Glutamate Receptors in the Rod Pathway of the Mammalian Retina

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The Journal of Neuroscience, November 1, 2001, 21(21):8636-8647

Glutamate Receptors in the Rod Pathway of the Mammalian Retina
Krishna K. Ghosh, Silke Haverkamp, and Heinz Wässle
Max-Planck-Institut für Hirnforschung, Neuroanatomie, D-60528 Frankfurt, Germany

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Rod bipolar (RB) cells of the mammalian retina release glutamate in a graded, light-dependent fashion from 20 to 40 ribbonsynapses (dyads). At the dyads, two classes of amacrine cells,the AI and AII cells, are the postsynaptic partners. We examinedthe glutamate receptors (GluRs) that are expressed by AI and AIIcells using immunocytochemistry with specific antibodies againstGluR subunits. Sections of macaque monkey and rabbit retina wereexamined by confocal microscopy. AII amacrine cells were selectivelylabeled for calretinin, and AI cells in rabbits were labeled for5-HT uptake. Thus, double- and triple-labeling for these markersand GluR subunits was possible. Electron microscopy using postembeddingimmunocytochemistry and double-labeling was applied to show thesynaptic expression of GluRs. We also studied the synaptic localizationof the two postsynaptic density proteins PSD-95 and glutamatereceptor-interacting protein (GRIP). We found that AII amacrinecells express the AMPA receptor subunits GluR2/3 and GluR4 atthe RB cell dyads, and they are clustered together with PSD-95.In contrast, AI amacrine cells express the $delta$ 1/2 subunits thatappear to be associated with kainate receptor subunits and tobe clustered together with GRIP. The RB cell dyad is thereforea synapse that initiates two functionally and molecularly distinctpathways: a "through conducting" pathway based on AMPA receptorsand a modulatory pathway mediated by a combination of $delta$ 1/2 subunitsand kainatereceptors.

Key words: AMPA receptors; $delta$ subunits; kainate receptors; GRIP; PSD-95; monkey retina; rabbit retina; AI amacrine cells; AII amacrine cells; rod bipolar dyad

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In the scotopic pathway of the mammalian retina, rods are connected to rod bipolar (RB) cells. These do not synapse directlyonto ganglion cells in the inner plexiform layer (IPL); instead,their output synapses (dyads) involve two classes of amacrinecells, generally named AI and AII cells (Kolb and Famiglietti,1974; Famiglietti and Kolb, 1975). AII amacrine cells are a singletype that makes glycinergic inhibitory synapses with off-conebipolar cells (Sassoè-Pognetto et al., 1994; Grünert and Wässle,1996) and contacts on-cone bipolar cells via large gap junctions(Mills and Massey, 2000; Feigenspan et al., 2001). In this waythey produce signals of opposite polarity in on- and off-ganglioncells. AI cells are a mixed group of GABAergic amacrine cellsthat often provide a reciprocal synapse back onto the RB cellaxon terminal. This summary of the rod synaptic pathway appearsto be a constant constituent of mammalian retinal organization,despite alternative pathways described more recently (Soucy etal., 1998; Hack et al., 1999).

RB cells are depolarized by a light stimulus that is projected into their receptive field center (Dacheux and Raviola, 1986;Euler et al., 1996; Berntson and Taylor, 2000; Euler and Masland,2000). Glutamate, their transmitter, is continuously releasedin a light-dependent manner at their axon terminals in the IPL(von Gersdorff et al., 1996; Tachibana, 1999). The actual releasesites are the active zones at the ribbons (von Gersdorff, 2001).In the rabbit retina, up to 40 ribbons were found in RB terminals(Strettoi et al., 1992), whereas in the macaque monkey retina,~20 ribbons were observed (Grünert and Martin, 1991). Hence,between 40 and 80 postsynaptic contacts are expected at individualRB axon terminals. At these contacts, aggregates of glutamatereceptors (GluRs) and postsynaptic density proteins have beendemonstrated (Brandstätter et al., 1998; Koulen et al., 1998a,b;Qin and Pourcho, 1999a,b, 2000, 2001). However, a detailed studyof the GluRs expressed by the AI and AII amacrine cells at theRB cell dyad is stillmissing.

Ionotropic GluRs have been subdivided into three major groups: AMPA, kainate, and NMDA receptors. Our laboratory has previouslyshown that the NMDA receptor subunits NR1, NR2A, and NR2B areabsent from RB cell dyads (Fletcher et al., 2000); therefore,they will not be dealt with here. Molecular cloning has shownthat AMPA receptors are complexes of the subunits GluR1, GluR2,GluR3, or GluR4. Kainate (KA) receptors are composed of the subunitsGluR5, GluR6, GluR7, KA-1, or KA-2. In addition, the orphan receptorsubunits $delta$ 1 and $delta$ 2 are associated with these GluRs (Hollmann andHeinemann, 1994; Ozawa et al., 1998; Dingledine et al., 1999).

