Cell Type- and Input-Specific Differences in the Number and Subtypes of Synaptic GABAA Receptors in the Hippocampus

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The Journal of Neuroscience, April 1, 2002, 22(7):2513-2521

Cell Type- and Input-Specific Differences in the Number and Subtypes of Synaptic GABA_A Receptors in the Hippocampus
Thomas Klausberger, J. David B. Roberts, and Peter Somogyi
Medical Research Council, Anatomical Neuropharmacology Unit, Department of Pharmacology, Oxford University, Oxford OX1 3TH, United Kingdom

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Networks of parvalbumin (PV)-expressing basket cells are implicated in synchronizing cortical neurons at various frequencies,through GABA_A receptor-mediated synaptic action. These cells areinterconnected by GABAergic synapses and gap junctions, and convergewith a different class of cholecystokinin-expressing, PV-negativebasket cells onto pyramidal cells. To define the molecular specializationsin the synapses of the two basket cell populations, we used quantitativeelectron microscopic immunogold localization of GABA_A receptors.Synapses formed by PV-positive basket cells on the somata of pyramidalcells had several-fold higher density of $alpha$ ₁ subunit-containingreceptors than synapses made by PV-negative basket cells, mostof which were immunonegative. The density of the $beta$ _2/3 subunitswas similar in the two populations of synapse, indicating similaroverall receptor density. Synapses interconnecting parvalbumin-expressingbasket cells contained a 3.6 times higher overall density of GABA_Areceptor ( $beta$ _2/3 subunits) and 3.2 times higher density of $alpha$ ₁ subunitlabeling compared with synapses formed by boutons of PV-positivebasket cells on pyramidal cells. Thus, PV-positive basket cellsmainly act through $alpha$ ₁ subunit-containing GABA_A receptors, butthe receptor density depends on the postsynaptic cell type. Theseobservations, together with previously reported enrichment ofthe $alpha$ ₂ subunit-containing receptors in synapses made by PV-negativebasket cells, indicate that the number and subtypes of GABA_A receptorspresent in different synapse populations are regulated by bothpresynaptic and postsynaptic influences. The high number of GABA_Areceptors in synapses on basket cells might contribute to theprecisely timed phasing of basket cellactivity.

Key words: basket cell; pyramidal cell; IPSP; interneuron; inhibition; receptor targeting

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The heterooligomeric GABA_A receptors are anion channels opened by GABA and modulated by a variety of pharmacologically andclinically important drugs. (Macdonald and Olsen, 1994; Sieghart,1995). They are composed of five subunits, and, so far, 19 differentsubunits have been identified in the mammalian brain (Barnardet al., 1998; Sieghart et al., 1999). Most receptors consist oftwo $alpha$ , two $beta$ , and one $gamma$ subunit, but the subunit composition ishighly variable, suggesting the existence of receptors with differentfunctional and pharmacological properties (McKernan and Whiting,1996; Rudolph et al., 2001).

Hippocampal pyramidal cells receive GABAergic innervation from several distinct interneurons (Freund and Buzsaki, 1996). Forexample, axo-axonic cells innervate only axon initial segments,basket cells innervate mainly somata and the proximal dendrites,and other interneurons innervate only dendrites. The same postsynapticdomain of pyramidal cells may be targeted by more than one classof interneuron. Thus, pyramidal cell somata are innervated bytwo distinct basket cells expressing either parvalbumin (PV) orcholecystokinin (CCK). These distinct basket cells differ in theirsoma position, local and subcortical innervation, and in the presynapticcontrol of transmitter release (Hajos et al., 1998; Katona etal., 1999), predicting distinct roles in the hippocampalnetwork.

The multiple sources of GABA, released by distinct interneurons, and the large variety of distinct GABA_A receptors raise thepossibility that the segregation of inputs is supported by molecularspecializations in postsynaptic receptors. The $alpha$ ₁, $beta$ _2/3, and $gamma$ ₂subunits have been demonstrated in many GABAergic synapses onpyramidal cells (Nusser et al., 1996; Somogyi et al., 1996). However,the $alpha$ ₂ subunit was found more frequently in synapses on axon-initialsegments than on somata (Nusser et al., 1996), and, on the latter, $alpha$ ₂ subunit immunoreactivity was present at much higher levelsin synapses formed by PV-negative (presumably CCK-positive) basketcells than in synapses formed by PV-positive cells (Nyiri et al.,2001). The input-specific enrichment of $alpha$ ₂ subunit-containingreceptors raises the question whether the synapses formed by PV-positivebasket cells contain receptors formed by other subunits expressedby pyramidal cells, such as the $alpha$ ₁ subunit (Wisden et al., 1992;Fritschy and Mohler, 1995). This may be important, because the $alpha$ ₁ and $alpha$ ₂ subunit-containing receptors are responsible for differentbehavioral and pharmacological responsiveness in mice (McKernanet al., 2000; Rudolph et al., 2001).

