwardly rectifying; Kir channel; GIRK; postsynaptic density; chapsyns; MAGUK; yeast two-hybrid

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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Ion channels, receptors, signaling enzymes, and adhesion molecules in neurons are typically localized at specific subcellularspecializations such as axon terminals, presynaptic and postsynapticsites, or nodes of Ranvier. A series of anchor and adapter elementshave now been identified to coordinate the targeted distributionof these proteins on the cell surface for proper signaling withinand between neurons (Sheng, 1996; Sheng and Kim, 1996; Kornauet al., 1997; Craven and Bredt, 1998). Well known examples constituterapsyn, which clusters nicotinic acetylcholine receptors at theneuromuscular junction (Colledge and Froehner, 1998), the 93 kDaprotein gephyrin, which aggregates glycine and GABA_A receptorsin the postsynaptic membrane of spinal cord neurons (Kirsch etal., 1993), and syntaxin/soluble N-ethylmaleimide-sensitive factorattachment protein 25, which complexes presynaptic N-type Ca²⁺ channels and possibly other components of the exocytotic machinery(Sheng et al., 1994). Protein targeting to the postsynaptic density(PSD; Kennedy, 1993), the electron-dense cytoskeletal specializationof excitatory synapses in CNS neurons, is typically associatedwith members of the PSD-95/SAP90 (synapse-associated proteins)protein family. They are alternatively referred to as chapsyns(channel-associated proteins of the synapse) or MAGUK proteins(membrane-associated guanylate kinases; Ehlers et al., 1996; Shengand Kim, 1996). In mammals this family includes four members,PSD-95/SAP-90, PSD-93/chapsyn110, SAP102, and SAP97/hdlg. In theirN termini these proteins are characterized by the presence ofthree, 90 amino acid long PDZ domains, initially recognized asrepeats in PSD-95, discs large protein and the tight junctionprotein ZO-1. In the C terminus they contain additional modulesfor interaction with cellular proteins, such as the src homology3 domain and an enzymatically inactive guanylate kinase-like domain.Together with other proteins PSD-95/SAP90 proteins have now beenshown to organize a complex PSD signaling matrix that may containkainate and NMDA receptors (Kornau et al., 1995; Niethammer etal., 1996; Garcia et al., 1998), neuronal nitric oxide synthase(nNOS; Brenman et al., 1996), voltage-gated K⁺ (Kv; Kim et al., 1995), and inwardly rectifying K⁺ (Kir) channels (Cohen et al., 1996; Horio et al., 1997), fasciclinII (Tejedor et al., 1997; Thomas et al., 1997; Zito et al., 1997),calmodulin (Masuko et al., 1999), Ca²⁺ ATPase 4 $beta$ (Kim et al., 1998a); regulator of G protein signaling12 (Snow et al., 1998), synaptic rasGAP (Kim et al., 1998b), guanylate-kinase-associatedprotein (Kim et al., 1997; Takeuchi et al., 1997), the putativecell adhesion molecule neuroligin (Irie et al., 1997), and cysteine-richinteractor of PDZ three (CRIPT; Niethammer et al., 1998).

It was originally demonstrated that the C-terminal tetrapeptide of both Kv1.4 channels and NMDA 2B subunits (NR2B) interactwith PDZ domains I and II of PSD-95. Sequence comparison of theproteins listed above and supported by random peptide libraryscreening (Songyang et al., 1997), as well as x-ray crystallography(Doyle et al., 1996) suggested the sequence X-S/T-X-I/V as theconserved recognition motif for PDZ domains in PSD-95/SAP90 proteins.In the mammalian CNS, the abundantly expressed Kir2 and Kir3 channelsare synaptically regulated by protein phosphorylation and directG protein activation, respectively, and thus play a role in thefine tuning of neuronal excitability after synaptic input (Doupniket al., 1995; Isomoto et al., 1997). Because Kir2.1, Kir2.2, Kir2.3,Kir3.2, and Kir3.3 subunits harbor the PDZ binding consensus intheir C termini, whereas others (Kir2.4, Kir3.1, and Kir3.4) donot, we investigated their possible differential association withPSD-95.