In the present study, we first focused on the macaque monkey retina and studied the localization of GluRs with immunocytochemicalmarkers using both light and electron microscopy. RB cells werelabeled with antibodies against protein kinase C (PKC) (Grünertand Martin, 1991), and AII cells were labeled with antibodiesagainst calretinin (Wässle et al., 1995; Mills and Massey, 1999).Different GluR subunits and synapse-associated proteins couldbe localized to the RB cell dyads. Their precise position at thedyad was studied by labeling the RB cell ribbons with antibodiesagainst kinesin (Muresan et al., 1999). Unfortunately, it is notpossible to label AI cells of the macaque monkey selectively.However, AI cells of the rabbit retina can be labeled by theiruptake of serotonin (5-HT) (Holmgren-Taylor, 1982; Sandell andMasland, 1986; Vaney, 1986; Sandell et al., 1989). We thereforestudied the expression of GluRs by AI cells in the rabbit retina.Because AII cells of the rabbit retina are immunoreactive forcalretinin (Massey and Mills, 1999) and RB cells are immunoreactivefor PKC (Greferath et al., 1990), all three members of the dyadcould be studied by immunocytochemicalmethods.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals and tissue preparation. The monkey retinas that were studied were from adult macaque monkeys, Macaca fascicularis,that were killed after electrophysiological experiments unrelatedto those described here. All procedures were approved by the localanimal care committee and were in accordance with the law foranimal experiments issued by the German government (Tierschutzgesetz).The animals were given a lethal dose of pentobarbitone, and theeyes were quickly removed. The posterior eyecup was immersion-fixedin 2 or 4% paraformaldehyde in 0.1 M phosphate buffer (PB), pH7.4, for 10-30 min. After fixation, the retinas were dissectedfrom the eyecup and cryoprotected in graded sucrose solutions(10, 20, and 30%). Retinal pieces were sectioned vertically at14 µm. Albino rabbits were deeply anesthetized with Ketanest andRompun before being given a lethal injection of pentobarbitol.The eyes were quickly removed and prepared as described abovefor the monkey retinas. In some cases, the eyecup was incubatedfirst in 25 µM 5-hydroxytryptamine (5-HT) (Sigma, Taufkirchen,Germany) in continuously carboxygenated Ames medium for 1 hr beforefixation andcryoprotection.

For electron microscopy (EM), it was necessary to make a compromise between the preservation of the tissue and the protectionof the antigenicity. Epitopes of proteins aggregated in postsynapticdensities are very fixation-sensitive; to maximize immunoreactivity,the tissue received only minimal fixation (4% paraformaldehyde;30 min) and was cryoprotected in up to 50% sucrosesolution.

Antisera. Rod bipolar cells were labeled with antibodies against PKC $alpha$ : mouse anti-PKC (clone MC5; Biodesign International,Saco, ME) and goat anti-PKC (Santa Cruz Biotechnology, Santa Cruz,CA). AII amacrine cells were labeled with antibodies against calretinin(CR): mouse anti-CR and goat anti-CR (Chemicon, Temecula, CA).In addition, in the rabbit retina, AI amacrine cells were labeledby uptake of 5-HT, which was then visualized using an antibodyagainst 5-HT, mouse anti-5-HT (Dako, Glostrup, Denmark). Specificantibodies against glutamate receptor subunits were used: rabbitanti-GluR1, rabbit anti-GluR2, rabbit anti-GluR2/3, rabbit anti-GluR4,and rabbit anti- $delta$ 1/2 (Chemicon). Ribbon synapses were labeledusing a marker for the membrane traffic motor protein kinesin,mouse anti-kinesin II (Babco, Richmond, CA). The postsynapticdensity protein PSD-95 was labeled with mouse anti-PSD-95 (UpstateBiotechnology Inc., Lake Placid, NY), and the glutamate receptor-interactingprotein (GRIP) was labeled with rabbit anti-GRIP (kind gift fromDr. M. Sheng, Massachusetts General Hospital, Boston, MA) andmouse anti-GRIP (Transduction Laboratories, Lexington,KY).

Light microscopic immunocytochemistry. The antisera were diluted as follows: mouse anti-PKC, 1:100-1:2000; goat anti-PKC,1:2000; mouse anti-CR, 1:1000-1:2000; goat anti-CR, 1:1000; 5-HT,1:1000; GluR1, 1:25-1:50; GluR2, 1:50; GluR2/3, GluR4, and $delta$ 1/2,1:100; kinesin II, 1:50; PSD-95, 1:1000; rabbit anti-GRIP, 1:500;mouse anti-GRIP, 1:5000; in PBS, pH 7.4, containing 3% normalgoat serum (NGS), 1% bovine serum albumin (BSA), and 0.5% TritonX-100. Immunocytochemical labeling was performed using the indirectfluorescence method. After preincubation in PBS containing 10%NGS, 1% BSA, and 0.5% Triton X-100, the sections were incubatedovernight in the primary antibodies, followed by incubation (1hr) in the secondary antibodies, which were conjugated eitherto Alexa TM 594 (red fluorescence) or Alexa TM 488 (green fluorescence)(purchased from Molecular Probes, Eugene,OR).

In double-labeling experiments, sections were incubated in a mixture of primary antibodies followed by a mixture of secondaryantibodies. In the case of the PKC and CR antibodies raised ingoat, we have used normal donkey serum (NDS) instead of NGS plusAlexa TM 488 donkey anti-goat (Molecular Probes) and Cy3 donkeyanti-rabbit (Jackson ImmunoResearch, West Grove, PA) as secondaryantibodies.