In the present study, we tested the relative abundance of $alpha$ ₁ subunit-containing GABA_A receptors in synapses made by PV-positiveor PV-negative boutons on pyramidal cell somata. The subunit compositionof synaptic receptors may be influenced by both the source ofthe input and the identity of the target cell, but, for GABAergicconnections, this has not been tested. Because basket cells innervateboth pyramidal cells and other basket cells (Fukuda et al., 1996;Cobb et al., 1997), the subunit composition and abundance of receptorsat the synapses made by basket cells on other PV-positive basketcells was compared with those made on pyramidalcells.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Preparation of animals and tissues. Three adult male Wistar rats (~150 gm) obtained from Charles River (Kent, UK) were anesthetizedwith Sagatal (pentobarbitone sodium, 220 mg/kg, i.p.) and perfusedthrough the heart with 0.9% NaCl, followed by a fixative containing4% paraformaldehyde, 0.05% glutaraldehyde, and 0.2% picric acidin 0.1 M phosphate buffer, pH 7.4 (PB), for 20-25 min. After perfusion,the brains were left in situ for 10-15 min, and then they wereremoved from the skull. Blocks from the dorsal hippocampi weredissected and washed in 0.1 M PB, followed by sectioning on avibratome at 500 µm thickness. They were post-fixed for 15-20min and washed in 0.1 M PBovernight.

Freeze substitution and low-temperature embedding in Lowicryl resin. The same procedure was used as described previously (Baudeet al., 1993; Nusser et al., 1995; Nyiri et al., 2001). Briefly,after washing in PB overnight, the sections were placed into increasingconcentration of sucrose solutions (0.5, 1, and 2 M sucrose for0.5, 1, and 2 hr, respectively) for cryoprotection. After slammingonto copper blocks cooled in liquid N₂, and after low-temperaturedehydration and freeze substitution, the sections were embeddedin Lowicryl HM 20 resin (Chemische Werke Lowi, Waldkraiburg,Germany).

Antibodies. Rabbit polyclonal antibody (code number P16) was raised to a synthetic peptide corresponding to amino acids 1-9of the mature rat $alpha$ ₁ subunit and was affinity purified. Antibodyspecificity was described previously (Zezula et al., 1991). Thisantibody has been used in other postembedding immunocytochemicalstudies (Nusser et al., 1996, 1997, 1998a,b). Immunoreactionswere performed at a final protein concentration of 32 µg/ml. Themouse monoclonal antibody bd-17 (Haring et al., 1985) was kindlyprovided by Dr. J.-M. Fritschy (Institute of Pharmacology, Zurich,Switzerland) and has been shown to react with both the $beta$ ₂ and $beta$ ₃ subunits of GABA_A receptors (Ewert et al., 1990). The antibodywas diluted to 20 µg/ml protein. A rabbit polyclonal antiserum(code R302; 1:500 dilution) was raised to rat muscle PV (Calbiochem,Nottingham, UK) and was a gift from Dr. K. G. Baimbridge (Universityof British Columbia, Vancouver, Canada). It has been describedto be specific to PV (Mithani et al., 1987) and was used previouslyfor postembedding immunoreaction (Nyiri et al., 2001).

Postembedding immunocytochemistry. Postembedding immunocytochemistry was performed on ~70-nm-thick serial sections of slam-frozen,freeze-substituted, Lowicryl-embedded hippocampi. The sectionswere picked up on pioloform-coated nickel grids. Then they wereincubated on drops of blocking solution for 1 hr, followed byincubation on drops of primary antibodies overnight. The blockingsolution, which was also used for diluting the primary and secondaryantibodies, consisted of 0.05 M Tris-HCl, pH 7.4, containing 0.9%NaCl (TBS) and 2% human serum albumin (Sigma, Poole, UK). Afterincubation overnight in primary antibodies, sections were washedin TBS and incubated for 4 hr on drops of goat anti-rabbit orgoat anti-mouse IgG coupled to 10 or 5 nm (British BioCell International,Cardiff, UK) or ultra small gold particles (<0.8 nm; Aurion, Wageningen,Netherlands) to increase sensitivity. After several washes, sectionswere fixed in a 2% glutaraldehyde solution for 2 min. Sectionslabeled with ultra small gold particles were subjected to silverenhancement (Aurion) for 30 min. After washing in ultra pure water,all sections were contrasted with saturated aqueous uranyl acetate,followed by leadcitrate.