  MATERIALS AND METHODS

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Plasmids and clones. cDNAs encoding the rat Kv1.4 (Stühmer et al., 1989), rat Kir2.1 (Wischmeyer et al., 1995), rat Kir2.3(Falk et al., 1995), rat Kir3.1 (Wischmeyer et al., 1997), humanKir3.2 (Wischmeyer et al., 1997), rat Kir3.3 (Dissmann et al.,1996), human Kir3.4 (Spauschus et al., 1996), and rat PSD-95 (Choet al., 1992) were subcloned into the mammalian expression vectorpcDNA3 (Invitrogen, Leek, The Netherlands). For biochemical andfunctional analysis cDNAs of Kir subunits were alternatively clonedtogether with PSD-95 into a modified pcDNA3-internal ribosomeentry site (IRES) vector, which contained a single promoter andan additional IRES of the poliovirus to allow translation of twoopen reading frames from one mRNA (LaMonica et al., 1986). Forimmunodetection PSD-95, Kir2.3, Kv1.4, and Kir2.1 were epitope-taggedat the N terminus with the c-myc sequence MEQKLISEEDLN. The assemblyof concatemeric Kir3.1/3.2 constructs has been described elsewhere(Wischmeyer et al., 1997).

Yeast two-hybrid assay. The entire C-terminal domains of Kir2.1 [amino acids (aa) 179-427], Kir2.3 (aa 171-446), Kir2.4 (aa195-435; Töpert et al., 1998), Kir3.1 (aa 180-501), Kir3.2 (aa191-425), Kir3.3 (aa 157-393), and Kir3.4 (aa 186-419) were amplifiedby PCR and subcloned into the yeast DNA-binding domain vectorpGBT9 (Clontech, Palo Alto, CA). As positive controls the C-terminaldomains of the voltage-gated rat Kv1.4 channel (aa 568-655; Stühmeret al., 1989) and the rat NR2B (aa 1371-1482; Monyer et al., 1992)were also cloned into pGBT9. PDZ domains 1-3 of PSD-95/SAP90 (aa1-401) were inserted into the activation domain vector pGAD-GH(Clontech). Deletion constructs of Kir2.1, Kir2.3, and Kir3.2were generated by PCR with appropriate oligonucleotides, and aKir2.1/Kir3.2 chimera was constructed as described (Higuchi etal., 1988). Yeast strain HF7c was cotransformed with 100 ng eachof bait and prey vector and was streaked out on agar plates lackingtryptophan, leucine, and histidine. Colony growth showing activationof the nutritional reporter gene HIS3 was controlled for the individualconstructs after 4d.

Coimmunoprecipitation. COS-7 cells were transiently transfected with Kir channel subunits and PSD-95 individually in pcDNA3and together in pcDNA3-IRES, respectively, by calcium phosphateprecipitation. In brief, transfected cells were washed with PBS60 hr after transfection, harvested, and homogenized in ice-coldlysis buffer [50 mM Tris, pH 7.4, 150 mM NaCl, 5 mM EGTA, proteaseinhibitors (1 µg/ml leupeptin and pepstatin A, 2 µg/ml aprotenin,and 1 mM PMSF), and 1% Triton X-100]. Nonsoluble components wereremoved by centrifugation at 4°C, and extracts were preincubatedwith 50 µl of protein A- or protein G-agarose beads (Roche Diagnostics,Mannheim, Germany) to avoid unspecific binding. For immunoprecipitationpreadsorbed extracts were incubated for 1 hr with mouse anti-myc(Santa Cruz Biotechnology, Santa Cruz, CA) or rabbit anti-myc(Upstate Biotechnologies, Lake Placid, NY) to precipitate taggedproteins. After overnight incubation on a rotating disk, boundproteins were pulled down with either protein A- or protein G-agarosebeads and washed four times for 20 min each with lysis buffer.Pull-down experiments in the absence of specific antibodies wereperformed to verify the specificity of the immunoprecipitations(data not shown). Cell extracts and precipitated proteins wereanalyzed by Western immunoblots probed with monoclonal mouse $alpha$ -PSD-95antibodies (1:1000, clone K28/43; Upstate Biotechnology), polyclonalrabbit $alpha$ Kir3.2 and $alpha$ Kir2.1 antibodies (1:100 and 1:1000, respectively),and $alpha$ -myc antibody (mouse, 1:100; rabbit, 1:1000). Blots weredeveloped using horseradish peroxidase-conjugated goat $alpha$ -rabbitand goat $alpha$ -mouse Igs (Jackson ImmunoResearch Laboratories, WestGrove, PA), respectively, and an enhanced chemoluminescence detectionsystem (ECL; Amersham, Buckinghamshire,UK).