In the triple-labeling experiments, Cy5 donkey anti-mouse (Jackson ImmunoResearch) was used in addition to the Alexa TM 488and Cy3 secondary antibodies. All secondary antibodies were diluted1:500 in PBS containing 3% NGS, 1% BSA, and 0.5% Triton X-100.

Fluorescent specimens were viewed using a Zeiss (Oberkochen, Germany) Axiophot microscope equipped with a fluorescent filterset that was wedge-corrected, i.e., shifting from one filter tothe other filter did not introduce spatial displacements. Forthe high-power fluorescence micrographs, a Plan-Neofluar 100×/1.3objective was used. Black-and-white digital images were takenwith a cooled CCD camera (Spot 2; Diagnostic Instruments, SterlingHeights, MI). Using the Metaview software (Universal Imaging,West Chester, PA), images taken with the red and green fluorescencefilters were pseudocolored and superimposed (see Figs. 2F-K, 4B-D,F-H).Confocal micrographs were taken using a Leica TCS SP confocalmicroscope equipped with a krypton-argon laser or a Zeiss LSM5Pascal confocal microscope equipped with an argon laser and aHeNe laser. High resolution scanning was performed with a Plan-Apochromat63×/1.4 objective and with 1024 × 1024 or 2048 × 2048 pixels.Single optical sections are shown in Figures 1, 4, A and E, 5,and 7. Serial sections were also taken (z-axis step size, 0.5µm) and the stacks were subsequently collapsed into a single plane(see Fig. 2A-E; 10 sections of 0.5 µm.) The brightness and thecontrast of the final images were adjusted using Adobe Photoshop5.5.

Postembedding immunoelectron microscopy. The slam-freezing and cryosubstitution methods used in this study are a modificationof those previously described (Baude et al., 1993). Briefly, smallpieces of retina were slam-frozen onto a precooled copper blockusing a Reichert MM80 U (Leica, Bensheim, Germany). The frozenspecimens were transferred then to a cryosubstitution unit (ReichertAFS; Leica) and placed into a solution of 0.5% uranyl acetate(w/v) in 100% methanol at $-$ 90°C. After 36 hr, the temperaturewas increased stepwise to $-$ 30°C. Then, the samples were washedseveral times in precooled methanol and progressively infiltratedwith Lowicryl HM20 (Chemische Werke Lowi GmbH, Waldkraiburg, Germany)(1:1 Lowicryl to methanol, 90 min; 2:1 Lowicryl to methanol, 90min; 100% Lowicryl, 90 min; 100% Lowicryl, overnight). Polymerizationwas achieved by exposure to UV light for 12hr.

Ultrathin sections were cut and collected on Formvar-coated nickel grids. The sections were incubated first in 0.05 M Tris-bufferedsaline (TBS), pH 7.6, for 15 min, followed by a blocking solutioncontaining 10% NDS, 0.1% cold-water fish skin (CWSC) gelatin (Aurion,Wageningen, The Netherlands) and TBS with 0.1% Triton (TBST) for20 min. Sections were incubated overnight in primary rabbit anti-GluR2/31:10 alone or in a mixture of GluR2/3 and goat anti-CR 1:500 dilutedin 1% NDS, 0.1% CWSC gelatin, and TBST. After washing in TBS,sections were incubated for 2 hr in secondary donkey anti-rabbitIgG conjugated to 12 nm gold (Jackson ImmunoResearch) diluted1:20 in 1% NDS, 0.1% CWSC gelatin, and TBST or in a mixture ofdonkey anti-goat IgG conjugated to 12 nm gold and donkey anti-rabbitIgG conjugated to 6 nm gold. After further washing in TBS andPB, the sections were fixed for 5 min in 2% glutaraldehyde inPB, washed in distilled water, and counterstained with uranylacetate and lead citrate. Then, the grids were viewed with a ZeissEM10 electronmicroscope.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

AMPA-receptor subunits at the rod bipolar cell axon terminal

RB cells of a macaque monkey retina are labeled in Figure 1A for PKC $alpha$ . RB cell dendrites contact rod spherules in the outerplexiform layer (OPL), and RB cell axons descend into the lower(inner) part of the IPL where they terminate in lobular swellings(Fig. 1A). In the primate retina, PKC immunoreactivity is alsofound in an on-cone bipolar cell type (Grünert et al., 1994;Mills and Massey, 1999); however, the labeling is weaker thanthat of RB cells, and the axon terminals occupy a narrow bandabove the RB axon terminals (Fig. 1A, double-headed arrow). Thesame section was also labeled for GluR4 (Fig. 1B), and immunoreactivepuncta are found at the positions of the cone pedicles in theOPL (Haverkamp et al., 2001) and throughout the IPL. Such punctatestaining of transmitter receptors in the IPL has been shown previouslyto represent a clustering of the receptors in postsynaptic densities(Brandstätter et al., 1998; Wässle et al., 1998). Few outputsynapses have been described along the descending axons of theRB cells, the majority being found on their lobular axon terminals(Grünert and Martin, 1991). Most of the GluR4 clusters in theIPL are, therefore, associated with off- and on-cone bipolar cellterminals; only those in the lower part of the IPL are expectedto be postsynaptic to RB cells (Fig. 1B). Only this particularregion is shown in the high-power micrographs of Figure 1, C-J.A section that was double-labeled for PKC and GluR1 is shown inFigure 1, C and D, respectively. There are no GluR1 immunoreactivepuncta in close apposition to the RB axon terminals, and we concludethat this subunit is not expressed postsynaptically to RB cells.A section that was double-labeled for PKC and GluR2 (Fig. 1E,F)shows a few puncta in register with the RB axon terminals (arrowheads).The section in Figure 1, G and H, was double-labeled for PKC andthe GluR2/3 subunits. The RB axon terminals are decorated by manyGluR2/3 immunoreactive puncta (arrowheads). The same holds truefor a section that was double-labeled for PKC and the GluR4 subunit(Fig. 1I,J). Most GluR4 immunoreactive puncta in this inner partof the IPL coincide with RB axon terminals (arrowhead). The resultspresented in Figure 1 suggest that AMPA receptors are aggregatedin postsynaptic densities at the RB axon terminals. Clusters containingthe GluR2/3 and/or the GluR4 subunits are observed most frequentlythere. The GluR1 subunit is not found in association with RB axonterminals.