Because antibodies to the $alpha$ ₁ subunit and to PV were both raised in rabbit, no double labeling could be performed on the samesection. To identify PV-positive and PV-negative boutons and todifferentiate between pyramidal cells and PV-positive interneurons,one to three sections were labeled with rabbit anti-PV serum andwere detected with 10 nm gold particle-conjugated secondary antibodies.Other serial sections placed on different grids, both before andafter the PV-reacted section(s), were incubated with rabbit anti- $alpha$ ₁subunit antibodies and labeled with ultra small gold particle-conjugatedsecondary antibodies, followed by silver intensification. Fordetection of the $beta$ _2/3 subunits, serial sections were incubatedwith rabbit anti-PV and mouse anti- $beta$ _2/3 antibodies mixed together.Antibodies to PV were labeled with 5 nm gold particle-conjugatedsecondary antibodies, and antibodies to $beta$ _2/3 subunits were colabeledwith 10 nm gold particle-conjugated secondaryantibodies.

Measurement of immunoreactivity. Overall, 104 synapses in 247 sections for the $alpha$ ₁ subunit labeling and 71 synapses in 169sections for the $beta$ _2/3 subunit labeling were recorded and analyzed.In each section, several synapses were monitored. Measurementswere taken from well preserved strips of Lowicryl-embedded ultrathinsections. One block was used from each of the three rats. BecausePV-positive interneurons were relatively infrequent, blocks weresectioned repeatedly and systematically searched until sectionswith a PV-positive interneuron receiving type I synapses on thesoma were found. All type II synapses (Gray, 1959) encounteredon the somata of pyramidal cell and PV-positive interneurons wererecorded in the hippocampal CA1 region. On interneurons, typeII synapses could not always be unequivocally distinguished fromtype I synapses; therefore, here only the synapses made by PV-positiveboutons were collected, which only form type II synapses. Synapseswere defined on the basis of the rigid appositions of the plasmamembranes, the widening of the extracellular space, and, whenpresent, the postsynaptic membrane thickening. They were photographedor digitally recorded and followed through serial sections. Thenumber of gold particles was counted in a band of 35 nm from eitherside of the postsynaptic plasma membrane (Nyiri et al., 2001).The $alpha$ ₁ subunit labeling of synapses could not be fully reconstructedbecause of the use of some sections on different grids to detectPV immunoreactivity. Therefore, the density of immunogold particles,calculated as the number of gold particles per length of synapticjunction summed from one to five serial sections, was used tomeasure immunoreactivity for each individualsynapse.

For publication, photographs were scanned, and contrast and brightness of the electronic picture were adjusted. All correctionswere subjected to the whole picture; parts of the picture, e.g.,gold particles or synapses, were not selectivelyenhanced.

As a control for the specificity of the method, primary antibodies were either omitted or replaced by 5% normal rabbit ormouse sera. Selective labeling, resembling that obtained withthe specific antibodies, could not be detected under these conditions.The concentrations of primary antibodies were chosen such thatthey resulted in a very low background labeling. To estimate thecontribution of background labeling to the labeling of synapses,the density of particles was measured over synaptic vesicle-containingpresynaptic terminals, including areas occupied by mitochondria,randomly in the neuropil. These particles are assumed to representbackground labeling. Using the calculation described previously(Nyiri et al., 2001), background labeling was estimated to makea small potential contribution of 0.1 ± 0.04 particles/µm synapselength for the $alpha$ ₁ antibodies and 0.3 ± 0.1 particles/µm synapselength for the $beta$ _2/3 antibodies. Therefore, correction for backgroundlabeling was not performed. Because the center of immunoparticlesmay be up to 30 nm from the epitope and the synapses are cut atvarious angles, a contribution of the presynaptic membrane tothe labeling cannot be excluded with this method. In addition,the absence of immunolabeling cannot be taken as necessarily representingthe absence ofreceptors.