Immunocytochemistry. COS-7 cells were plated on poly-L-lysine-coated coverslips 1 d before transfection. Plasmids were transfectedusing LipofectAMINE (Life Technologies, Gaithersburg, MD). After2 d cells were fixed with 2% paraformaldehyde and 0.1% TritonX-100 and blocked with 2% normal goat serum. For double stainingcells were incubated overnight with the primary rabbit $alpha$ -myc (1:1000)or $alpha$ -Kir3.2 antisera (1:100), together with the monoclonal mouse $alpha$ -PSD-95 antibody (1:1000). After washing with PBS cells wereincubated 1 hr with Cy3-conjugated goat secondary IgG (1:1000;Jackson ImmunoResearch) and FITC-conjugated goat secondary IgG(1:200, Jackson ImmunoResearch). Coverslips were washed againwith PBS, mounted on slides, and analyzed on an LSM410 laser scanningmicroscope equipped with an argon-crypton laser (Zeiss, Oberkochen,Germany).

Electrophysiology. Semiconfluent HEK-293 cells, grown on glass coverslips, were transfected with 0.8 µg/ml cDNAs using LipofectAMINEand Opti-MEM I (Life Technologies) following the manufacturer'sprotocol. Whole-cell recordings were performed at room temperature48-72 hr after transfection in a bath solution consisting of 135mM NaCl, 5.4 mM KCl, 1.8 mM CaCl₂, 1 mM MgCl₂, 10 mM glucose,and 5 mM HEPES, pH 7.4. Patch pipettes were pulled from borosilicateglass capillaries (Kimble Products, Sussex, UK), and heat-polishedto give input resistances of 4-6 M $Omega$ . The pipette recording solutioncontained 140 mM KCl, 2 mM MgCl₂, 1 mM EGTA, 1 mM Na₂ATP, 100µM cAMP, 100 µM GTP, and 5 mM HEPES, pH 7.3. Currents were recordedwith an EPC9 (Heka Electronics, Lamprecht, Germany) patch-clampamplifier and low-pass-filtered at 1-2 kHz. Stimulation and dataacquisition were controlled by the Pulse/Pulsefit software package(Heka) on a Macintosh computer (Apple, Cupertino, CA), and dataanalysis was performed with Igor software (WaveMetrics, Lake Oswego,OR). Data are presented as mean ± SD (number ofcells).

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Yeast two-hybrid assay

The presence of the C-terminal PDZ domain recognition motif X-S/T-X-V/I prompted us to investigate on the association of neuronalKir2 and Kir3 channel members with proteins of the PSD-95/SAP90family. In a first assay the complete C termini of Kir2.1, Kir2.3,Kir3.2, Kir3.3 (harboring the motif), as well as Kir2.4, Kir3.1,and Kir3.4 (in which the motif is absent) were used as bait inthe yeast two-hybrid (Y2H) system (Fields and Song, 1989) forinteraction with PDZ domains 1-3 (aa 1-401) of PSD-95/SAP90 (Fig.1A). The C termini of voltage-dependent Kv1.4 channels (Kim etal., 1995) as well as NR2B subunits (Kornau et al., 1995), forwhich PSD-95 interaction had been originally demonstrated, wereused as positive control baits for strong interaction. As reportedby the yeast HIS3 selection marker, we found that only Kir2.1,Kir2.3, Kv1.4, and NR2B but not Kir2.4 and none of the Kir3 channelsubunits associated with PDZ domains 1-3 in the Y2H assay (Fig.1A). Whereas lack of interaction was expected for Kir2.4, Kir3.1,and Kir3.4 in which the PDZ recognition motif is not conserved,we sought to analyze in more detail why the presence of the X-S/T-X-V/Isequence in Kir3.2 and Kir3.3 subunits did not confer the capabilityto bind to PDZ domains 1-3. A series of C-terminal deletion constructsand chimera between Kir2.1 and Kir3.2 were generated and usedas bait in a more precise interaction domain analysis (Fig. 1B).We first demonstrated that in Kir2.1 subunits indeed removal ofthe last three residues (Kir2.1 $Delta$ SEI) completely disrupted PDZbinding. Exchange of these residues by the terminal triplet presentin Kir3.2 subunits, however, restored its proper binding functionKir2.1(SKV). Moreover, yeast transformed with the Kir2.1 constructin which the triplet SEI was maintained but 13 amino acids weredeleted further upstream of the C terminus was HIS3-negative,indicative of a contribution of this region in binding PDZ1-3.An interesting phenomenon was observed in equivalent experimentsusing Kir2.3 subunits. When the isoleucine at position 0, theserine at position $-$ 2, or the complete C-terminal triplet SAIwas removed, a few transformants still contained the prey, suggestingan additional interaction site in Kir2.3 for PSD-95 (see below).