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Figure 1. Localization of the AMPA receptor subunits GluR1, GluR2, GluR2/3, and GluR4 at the RB cell axon terminals of the macaque monkey retina. A, Fluorescence micrograph of a vertical section immunostained for PKC. The retinal layers are indicated. OPL, Outer plexiform layer; INL, inner nuclear layer; IPL, inner plexiform layer; arrow, axon terminals of labeled cone bipolar cells. B, Same section as in A immunostained for GluR4. C, D, The inner part of the IPL of a vertical section that was double-labeled for PKC (C) and GluR1 (D). The bright puncta in D represent synaptic clusters of GluR1. The RB axon terminals are also shown faintly in D (and in micrographs F, H, and J). E, F, The inner part of the IPL of a vertical section that was double-labeled for PKC (E) and for the GluR2 subunit (F). The arrowhead shows an axonal varicosity that is decorated by GluR2-immunoreactive puncta. G, H, The inner part of the IPL of a vertical section that was double-labeled for PKC (G) and for the GluR2/3 subunit (H). The arrowheads show axonal varicosities that are surrounded by GluR2/3-immunoreactive puncta. I, J, The inner part of the IPL of a vertical section that was double-labeled for PKC (I) and for the GluR4 subunit (J). The arrowhead shows an axonal varicosity that is covered by GluR4-immunoreactive puncta. Scale bars: A, B, 20 µm; C-J, 5 µm.

To show more directly the clustering of AMPA receptors at the RB cell dyad, we triple-labeled a section through the rabbitretina for PKC, GluR2/3, and kinesin (Fig. 2). Kinesin has recentlybeen shown to be a marker of the synaptic ribbons both in theOPL and the IPL (Muresan et al., 1999). In the low-power micrograph(Fig. 2A), the OPL appears overexposed because of the very strongred immunofluorescence of the horseshoe-shaped ribbons in therod spherules (arrows). The rod bipolar cells are shown in blue,and their descending axons terminate in the lower IPL. The IPLis filled with red (kinesin), green (GluR2/3), and yellow puncta(kinesin-GluR2/3 double-labeled). The RB axon terminal region,indicated by a box, is magnified in Figure 2, B-E, and the RBaxon terminals (Fig. 2B), the ribbons (Fig. 2C), and the GluR2/3clusters (Fig. 2D) are shown separately or superimposed (Fig.2E). Observing this region through all four micrographs showsthat most of the ribbons in this lower part of the IPL coincidewith RB axon terminals and thus represent RB cell dyads. Moreover,there is basically a one-to-one relation between the ribbons (Fig.2C, red puncta) and the GluR2/3 clusters (Fig. 2D, green puncta).At every dyad of RB cell axon terminals, AMPA receptors are expressed.The same result was also found for RB axon terminals of the macaquemonkey retina (data not shown).

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Figure 2. A-E, Confocal micrographs of a section through the rabbit retina that was triple-labeled for PKC (blue), kinesin (red), and GluR2/3 (green). A, Low-power micrograph showing the retinal layers. The arrows in the OPL indicate the ribbons of rod spherules. The inner part of the IPL is shown at higher magnification in B-E. B, PKC-immunostained RB cell axon terminals. C, Kinesin-labeled presynaptic ribbons. D, GluR2/3-labeled hot spots. E, Superposition of B, C, and D. All GluR2/3-immunoreactive puncta in the bottom half of the IPL coincide with kinesin-labeled ribbons and PKC-labeled RB cell axon terminals. F-H, Fluorescence micrographs of the inner part of a macaque monkey IPL that was double-labeled for GluR2/3 (red) and PSD-95 (green). The superposition of the immunoreactive puncta in H shows that all GluR2/3 puncta coincide with PSD-95 puncta. I-K, Fluorescence micrographs of the inner part of a macaque monkey IPL that was double-labeled for GluR4 (red) and PSD-95 (green). K, All GluR4- immunoreactive puncta coincide with PSD-95 labeled puncta. Scale bar (shown in A): A, 10 µm; B-E, 7.5 µm; F-K, 2.5 µm.