Statistics. We used nonparametric statistics for the analysis of the distribution of gold particles and for the comparisonof populations of synapses because, in many cases, their distributionwas not normal, as shown by the Kolmogorov-Smirnov test. The cutlengths of synaptic junctions were also described with nonparametricalstatistics, although their distribution was found normal withthe Kolmogorov-Smirnov test but not normal by the $chi$ ² test. The Kruskal-Wallis test was used for comparing data fromthree different groups, followed by post hoc comparisons usingthe Dunn test (Zar, 1999). Two groups were compared using theMann-Whitney U test. Statistical analysis was performed usingthe software package Statistica (StatSoft, Tulsa, OK), exceptfor the Dunntest.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Quantitative comparison of immunolabeling for the $alpha$ ₁ subunit of the GABA_A receptor in different synapses

To test a possible differential distribution of the $alpha$ ₁ subunit-containing GABA_A receptors in synapses formed by PV-negativeand PV-positive boutons on CA1 pyramidal cell somata, we performedpostembedding immunoreactions using $alpha$ ₁ subunit- and PV-specificantibodies. Because both antibodies were raised in rabbit, doublelabeling could not be performed on the same section. Instead,one to three sections were labeled with antibodies to PV (Fig.1A), and other serial sections of the same synapse were labeledfor $alpha$ ₁ subunits (Fig. 1B-D). The immunoreaction indicated a higheramount of $alpha$ ₁ subunit in synapses formed by PV-positive than insynapses formed by PV-negative boutons (Fig. 1).

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Figure 1. Differential immunolabeling for the $alpha$ ₁ subunit of the GABA_A receptor in synapses (open arrows) formed by PV-negative (b1) or PV-positive (b2) boutons on a pyramidal cell soma. A, Electron micrograph of a section immunolabeled for PV (10 nm gold particles; small arrows) showing an immunopositive (b2, small arrows) and an immunonegative (b1) bouton converging on the same pyramidal cell body. B-D, Three sections serial to A are immunolabeled for the $alpha$ ₁ subunit (silver-intensified ultra small gold particles; arrowheads). The synapse made by the PV-positive, but not the one made by the PV-negative, bouton is consistently labeled (arrowheads) for the $alpha$ ₁ subunit. Scale bar: A-D, 0.2 µm.

To compare the degree of immunolabeling of GABAergic synapses on pyramidal cells and interneurons, synapses formed by PV-positiveboutons on PV-positive cells in the pyramidal cell layer werealso investigated within the same experiment (Fig. 2). These synapseswere uniformly strongly labeled for $alpha$ ₁ subunits. In the pyramidalcell layer of the hippocampus, basket cells and axo-axonic cellshave been described to express PV (Katsumaru et al., 1988). Thecells investigated in this study received a high density of typeII synapses on their soma (Fig. 2) and, therefore, presumablyrepresent basket cells, because they have been described to beencrusted with numerous GABAergic boutons (Fukuda et al., 1996).The somata of axo-axonic cells receive a much lower density ofsynapses (P. Somogyi, unpublished observation). The hippocampusreceives a GABAergic innervation from PV-positive cells of theseptum, which terminate on interneurons, including PV-positiveones, but not on pyramidal cells (Freund and Antal, 1988; Gulyaset al., 1990). Nevertheless, most, if not all, of the PV-positiveboutons terminating on PV-positive cells are of hippocampal origin,as shown by transection of the fimbria/fornix (Fukuda et al.,1996). This might be attributable to a very low level of PV immunoreactivityof the septo-hippocampal boutons.

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Figure 2. Strong immunolabeling for the $alpha$ ₁ subunit of the GABA_A receptor in synapses made by PV-positive boutons on a PV-positive interneuron soma in the pyramidal cell layer. A, Electron micrograph of a section immunolabeled for PV (10 nm gold particles; small arrows). Three synaptic boutons (b), as well as the soma of the interneuron, are PV positive. The rightmost bouton is connected to the cell body via three punctae adherentiae. B-E, Four sections serial to A are immunolabeled for the $alpha$ ₁ subunit (silver-intensified ultra small gold particles; arrowheads), demonstrating consistent and strong immunolabeling in the synapses made by all three boutons. Scale bar: A-E, 0.2 µm.