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Figure 1. Kir2 channels but not Kir3 channels interact with PDZ domains 1-3 in the Y2H system. A, C termini of the Kir channels listed were used as bait in pGBT9 to test the interaction with PDZ1-3 of PSD-95 in pGAD-GH. The NR2B subunit and the Kv1.4 C termini were used as positive controls. The consensus sequence X-S/T-X-I/V is shown in bold letters. Numbers on the left denote amino acid positions of C-terminal fragments. B, Cross-mutational analysis of Kir2.1 and Kir3.2 mutants. See Results for details. Colony growth was controlled after 4 d.

Conversely, all manipulations performed on Kir3.2 subunits in which (1) the functional SEI motif of Kir2.1 was introducedand (2) 13 amino acids upstream of this motif in Kir2.1 were insertedor (3) the first half of the C terminus of Kir3.2 was replacedby the equivalent region in Kir2.1 (aa 179-305; aa 318-425 derivefrom Kir3.2), failed to transfer PDZ binding affinity to Kir3.2channels. For demonstrating a putative interaction with otherPSD-95/SAP90 family members, various fragments including the completeC termini of all Kir3 subunits were used as bait in a Y2H screenof two (E16 and P5) rat brain cDNA libraries constructed in theactivation domain vector pAD-GAL4. In these experiments no interactionpartner was identified for Kir3.1 (amino acids 1-85, 180-363,321-501, and 180-501) or any other Kir3 subunit. As test for thequality of our assay, the full-length cDNA of PSD-95/SAP90 wasisolated when the NR2B C terminus was used as bait (data not shown).From these results it is concluded that at least in the Y2H systemthe PDZ-binding motif X-S/T-X-I/V in Kir3.2 or Kir3.3 subunitsis insufficient for binding PDZ domains 1-3 of PSD-95/SAP90.

Coimmunoprecipitations

The apparent differential association of PSD-95/SAP90 with Kir subunits in the yeast assay was also analyzed for the full-lengthKir proteins biochemically by immunoprecipitation and Westernimmunoblotting in membranes of transfected COS-7 cells. Whole-cellextracts were prepared from COS-7 cells that had been cotransfectedwith myc-tagged Kir2.1 and PSD-95 (Fig. 2A, left panel) or alternativelya pcDNA3IRES vector that contained both Kir2.1 and myc-taggedPSD-95 (Fig. 2A, right panel). In both experiments $alpha$ -myc antibodieswere used to precipitate tagged Kir2.1 and PSD-95, respectively.Western blot analysis of immunoprecipitates demonstrated thateach protein could be coprecipitated with the tagged interactionpartner, showing that the association is revealed independentof which protein is initially pulled down. A corresponding analysisfor Kir2.3 subunits showed a similarly strong bonding to PSD-95(Fig. 2B). The construct mycKir2.3( $Delta$ SAI) in which the terminalamino acid triplet was removed did not precipitate significantlywith PSD-95 in this assay (Fig. 2B, right panel).