Next, we wanted to know the subunit composition of the AMPA receptors expressed at RB axon terminals. Because both the GluR2/3and the GluR4 antibodies were raised in rabbits, we could notperform direct double-labeling and thus used a different approach.We have shown previously that the postsynaptic density proteinPSD-95 is aggregated at postsynaptic densities of RB cell dyads(Koulen et al., 1998a). PSD-95 belongs to a family of GluR-clusteringmolecules (for review, see Kennedy, 2000; Scannevin and Huganir,2000). We double-labeled sections through the macaque monkey retinafor PSD-95 and GluR2/3 (Fig. 2F-H), and for PSD-95 and GluR4 (Fig.2I-K). All GluR2/3 immunoreactive puncta coincided with PSD-95immunoreactive clusters. The same holds true for GluR4 immunoreactivepuncta. There were only a few PSD-95 immunoreactive clusters leftthat were not in register with GluR2/3 or GluR4 puncta. This showsthat the great majority of GluR2/3 and GluR4 puncta must be inregister and occur in the same postsynaptic density. This wouldsuggest that most AMPA receptors expressed at the RB cell dyadare composed of the GluR2/3 and the GluR4 subunits. Finally, PSD-95appears to be a reliable marker for AMPA receptors at RB celldyads.

We also studied the localization of AMPA receptors at RB cell dyads by pre-embedding and post-embedding immunocytochemistryand EM. In the EM micrographs, as a rule, only one of the twopostsynaptic elements expressed an AMPA receptor subunit (Fig.3). Only rarely were both members of the dyad labeled. Unfortunatelythe tissue preservation was compromised because of the necessityof using short fixation times. For this reason, we were not ablein the EM micrographs to observe reciprocal synapses in the vicinityof the dyads that would indicate that the labeled processes belongto AI amacrine cells. In addition, we could not recognize AIIamacrine cells from the characteristic organelles in their cytoplasm(Kolb and Famiglietti, 1974). However, it will be shown laterthat we were able to recognize AII amacrine cells in EM micrographsof calretinin-labeled sections.

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Figure 3. Electronmicrograph of a section through a RB cell dyad of a macaque monkey retina. The section was immunolabeled for GluR2/3 using postembedding immunocytochemistry and secondary antibodies that were coupled to gold particles of 12 nm diameter. RB, Axon terminal; A, unlabeled postsynaptic process; A*, labeled postsynaptic process; arrowhead, presynaptic ribbon. Scale bar, 0.2 µm.

Further GluR receptor subunits at the rod bipolar cell axon terminal

Our laboratory has described the expression of the KA receptor subunit KA2 at the RB cell dyads of the rat retina (Brandstätteret al., 1997). Only one of the two members of the dyad expressedKA2 immunoreactivity. Brandstätter et al. (1997) also localizedthe KA receptor subunit GluR6/7 and the orphan receptor subunits $delta$ 1/2 to one member of the RB cell dyad. We applied the same KA2antiserum to the monkey; however, as reported elsewhere, thisantiserum showed a prominent cross-reactivity with some unknownantigen in these retinas and did not recognize the correct protein(Haverkamp et al., 2001). We studied the distribution of the KAreceptor subunit GluR5 in the monkey retina and observed synapticlabeling only in the OPL, with no labeling in the IPL (Haverkampet al., 2001). We also applied the GluR6/7 antiserum; however,once again this antiserum showed an unusual pattern of stainingand was not further analyzed here. However, we were able to observea reliable immunostaining of monkey and rabbit retinas for the $delta$ 1/2subunits.

Originally, the $delta$ subunits were named orphan receptors, because the recombinantly expressed protein lacks all channel activity(Araki et al., 1993; Lomeli et al., 1993). However, recently ithas been shown that the $delta$ subunits are clustered at the dendriticspines of cerebellar Purkinje cells (Landsend et al., 1997). Moreover,a mutation of the $delta$ 2 subunit in the Lurcher mouse results in anopening of channels even in the absence of glutamate (Zuo et al.,1997). All this suggests that the $delta$ subunits, together with anunknown subunit partner, form cation channels that are activatedby glutamate (Seeburg, 1997; Kohda et al., 2000).

Figure 4A shows the RB cell axon terminals in a section through the monkey retina that was double-labeled for PKC and forthe $delta$ 1/2 subunits. The $delta$ label is punctate, suggesting that, comparableto the cerebellum (Landsend et al., 1997; Bergersen et al., 2001),the $delta$ subunits are clustered in postsynaptic densities. In addition,many $delta$ clusters appear to be in close apposition to the RB cellaxon terminals (Fig. 4A, arrow) that have been shown in the ratretina by EM to represent an expression of the $delta$ 1/2 subunits atthe dyads (Brandstätter et al., 1997). It now needs to be clarified(1) which other GluR subunits are the partners of the $delta$ subunitsat the RB cell terminals and (2) which of the two postsynapticelements, AI or AII cells, express the $delta$ subunits.