Quantitative analysis of the $alpha$ ₁ subunit immunoreactivity from three animals revealed differences in three populations of synapse(Kruskal-Wallis test, p < 0.001; post hoc Dunn test, p < 0.05):synapses from PV-negative boutons on pyramidal cell somata, synapsesfrom PV-positive boutons on pyramidal cell somata, and synapsesfrom PV-positive boutons on PV-positive interneurons (Fig. 3).The median level of immunoreactivity was different in the threeanimals, possibly attributable to different antigen preservationof the blocks. However, the differences between the synapse populationswere comparable in the three animals tested (Fig. 3). The averagemedian particle densities in PV-positive synapses on PV-positiveinterneurons were 3.2 ± 1.5 (mean ± SD; 2.1, 2.7, and 4.9, respectively)times higher than the median particle density of PV-positive synapseson pyramidal cells. Differences between PV-positive and PV-negativesynapses on pyramidal cells could be demonstrated for all threerats but could be calculated only for rat 3, because the medianparticle density of PV-negative synapses on pyramidal cells was0 for rats 1 and 2 (Fig. 3). In rat 3, the median particle densitywas 3.0 times higher in synapses of PV-positive boutons than inthose of PV-negative boutons on pyramidal cells. In addition,in rat 3, the median particle density in synapses of PV-positiveboutons on PV-positive interneurons was 6.2 times higher thanthat in PV-negative boutons on pyramidal cells.

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Figure 3. Differences in immunoreactivity for the $alpha$ ₁ subunit of the GABA_A receptor in synapses made by PV-negative or PV-positive boutons on pyramidal cell somata (PYR) and PV-positive boutons on PV-positive interneuron somata in three adult rats. Immunoreactivity is measured as density values (number of gold particles per length of synaptic junction) obtained from one to five serial sections of each synaptic membrane. Small squares, rectangles, and bars indicate median, interquartile range (IqR), and minimum-maximum values, respectively. The three synapse populations were different from each other in all combinations and in all three rats (Kruskal-Wallis test, p < 0.001; post hoc Dunn test, p < 0.05). Note that the overall level of immunoreactivity was different in the three rats, but differences among synapse populations were comparable.

Quantitative comparison of immunolabeling for the $beta$ _2/3 subunits of the GABA_A receptor in different synapses

The different densities of $alpha$ ₁ subunits in the three types of synapses investigated could have been attributable to an overalldifferent density of GABA_A receptors or to an $alpha$ subunit-dependentdifferential distribution of GABA_A receptor subtypes in thesesynapses. The latter has been shown to be true for the $alpha$ ₂ subunit-containingGABA_A receptors in synapses of PV-negative and PV-positive boutonson CA1 pyramidal cell somata (Nyiri et al., 2001). To test whetherthe same holds true for synapses on PV-positive interneurons andpyramidal cells, synaptic immunoreactivity for the $beta$ _2/3 subunitswas investigated. The great majority of GABA_A receptors in thehippocampus are thought to contain $beta$ ₂ and/or $beta$ ₃ subunits, becausea $beta$ subunit is required for a functional receptor and the $beta$ ₁ subunitis expressed at a relatively low level in hippocampal CA1 pyramidalcells (Persohn et al., 1992; Sperk et al., 1997).

Serial sections were coimmunolabeled with mouse antibodies to $beta$ _2/3 subunits (10 nm gold particles) and rabbit antibodies toPV (5 nm gold particles). Synapses made by PV-negative and PV-positiveboutons on pyramidal cells seemed to express the similar amountof $beta$ _2/3 subunits (Fig. 4). In the same experiment, immunolabelingfor $beta$ _2/3 subunits was also investigated in synapses made by PV-positiveboutons on PV-positive interneurons in the pyramidal cell layer.These synapses were strongly immunolabeled (Fig. 5).

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Figure 4. Similar immunolabeling for the $beta$ _2/3 subunits of the GABA_A receptor in synapses (open arrows) formed by PV-negative (b1) or PV-positive (b2) boutons on a pyramidal cell soma. A, B, Electron micrographs showing two serial sections coimmunolabeled for $beta$ _2/3 subunits (10 nm gold particles; arrowheads) and for PV (5 nm gold particles; small arrows). The synaptic junction of each bouton comes into the section plane in different sections. Scale bar: A, B, 0.2 µm.

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Figure 5. Immunolabeling for the $beta$ _2/3 subunits of the GABA_A receptor in a synapse (open arrows) on the soma of a PV-positive interneuron in the pyramidal cell layer. A-C, Electron micrographs showing three serial sections coimmunolabeled for the $beta$ _2/3 subunits (10 nm gold particles; arrowheads) and for PV (5 nm gold particles; small arrows). Note that the bouton (b), as well as the soma of the interneuron, is PV positive (small arrows). Scale bar: A-C, 0.2 µm.