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Figure 2. PSD-95 coprecipitates with Kir2.3 but not with Kir3.2 channels. Proteins from whole-cell extracts of COS-7 cells, cotransfected with mycKir2.1 and PSD-95 (or Kir2.1IRESmycPSD-95) (A), mycKir2.3IRESPSD-95 and mycKir2.3( $Delta$ SAI)IRESPSD-95 (B), as well as Kir3.2 (Kir3.2K422A) and mycPSD-95 (C), were immunoprecipitated with $alpha$ -myc antibodies. Immunoprecipitates were separated on 10% SDS gels, blotted onto polyvinylidene difluoride membranes, and probed with specific antibodies as indicated. Note that in A when either interaction partner is myc-tagged, the corresponding protein can be detected in the $alpha$ -myc precipitates. Bottom panels in C show the presence of Kir3.2 and mycPSD-95 in whole-cell extracts of cotransfected COS-7 cells. In all other blots marker bands are shown on the left.

Under the same conditions we precipitated mycPSD from extracts of COS-7 cells cotransfected with mycPSD-95/Kir3.2. However,no signal was detected with $alpha$ Kir3.2 antibodies in the precipitates(Fig. 2C). This experiment was also performed with mutant Kir3.2K422Asubunits in which the lysine at position $-$ 1 had been changed toan alanine residue (SAV), which approximates the C terminus tothat of Kir2.3 (SAI) and optimizes the motif for recognizing PDZdomains. Yet, using $alpha$ -Kir3.2 antibodies we were again unable todetect the appropriate band in the precipitates of PSD-95. Thusour data verify in mammalian cells that entire Kir2 subunits interactwith PSD-95/SAP90 proteins and support the failure of strong complexingbetween Kir3.2 and PSD-95, as suggested by the yeastassay.

Coclustering

Myc-tagged Kir2.3 and Kir3.2 channels were also probed for colocalization with PSD-95 when cotransfected in COS-7 cells. Usingconfocal microscopy we confirmed earlier results (Kim et al.,1995) that voltage-gated Kv1.4 channels and PSD-95 are distributedhomogeneously when transfected individually (data not shown) butcolocalize and cluster with a typical punctuate staining aftercoexpression (Fig. 3A,B). A less homogenous distribution and moderateclustering were observed for transfected Kir2.3 channels. In thepresence of PSD-95 both proteins were found to overlap completely(Fig. 3C,D). Contrasting these results, PSD-95 remains homogeneouslydistributed in COS-7 cells in the presence of Kir3.2 subunits,which demonstrate punctate distribution and profound perinuclearlocalization (Fig. 3E,F).

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Figure 3. Kir2.3 channels are coclustered with PSD-95 after transfection in COS-7 cells. Confocal images are shown of COS-7 cells cotransfected with PSD-95 and mycKv1.4 (A, B), PSD-95 and myc Kir2.3 (C, D), and PSD-95 and Kir3.2 (E, F), respectively. The distribution of FITC-labeled PSD-95 is shown in A, C, and E; distribution of Cy3-labeled channel subunits is shown in B, D, and F using two different sets of filters. Sites of PSD-95/channel clustering are marked with arrowheads. Scale bar, 20 µm.

Functional consequences

The question was addressed of whether the association of Kir2 channels with PSD-95/SAP90 affects (1) the expression and (2)acute or long-term functional channel properties. For a quantitativeanalysis of Kir channel activity in the presence and absence ofPSD-95, we compared Kir channel expression in mammalian cellsfrom pcDNA3 containing just the cDNA of Kir2.3 and the bicistronicpcDNA3IRES vector that permits translation of both Kir and PSD-95from one mRNA. In these experiments Kir2 subunits were expressedindividually, and Kir3 subunits were expressed as concatemersfrom Kir3.1 and Kir3.2 subunits. The latter were found to generatecurrents indistinguishable from those that originated from a mixtureof individual Kir3.1 and Kir3.2 subunits with respect to single-channelcharacteristics, activation potential and kinetics, dependenceon extracellular [K⁺], as well as block by extracellular Ba²⁺ and Cs⁺ (Wischmeyer et al., 1997; data not shown). For both Kir2.3 andKir3.1/3.2, macroscopic basal (in 25 mM external K⁺) currents were measured in transfected HEK-293 cells using stepand ramp voltage-clamp whole-cell recordings. Kir2.3 current density(49 ± 24 pA/pF; n = 32; amplitude range, 0.33-7.18 nA) was reducedby 61% in the presence of PSD-95 (20 ± 15 pA/pF; n = 34; amplituderange, 0.17-2.61 nA; p < 0.01, Student's t test). Swapping theinsertion site for Kir2.3 and PSD-95 in the pcDNA3IRES vectordid not affect current suppression by PSD-95. In contrast, agonist(5-HT)-induced Kir3.1/3.2 inward current density at $-$ 100 mV averagedto 39 ± 19 pA/pF (n = 10) and was not significantly altered aftercoexpression of PSD-95 (37 ± 16 pA; n = 10; Fig. 4A).