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Figure 4. A, Confocal fluorescence micrograph of a vertical section through the inner part of the IPL of a macaque monkey retina that was double-labeled for PKC (green) and the $delta$ 1/2 subunit (red). Many $delta$ 1/2 immunoreactive puncta coincide with the RB axonal varicosities (arrow). B-D, Fluorescence micrograph of a section through the inner IPL of a macaque monkey retina that was double-labeled for $delta$ 1/2 (red) and PSD-95 (green). The superposition in D shows that the puncta are not in register. E, Confocal fluorescence micrograph of a vertical section through the inner IPL of a macaque monkey retina that was double-labeled for PKC (green) and for GRIP (red). Many GRIP-immunoreactive puncta coincide with RB cell axonal varicosities (arrows). F-H, Fluorescence micrograph of a section through the inner IPL of a macaque monkey retina that was double-labeled for GRIP (red) and PSD-95 (green). The superposition in H shows that the puncta are not in register. I-K, Fluorescence micrographs of a section through the inner IPL of a macaque monkey retina that was double-labeled for GRIP (red) and $delta$ 1/2 (green). The superposition in K shows that many puncta are in register. The circles indicate groups of puncta to facilitate comparison between the micrographs. Scale bars: A, E, 5 µm; B-D, F-K, 2.5 µm.

Because most of the antibodies against the AMPA receptor subunits, as well as the antibodies against the $delta$ 1/2 subunits, wereraised in rabbits, we could not perform a direct comparison bydouble-labeling experiments. However, as shown before, PSD-95appears to be aggregated together with the GuR2/3 and the GluR4subunits (Fig. 2). Therefore, the possible colocalization of the $delta$ 1/2 subunits with the AMPA receptor subunits was studied by double-labelingsections for $delta$ 1/2 and PSD-95 (Fig. 4B-D). Comparison of panelsB-D in Figure 4 shows that $delta$ 1/2 clusters and PSD-95 clusters arenot colocalized, suggesting that they are aggregated at differentpostsynaptic densities. Therefore, it appears unlikely that $delta$ 1/2subunits together with AMPA receptor subunits coassemble at theRB cell dyads. Close inspection of the labeled PSD-95 and $delta$ 1/2immunoreactive puncta in Figure 4 (encircled) shows that theyoften occur as close neighbors, suggesting that one such pairrepresents the expression by the two members of the dyad. ApparentlyPSD-95 and AMPA receptors are expressed by one postsynaptic memberof the dyad, whereas the $delta$ 1/2 subunits appear to be clusteredat the other member of thedyad.

Synapse-associated proteins at the RB cell dyad

In addition to PSD-95, which was found to be associated with AMPA receptors at the RB cell dyads, we localized another synapse-associatedprotein. GRIP has been described in other parts of the CNS tobe associated with glutamate receptors (Dong et al., 1997) andpossibly with GABA receptors (Dong et al., 1999).

A section through the lower part of the IPL of a macaque monkey retina that was double-labeled for PKC and GRIP is shown inFigure 4E. The GRIP label is punctate, suggesting it is aggregatedin postsynaptic densities as has been shown in other parts ofthe CNS (Dong et al., 1997, 1999; Wyszynski et al., 1998; Buretteet al., 2001). Many of the GRIP hot spots (Fig. 4E, arrows) areassociated with PKC immunoreactive axon terminals of RB cells,similar to the $delta$ 1/2 subunit (Fig. 4A) and the AMPA subunits (Fig.1H,J). We also double-labeled sections for the ribbon marker kinesinand for GRIP and observed a GRIP immunoreactive hot spot at thegreat majority of the ribbons (data not shown). Together, theseresults indicate that GRIP is aggregated in postsynaptic densitiesat the RB celldyads.

This raises the following question: is GRIP clustered in the same postsynaptic densities as PSD-95? A section through theinner IPL of a macaque monkey retina was double-labeled for GRIP(Fig. 4F) and for PSD-95 (Fig. 4G). Both GRIP and PSD-95 showa punctate immunofluorescence; however, the superposition of thepuncta (Fig. 4H) shows that they do not coincide, suggesting thatthey are clustered at different postsynaptic densities. Closeinspection of the groups of puncta that are encircled in Figure4, F-H, suggests that they often occur as neighbors in the twopostsynaptic members of the dyads. We also double-labeled sectionsfor GRIP and the $delta$ 1/2 subunits (Fig. 4I-K) and observed that themajority of $delta$ 1/2 immunoreactive puncta coincided with GRIP immunoreactiveclusters. However, the coincidence rate between GRIP and the $delta$ 1/2subunits is not as high as that observed for PSD-95 and AMPA subunits(Fig. 2F-K). There are some GRIP hot spots not associated with $delta$ 1/2 and vice versa, suggesting that GRIP is not involved onlywith the clustering of $delta$ 1/2subunits.

The analysis of the localization of the AMPA and $delta$ 1/2 subunits and of the clustering proteins PSD-95 and GRIP using lightmicroscopy represents an undertaking at the limits of the resolutionof light microscopy. However, such an analysis has the advantagethat many more dyads can be observed than by the usual approachof EM serial reconstructions of this complex synapse (Marc andLiu, 2000). On the basis of the results presented so far, we concludethat AMPA receptor subunits and PSD-95 are expressed togetherin one postsynaptic member of the dyad, whereas the $delta$ 1/2 subunitsand GRIP appear to be clustered in the other member of thedyad.