Quantitative analysis of $beta$ _2/3 subunit immunoreactivity showed that synapses made by PV-negative and PV-positive boutons onpyramidal somata were not different in any of the three animals(Mann-Whitney U test, p > 0.5), confirming a previous study (Nyiriet al., 2001). Therefore, these synapses were pooled and comparedwith the immunoreactivity of synapses on interneurons (Fig. 6).Interestingly, the immunolabeling for $beta$ _2/3 subunits was significantlylower in synapses on pyramidal cell somata than in synapses onPV-positive interneurons in all three rats (Mann-Whitney U test,p < 0.005). The average median particle density in synapses madeby PV-positive boutons on PV-positive interneurons was 3.6 ± 0.6(mean ± SD; range of 2.9, 3.7, and 4.1, respectively) times higherthan the median particle density of synapses on pyramidal cells.These results indicate that synapses made by PV-positive boutonson basket cell somata have a higher overall GABA_A receptor densitythan synapses on pyramidal cell somata.

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Figure 6. Difference in immunoreactivity for the $beta$ _2/3 subunits of the GABA_A receptor on PV-negative, PV-positive, or pooled populations of synapses on pyramidal cell somata (PYR), and PV-positive synapses on PV-positive interneuron somata in three adult rats. Immunoreactivity is measured as density values (number of gold particles per length of synaptic junction) obtained from one to five serial sections of each synaptic membrane. Small squares, rectangles, and bars indicate median, interquartile range (IqR), and minimum-maximum values, respectively. Immunoreactivity for the $beta$ _2/3 subunits in synapses made by PV-negative and PV-positive boutons on pyramidal cell somata was not different in any of the rats (Mann-Whitney U test, p > 0.5) (Nyiri et al., 2001); therefore, the data were pooled. Synapses on pyramidal cell somata and PV-positive synapses on interneurons were different in all three rats (Mann-Whitney U test, p < 0.005).

Comparison of the size of GABAergic synapse populations

To test whether the three synapse populations differ in the size of the synaptic specialization, in addition to the densityof $alpha$ ₁ and $beta$ _2/3 subunit-containing receptors, the lengths of synapsespresented in Figures 3 and 6 were compared. Synapses from thesame population with respect to PV labeling, but from three differentanimals, were not different in size; therefore, they were pooled(Kruskal-Wallis test, p > 0.05). The median length of synapticmembrane per section was 0.21 µm (interquartile range of 0.17-0.26;n = 122) for synapses made by PV-negative boutons on pyramidalcell somata, 0.20 µm (interquartile range of 0.17-0.27; n = 126)for synapses made by PV-positive on pyramidal cell somata, and0.21 µm (interquartile range of 0.16-0.25; n = 166) for synapsesmade by PV-positive boutons on PV-positive interneuron somata.The three synapse populations do not differ in their average synapticlength per section (Kruskal-Wallis test, p > 0.3). These resultsindicate that the higher overall density of GABA_A receptors insynapses on basket cell somata compared with synapses on pyramidalcell somata is not a compensation for a smaller synaptic junctionalarea.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We showed that at least three synapse populations have different densities of $alpha$ ₁ subunit-containing GABA_A receptors in thehippocampal pyramidal cell layer. Synapses made by PV-negativeboutons on pyramidal cell somata contain very low density of $alpha$ ₁subunit; those made by PV-positive boutons on pyramidal cell somatacontain an intermediate level, and synapses on PV-positive basketcell somata contain the highest density of $alpha$ ₁ subunits. The highdensity of $alpha$ ₁ subunits in synapses on basket cells correspondsto a higher overall density of GABA_A receptors compared with pyramidalcell synapses, as shown by the correspondingly higher densityof immunoreactivity for the $beta$ _2/3 subunits. In contrast, the differentdensities of $alpha$ ₁ subunit labeling in synapses made by PV-negativeand PV-positive boutons on pyramidal cells are attributable toan input-specific difference in the $alpha$ subunit composition of GABA_Areceptors.

Different amounts of $alpha$ ₁ subunit-containing GABA_A receptor in synapses on pyramidal cells