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Figure 4. Coexpression of Kir2.3 channels with PSD-95 causes reduction of macroscopic current amplitude and unitary channel conductance. A, Whole-cell current responses to voltage pulses from +20 to $-$ 140 mV from a holding potential of $-$ 60 mV of HEK-293 cells transfected with Kir2.3 and Kir2.3 plus PSD-95 in the expression vector pcDNA3IRES, respectively. Currents are digitized at 5 kHz and filtered at 2.9 kHz. The bar graph shows current densities of Kir2.3 and Kir3.2 channels measured at $-$ 100 mV in elevated 25 mM extracellular K⁺ in the absence and presence of PSD-95. B, Amplitude histogram of cell-attached single-channel recordings from Kir2.3 channels (see inset) with the number of data points plotted against mean current flow per 0.75 msec bin for single-channel events recorded at $-$ 100 mV. Kir2.3 channels are shown in black, and Kir2.3 channels plus PSD-95 are overlayed in gray. Currents were digitized and filtered at 1 kHz. C, I-V plot (pipette potential on the abscissa) of the single-channel currents in B reveals strong inward rectification and a slope conductance of 14 pS for Kir2.3 and 8 pS for Kir2.3 plus PSD-95, respectively.

To clarify whether the PSD-95 interaction in HEK-293 cells affected the efficiency of channel expression or altered single-channelproperties, elementary currents were analyzed in the cell-attachedconfiguration with 140 K⁺ in the pipette (Fig. 4B). Kir2.3 currents were measured witha typically small unitary conductances of 14 pS (n = 2) that occurredat a frequency of p_o = 0.72 and is in accordance with previouslypublished values (Morishige et al., 1993; Makhina et al., 1994;Périer et al., 1994). The frequency of Kir2.3 channel eventswas unaltered in the presence of PSD-95 (p_o = 0.73), but the elementaryconductance was decreased to 8 ± 1.2 pS (n = 13; 10 differentexperiments; Fig. 4B,C). The product $gamma$ · p_o (as a measure of theaverage current flux through a single channel) for Kir2.3 andKir2.3/PSD-95 was calculated to differ by a factor of 1.85, indicatingthat the approximately twofold reduction by PSD-95 in macroscopiccurrents is primarily caused by a change in single-channelproperties.

Using this assay we finally investigated the observation that Kir2.3 mutants lacking the C-terminal PDZ domain recognitionmotif may still weakly interact with PSD-95. Two mutant channelswith the serine at position $-$ 2 exchanged to an alanine (AAI) andthe last triplet removed completely ( $Delta$ SAI) generated current densitiesthat were reduced in the presence of PSD-95 by 69, and 72%, respectively(Fig. 5). PDZ-mediated interactions have been recently found tooccur through modes other than by recognition of a C-terminalmotif (Hillier et al., 1999). Thus, in a mutant channel lackingthe C terminus, the sequence of a putative alternative interactionsite at aa position 409-412 (ETGI) was changed to EAGA. In thepresence of PSD-95 macroscopic currents generated by these mutantKir2.3 channels were reduced by only 23%, suggesting that interactionwith the C-terminal motif in Kir2.3 channels may not be the soledeterminant in the functional association with PSD-95.