The postsynaptic partners at the RB cell dyad

AII cells express the AMPA receptor subunits
Next, we wanted to know which of the two postsynaptic elements at the RB cell dyads express AMPA receptors. Qin and Pourcho(1999a,b) have shown in the cat retina that AMPA receptors areexpressed by AII amacrine cells at the RB cell dyad. In both themonkey and the rabbit retina, AII amacrine cells are immunoreactivefor the calcium-binding protein calretinin (Wässle et al., 1995;Massey and Mills, 1999; Mills and Massey, 1999). A section througha macaque monkey retina that was double-labeled for calretininand GluR4 is shown in the low-power micrographs of Figure 5, Aand B. The typical bistratified morphology of the AII amacrinecells, with lobular dendrites in the outer IPL and distal dendritesin the inner IPL, is apparent in Figure 5A. GluR4 immunoreactivityis present throughout the IPL (Fig. 5B); hence AII cells may wellreceive input through GluR4 subunits both at their lobular anddistal dendrites. However, in the context of the present study,we focus on the RB input into the distal dendritic tree (Fig.5A,B, squares). Figure 5, C-E, shows a section through this regionat higher magnification. Close inspection shows that many GluR4immunoreactive puncta are in register with small varicositiesat which AII amacrine cell dendrites apparently receive inputfrom RB cell axon terminals (arrows). However, one might arguethat because of the close apposition of AI and AII processes atthe dyad it is impossible by light microscopy to decide whetherthe GluR4 hot spots are on the AI cell or the AII cell.

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Figure 5. Localization of GluR4 immunoreactive puncta on AII amacrine cell dendrites. Confocal fluorescence micrographs that were double-labeled for calretinin (CR) and the GluR4 subunit. A, Calretinin-labeled AII amacrine cells. B, GluR4-immunoreactive puncta of the same section as in A. The area indicated by the frame and the inner IPL are shown at higher magnification in C-E. C, The distal dendrites of AII amacrine cells form a dense network of processes in the inner IPL. D, Many GluR4-immunoreactive puncta are found in the same region. E, The superposition of C and D shows that many GluR4-immunoreactive puncta are in register with the small varicosities of AII cell dendrites (arrows). Scale bars: A, B, 10 µm; C-E, 5 µm.

Therefore, this result was corroborated by EM double-labeling experiments (Fig. 6). Secondary antibodies coupled to largegold particles of 12 nm diameter were applied to reveal the calretininimmunolabeling. As shown in Figure 6, A and B, only one of thetwo amacrine cell processes at the RB dyad was labeled, thus representingthe AII amacrine cell. Secondary antibodies coupled to small goldparticles of 6 nm were applied to reveal the GluR2/3 immunolabeling(Fig. 6A,B). The small gold particles are aggregated in the AIIamacrine cell processes, close to the synaptic ribbons (arrows).The postsynaptic areas are shown at higher magnification in Figure6, C and D, and the different sized gold particles can be discriminatedmore readily. A total of 18 double-labeled RB cell dyads werestudied. In 17 dyads, only one postsynaptic dendrite expressedcalretinin, and in only one dyad both postsynaptic dendrites werefound to be labeled. In 14 dyads, the expression of the GluR2/3subunit was restricted to the calretinin-labeled dendrite. Intwo dyads, GluR2/3 expression was observed in both the calretinin-labeledand -unlabeled dendrite. In one dyad, GluR2/3 label was observedin the calretinin-unlabeled dendrite. In the case of the dyadin which both postsynaptic dendrites expressed calretinin, bothwere immunoreactive for GluR2/3.

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Figure 6. A, B, Electron micrographs of sections through two RB cell dyads of a macaque monkey retina. The sections were double-immunolabeled for GluR2/3 and calretinin using postembedding immunocytochemistry and secondary antibodies that were coupled to gold particles (GluR2/3, 6 nm; calretinin, 12 nm). The insets indicated by the frames are shown at higher magnification in C and D. The arrows point to the GluR2/3 label. RB, Axon terminal; AII, calretinin-labeled AII amacrine cell dendrite. Arrowhead indicates the faintly stained synaptic ribbon. Scale bar: A, B, 0.2 µm.

AI cells express the $delta$ 1/2 subunits
Unfortunately, there is no selective marker available for the AI cells of the macaque monkey retina. However, in the rabbitretina it has been shown that uptake of 5-HT is a selective markerfor amacrine cell types that are members of the AI class at theRB cell dyads (Holmgren-Taylor, 1982; Sandell and Masland, 1986;Vaney, 1986; Sandell et al., 1989). We therefore applied triple-labelingto sections through the rabbit retina to localize the GluRs toAI or AII cells. The section in Figure 7A shows 5-HT labeled amacrinecell bodies (blue) and a dense plexus of dendrites in the lowerIPL, which is the characteristic signature of these cells (Sandelland Masland, 1986; Vaney, 1986; Sandell et al., 1989). This plexusreceives synapses from RB cells and provides GABAergic feedbacksynapses back onto the RB cell terminals. Many AII amacrine cells(green) are also labeled in Figure 7A. The $delta$ 1/2 immunoreactiveclusters are shown in red (Fig. 7A). The area indicated by theframe in Figure 7A is shown at higher magnification in Figure7, B-D. Figure 7B shows only the calretinin and the $delta$ 1/2 labeling.Only two of the red $delta$ 1/2 puncta appear yellow (arrows), indicatingthat they coincide with the calretinin-labeled dendrites. Figure7C shows only the 5-HT and $delta$ 1/2 labeling. The majority of thered puncta appear purple, because they coincide with the blue,5-HT labeled amacrine cell processes. The two red spots that wereyellow in Figure 7B are also purple in Figure 7C (arrows). Finally,in Figure 7D all three markers are shown. Once again, the twoconspicuous spots are indicated by small arrows and they appearwhite in this micrograph, because they express all three labels(red, green, and blue). Clearly, in this instance we cannot decidewhether these two $delta$ 1/2 hot spots are on the AII cells (green-labeled)or on the AI cells (blue-labeled). However, all other $delta$ 1/2 clustersappear to coincide with the AI cells.