A relatively even frequency of synapses with $alpha$ ₁ subunit-containing receptors were reported on distinct postsynaptic domainsof pyramidal cells (Nusser et al., 1996). However, within onedomain, the soma, the present study revealed differences betweentwo synapse populations. The results are consistent with a higheramount of $alpha$ ₂ subunit-containing GABA_A receptor in synapses madeby PV-negative boutons compared with those made by PV-positiveboutons (Nyiri et al., 2001). The evidence provided here showsthat the enrichment of $alpha$ ₂ subunits in one of the synapse populationsis accompanied by a lower amount of $alpha$ ₁ subunits and vice versa.The immunocytochemical findings are in agreement with the differentialeffect of an $alpha$ ₁ subunit-selective benzodiazepine agonist on synapticresponses (Thomson et al., 2000). The results together clearlyindicate that different GABA_A receptor subtypes are selectivelydistributed in an input-dependent manner. For such a distributionof receptors, it is necessary that the presynaptic bouton signalsthe postsynaptic cell its identity and the postsynaptic cell convertsthis information to a selective targeting and/or maintenance ofdifferent GABA_A receptor subtypes (Connolly et al., 1996; Mossand Smart, 2001). Whether other $alpha$ subunits, such as $alpha$ ₄ and $alpha$ ₅subunits (Sperk et al., 1997; Fritschy et al., 1998), are alsoselectively distributed will be investigated in future studies,but pharmacological evidence indicates further receptor specializations(Pawelzik et al., 1999). In addition, different GABA_A receptorsubtypes may be targeted also selectively to different cell domains,such as the axon (MacDermott et al., 1999), or the extrasynapticplasma membrane (Nusser et al., 1998b).

Distribution of $alpha$ ₁ subunit-containing GABA_A receptors on pyramidal and basket cells

Immunoreactivity for the $alpha$ ₁ subunit is expressed throughout the entire hippocampus (Fritschy and Mohler, 1995; Sperk et al.,1997; Pirker et al., 2000). Consistent with the present study,very strong immunostaining for the $alpha$ ₁ subunit was reported inhippocampal PV-positive cells (Gao and Fritschy, 1994; Fritschyand Mohler, 1995; Sperk et al., 1997). Much of this is clearlyattributable to extrasynaptic receptors (Nusser et al., 1995;Somogyi et al., 1996). The strong $alpha$ ₁ subunit immunoreactivityof PV-positive cells has sometimes been interpreted as showingthat most $alpha$ ₁ subunits are on interneurons, and, consequently,drugs acting on $alpha$ ₁ subunit-containing receptors might exert theiraction through these cells. Because of the expression of the $alpha$ ₁subunit by all pyramidal cells (Persohn et al., 1992; Wisden etal., 1992) and the low number of basket cells compared with pyramidalcells, this suggestion is reevaluated in the followingcalculation.

Synapses made by PV-positive boutons on PV-positive basket cells somata have 3.2 times more immunolabeling for the $alpha$ ₁ subunitthan PV-positive synapses on pyramidal cells and 6.2 times morelabeling than PV-negative synapses (see rat 3). The dimensionsof synapses were not different. Assuming that the density of immunolabelingis proportional to the abundance of functional receptors containingthat subunit (Nusser et al., 1997), neglecting the minority ofPV-negative boutons on basket cell somata (Fukuda et al., 1996),and considering that 68% of synapses on pyramidal cell somataare from PV-positive boutons (Nyiri et al., 2001), it can be calculatedthat a type II synapse on a basket cell soma contains on averageof 3.8. times more $alpha$ ₁ subunits than one on a pyramidal cell soma.Because PV-positive basket cells receive 1.9 times more type IIsynapses on the soma than pyramidal cells (Gulyas et al., 1999;Megias et al., 2001) and there are 48 times more pyramidal thanPV-positive cells (Aika et al., 1994), it follows that overallthere are ~6.7 times more $alpha$ ₁ subunits in somatic synapses on pyramidalcells than in somatic synapses on PV-positive basket cells. Althoughthis rough estimation neglects $alpha$ ₁ subunits in dendritic synapses,in the extrasynaptic membranes, and on other cell types, it predictsthat the majority of synaptic $alpha$ ₁ subunits in the CA1 area of thehippocampus are on pyramidal cells and not on basket cells. Thepresence of the same subunit of the GABA_A receptor on differentcell types indicates that receptor subtype-specific drugs mightnot provide selective tools for specific celltypes.

Pathway-dependent synaptic enrichment of $alpha$ ₁ subunit-containing GABA_A receptors