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Figure 5. Analysis of C-terminal and internal PDZ domain recognition motifs in Kir2.3 subunits. The bar graph summarizes relative current amplitudes (measured at $-$ 100 mV) from HEK-293 cells cotransfected with PSD-95 and wild-type or mutated Kir2.3 subunits as depicted in the diagrams. In Kir2.3(444A) a serine residue has been replaced by an alanine at the $-$ 2 position; in Kir2.3( $Delta$ SAI) the terminal triplet has been removed; and in Kir2.3( $Delta$ SAI)EAGA a threonine (aa 420) and an isoleucine (aa 422) in putative internal PDZ domain recognition motif (E-T-G-I) have been replaced by alanine residues. Amplitudes in each bar have been normalized to currents revealed in the absence of PSD-95.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

As representative members of two different Kir subfamilies both Kir2.3 and Kir3.2 subtypes carry a conserved C-terminal recognitionmotif for PDZ domains of chapsyns. Yet in our hands the Y2H assayas well as biochemical and functional properties provide consistentevidence that Kir2.3 but not Kir3.2 subunits strongly interactwith these proteins (but see Inanobe et al., 1999). Consequently,it is concluded that the presence of the canonical C-terminalX-S/T-X-V/I sequence alone does not necessarily predict strongbonding of a candidate protein to PSD-95, even if closely relatedto another stable interaction partner. Instead, other structuraldeterminants of binding, e.g., in Kir channels the tertiary structureof the complete cytoplasmic tail, are likely to affect the specificityof coupling. Binding of G protein-gated Kir3.2 channels to PSD-95may be impaired because in the heterotetrameric channel proteinthe C termini are engaged in coupling to G $beta$ $gamma$ subunits, phosphatidylinositol-4,5phosphate Na⁺, and possibly other modulators of channel activity (Dascal, 1997).The crystal structure of PDZ domains complexed to their ligands(Doyle et al., 1996; Hillier et al., 1999) predicts that specificside chain interactions of residues upstream to the tetrapeptidealso affect the specificity of binding. As an example, these nearbyresidues in CRIPT determine the specific preference for interactionwith PDZ3 (Niethammer et al., 1998), even though the same C-terminalconsensus site applies to all three PDZ domains. Also, the multivalent"channel-interacting PDZ domain protein" CIPP whose PDZ domainsshow high homology to PDZ1-3 of PSD-95 selectively associateswith Kir4.1/Kir4.2 subunits (SNV) but not with Kir2.1 and Kir2.3subunits (Kurschner et al., 1998). Most recently, a specific internalPDZ domain recognition site, which mediates head-to-tail heterodimerizationwith PSD-95 and syntrophin, has been described for nNOS (Brenmanet al., 1996; Hillier et al., 1999). There, a two stranded $beta$ -fingerin nNOS, of which the first strand mimics the C-terminal PDZ motif,acts as a PDZ ligand to interact with an antiparallel $beta$ -sheetin syntrophin. In this interaction the normally required terminalcarboxylate is replaced by a sharp $beta$ -turn at the tip of the $beta$ -finger.Our electrophysiological data in HEK-293 cells may point to asimilar mode of PDZ domain scaffolding in Kir2.3 subunits. Atleast two pseudopeptide motifs, ESKI (aa 355-358) and ETGI (aa409-412), including several nearby $beta$ -turns, are present in theKir2.3 tail region in addition to the conserved terminal ESAIsequence (aa 442-445). Although direct PDZ domain interactionwith an internal Kir2.3 binding site has yet to be proven biochemically,the inhibitory action of PSD-95 on Kir2.3 currents was alleviatedwhen one of these sites was disrupted. Both internal motifs arenot present in Kir2.1 subunits (or Kir2.2 and Kir2.4), which mayexplain the slightly different results for the Kir2.1 and Kir2.3truncated mutants in the Y2Hassay.