Although most receptor subtypes are expressed by several cell types, there seems to be a pathway-dependent distribution ofsome GABA_A receptor subtypes. Basket cells expressing PV are stronglyinterconnected with each other and also innervate pyramidal cellsomata (Katsumaru et al., 1988; Fukuda et al., 1996). In bothsynapse populations, a high amount of $alpha$ ₁ subunit-containing GABA_Areceptor has been found. Interestingly, the preferential use of $alpha$ ₁ subunits by this pathway is consistent with recent genetic,pharmacological, and behavioral studies, indicating that $alpha$ ₁ subunit-containingreceptors are important for mnemonic processes. A point mutationin the $alpha$ ₁ subunit, rendering $alpha$ ₁ subunit-containing receptors insensitiveto benzodiazepines, leads to a decrease in the amnesic and sedativeeffects of diazepam (Rudolph et al., 1999; McKernan et al., 2000).It is possible that diazepam causes memory impairment and sedationvia synapses interconnecting PV-positive basket cells and thebasket cell to pyramidal cell circuit, which are enriched in $alpha$ ₁subunit-containing receptors. This synaptic organization is presentprobably also in the isocortex and amygdala. During exploration,when new memories are formed and established ones recalled, networkoscillations in the theta and gamma frequency range occur in thehippocampus (Bragin et al., 1995) and other cortical areas (Jefferyset al., 1997). These oscillations are thought to be strongly influencedby GABAergic and electrical interactions between PV-positive basketcells, which are able to regulate the precise timing of principalcell discharge (Buzsaki and Chrobak, 1995; Cobb et al., 1995;Tamas et al., 2000).

In contrast, PV-negative (CCK/vasoactive intestinal poly-peptide-positive) basket cells do not appear to express the $alpha$ ₁ subunit(Gao and Fritschy, 1994), and also their synapses made on pyramidalcells contain only a low amount of $alpha$ ₁ subunit. The role of thispathway remains to be clarified. However, the pathway-dependentdistribution of GABA_A receptor subtypes and their specific functionsin the brain demonstrate the opportunity for developing receptorsubtype-specific drugs for selective functionaleffects.

Implications of the high number of GABA_A receptor in synapses on basket cells

Synapses on PV-positive basket cell somata contain a higher density of GABA_A receptors than synapses on pyramidal cells. Thismight influence the amplitude of miniature IPSCs (Nusser et al.,1997), but we are unaware of electrophysiological data comparingthe two populations of synapse in the hippocampal CA1 region.The amplitude of IPSCs in other types of interneuron and pyramidalcells do not differ greatly (Hajos and Mody, 1997; Hajos et al.,2000), which could reflect a delicate balance between receptornumber and receptor occupancy (Nusser et al., 1997). However,in the dentate gyrus, the mean decay time constant of IPSCs wasapproximately twofold faster in interbasket cell synapses thanin granule cell synapses (Bartos et al., 2001). This may be explainedby the different GABA_A receptor subtypes of these cells (Lavoieet al., 1997) or by steric relationships of synapses or modulationof receptors, dependent on the postsynaptic cell (Overstreet etal., 2000; Moss and Smart, 2001). Bartos et al. (2001) also reporta larger peak amplitude of IPSCs in basket cells compared withgranule cells. This might be caused by a higher number of GABA_Areceptors on basket cell synapses, similar to that found in thepresent study for basket cells in the CA1 area. As a consequence,the synaptic peak conductance change was much higher in basketcell synapses compared with granule cell synapses. This is proposedto have a critical role in the generation of coherent, high-frequencyoscillations (Wang and Buzsaki, 1996; Bartos et al., 2001), whichare believed to be important for mnemonic processes. Overall,the higher number of synaptic GABA_A receptors and the bias forreceptor subtypes containing $alpha$ ₁ subunits by PV-positive basketcells supports a phasic, precisely timed inhibition of basketcells, leading to a coherent interneuron network oscillation.The lower amount of GABA_A receptors in GABAergic synapses on pyramidalcell somata, together with a wide variety of potential synapticreceptors, predicts a large variability in their inhibitoryresponses.

  FOOTNOTES

Received Sept. 24, 2001; revised Dec. 20, 2001; accepted Dec. 20, 2001.

T.K. was supported by an Erwin Schroedinger Fellowship of the Austrian Science Fund. We thank Dr. Werner Sieghart (Brain ResearchInstitute, Vienna, Austria) for providing the antibody to the $alpha$ ₁ subunit, Dr. J.-M. Fritschy (Institute of Pharmacology, Zurich,Switzerland) for antibody bd17, and Dr. K. G. Baimbridge, (Departmentof Physiology, University of British Columbia, Vancouver, Canada)for the rabbit antibodies to parvalbumin. We also thank Dr. YannisDalezios for help with statistics, and Dr. Zoltan Nusser and GaborNyiri for helpful comments on an earlier version of this manuscript.Philip Cobden, Paul Jays, and Dr. Laszlo Marton provided excellenttechnicalassistance.

Correspondence should be addressed to Dr. Thomas Klausberger, Medical Research Council, Anatomical Neuropharmacology Unit,Oxford University, Department of Pharmacology, Mansfield Road,Oxford OX1 3TH, UK. E-mail: thomas.klausberger{at}pharm.ox.ac.uk.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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