Kir2 channels, even though their activity is subject to modulation by phosphorylation, are constitutively active and thusbalance the postsynaptic potential in the PSD. We have demonstratedcolocalization of Kir2.3 and PSD-95 in the heterologous system,and both proteins have been shown earlier to occur together inforebrain PSD fractions (Cohen et al., 1996). However, ultrastructuralevidence for Kir localization at the PSD is still missing. Theexact mechanism by which members of the PSD-95/SAP90 family mediateclustering of Kir2.3 or any other channel protein is still uncertain.The channel protein may be initially targeted uniformly to themembrane and then immobilized and clustered at the synapse bymonomeric or oligomerized PSD-95 that has already aggregated atthe synapse (Craven and Bredt, 1998; Rao et al., 1998; Burke etal., 1999). There is also evidence that chapsyns must be palmitoylated(Topinka and Bredt, 1998) and interact with a membrane proteinto be localized to the PSD and that targeting of K⁺ channels is dependent both on permissive signals from chapsynsas well as an intrinsic signal that specifies location (Arnoldand Clapham, 1999). Previous findings suggested that as a functionalconsequence of this interaction the number of Kir channels inthe membrane is increased, possibly by slowing channel turnoveror promoting tetramer assembly. When Kir4.1 channels were expressedtogether with PSD-95, SAP97 (Horio et al., 1997), or CIPP (Kurschneret al., 1998), current densities were approximately doubled withno apparent effect on the channel properties. The associationof Kir2.3 and PSD-95 predominantly affects the Kir2.3 elementaryconductance and reduces current density by half, possibly becauseof a more complex PDZ domain scaffolding with PSD-95. It is interestingto note that in the presence of PSD-95 Kir2.3 channels on a timescale of 2-3 min are still subject to inhibition by PKA phosphorylation.The phosphorylated consensus serine overlaps with the C-terminalPDZ-binding motif, and an earlier report by Cohen et al. (1996)suggested that PKA stimulation interferes with the channel bindingto PSD-95. As predicted, the free phosphorylated C terminus inKir2.1 channels acts as a channel-closing gate (Wischmeyer andKarschin, 1996).

Heteromeric Kir3 channels in the mammalian brain are directly controlled by receptor-released G $beta$ $gamma$ subunits, and the majorityare constituted from Kir3.1, Kir3.2, and Kir3.3 subunits. Allthree subunits are expressed at high levels throughout the brainwith a large degree of overlap (Karschin and Karschin, 1999).At the cellular resolution level Kir3.1 and Kir3.2 immunoreactivityhas been found in various potentially postsynaptic sites on neuronalsomata and dendritic spines but also on distal axon terminals(Murer et al., 1997). Although PSD-95/SAP90 in most neurons hasa punctate distribution (Kornau et al., 1995) and is mostly associatedwith postsynaptic densities (Hunt et al., 1996), there is no obligatecolocalization with Kir3 channels. A recent study showed thatpostsynaptically on dendrites of dopaminergic substantia nigraneurons neither PSD-95 nor SAP97 coaggregates with the abundantKir3.2 channels (Inanobe et al., 1999). It should be consideredthat Kir3 channels are directly associated with a series of heptahelicalreceptors via G proteins in a mandatory manner (Dascal, 1997),underlying many forms of slow, inhibitory synaptic transmission.Thus there is no strict requirement for Kir3 channels to be localizedand tightly clustered at the postsynaptic density typical of fastexcitatory synapses. In fact, there is plenty of evidence thatboth G protein-coupled receptors and target channels are not concentratedopposite of the nerve terminals but are rather expressed uniformly.The time constraints of these slower signaling systems are suchthat Kir channels are in the proximity of their receptors, butthey do not have to be near the transmitter release sites (Hille,1992). Based on the unsuccessful Y2H screens of rat brain librarieswith Kir3 channel termini, we tend to believe that Kir3 localizationand assembly in the signaling cascade may not be crucially dependenton PDZ domain interactions but rather are controlled through otherintrinsic targetingsignals.

  FOOTNOTES

Received Aug. 30, 1999; revised Oct. 18, 1999; accepted Oct. 20, 1999.

This work was funded by Grants Ka1175/1-2 and Ve187/1-2 from the Deutsche Forschungsgemeinschaft. We thank D. Reuter for excellenttechnical help, S. Voigt for preparing the oocytes, and M. Stockerand T. Falk for supplying cDNAs. We also thank M. Niethammer forstimulating the collaboration between Göttingen and Boston andS. Stamm for invaluable advice on the Y2Hassay.
Correspondence should be addressed to Dr. Andreas Karschin, Max-Planck-Institut for Biophysical Chemistry, Molecular Neurobiologyof Signal Transduction, Am Fassberg 11, 37070 Göttingen, Germany.E-mail: akarsch{at}gwdg.de.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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