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Figure 7. A, Confocal fluorescence micrograph of a vertical section through the inner part of a rabbit retina that was triple-labeled for calretinin (CR; green), serotonin (5-HT; blue), and the $delta$ 1/2 subunit (red). The inner IPL (frame) is shown at higher magnification in B-D. B, The green AII cell dendrites and the red $delta$ 1/2 hot spots are not in register. Only two dots (arrows) coincide with green dendrites. C, The blue, 5-HT-labeled dendrites of AI amacrine cells coincide with the red $delta$ 1/2 hot spots, and as a consequence they appear purple. D, All three markers superimposed. The two dots (arrows) appear white. E, Confocal fluorescence micrograph of a vertical section through the inner part of a rabbit retina that was triple-labeled for calretinin (CR, green), serotonin (5-HT, blue), and GluR4 subunit (red). The inner IPL (frame) is shown at higher magnification in F-H. F, The green AII cell dendrites and the red GluR4 puncta are often in register. G, The blue, 5-HT-labeled dendrites of AI cells are not in register with the GluR4 puncta. H, All three markers superimposed. The dot indicated by the arrow colocalizes both 5-HT and CR. Scale bars: A, E, 10 µm.

Next, we triple-labeled a section through a rabbit retina for calretinin, 5-HT, and the AMPA receptor subunit GluR4 (Fig.7E). One 5-HT-labeled AI amacrine cell body (blue) and severalcalretinin labeled AII cell bodies (green) can be seen in theINL. In the lower part of the IPL, processes of AI and AII cellsform a dense plexus at the position of RB axon terminals (Vaneyet al., 1991; Fletcher and Wässle, 1999). Numerous GluR4 immunoreactivepuncta are present throughout the IPL. The area indicated by theframe is shown at higher magnification in Figure 7, F-H. Onlythe calretinin (green)-labeled descending dendrites of AII amacrinecells and the GluR4 immunoreactive puncta (red) are shown in Figure7F. Close inspection shows that the puncta are aligned with thedescending processes and also show some overlap. It is possiblethat calretinin does not fill the whole cytoplasm of the dendritesand, therefore, the GluR4 immunoreactive puncta turn only partiallyyellow. However, in this and in other sections we observed thatGluR4 puncta were aligned along the AII cell dendrites. In Figure7G, the 5-HT-labeled dendrites of AI cells and the GluR4 hot spotsare shown in isolation. There is no close correspondence betweenthe blue label and the red dots that would be comparable to Figure7F. However, some of the GluR4 hot spots are in register with5-HT-labeled processes (Fig. 7G, arrow). Finally, all three markersare shown together in the micrograph in Figure 7H, confirmingthat the GluR4 subunit is closely associated with the AII amacrinecells (green) and not so much with the AI cells (blue). However,some puncta (arrow) are in register with both the AI and AIIprocesses.
We also performed double-labeling experiments for AI cells and GRIP (data not shown) and observed, comparable to the $delta$ 1/2subunits, a close correspondence between the AI varicosities andthe GRIP immunoreactive hot spots. AI cells often provide GABAergicfeedback synapses onto RB cells, in close vicinity to the dyads(Strettoi et al., 1992). It is, therefore, to be expected thatmarkers of these feedback synapses are found in close associationwith GRIP. We double-labeled sections for GRIP and bassoon (tomDieck et al., 1998). Bassoon has been shown to be expressed atinhibitory synapses that RB axon terminals receive from amacrinecells (Brandstätter et al., 1999). We observed a close association,but not a coincidence of the GRIP immunoreactive puncta with thebassoon immunoreactive puncta (data not shown). The same holdstrue for sections that are double-labeled for GRIP and GABA_Creceptors.
Taken together, these results suggest that AMPA receptors and PSD-95 are preferentially expressed at the contacts betweenRB cells and AII cells, whereas the $delta$ 1/2 and the GRIP clustersare in register with the AIcells.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The bipolar cell dyad

At the cone bipolar cell dyad, the light signal is transferred to a ganglion cell dendrite and an amacrine cell process, whichoften makes a reciprocal synapse back onto the bipolar cell (Dowlingand Boycott, 1966). At the rod bipolar cell dyad, two amacrinecells are the postsynaptic partners, the AI cell and the AII cell.Similar to the cone pathway, the AII cell is a "through conducting"neuron (Masland, 1986), whereas the AI cell provides a feedbacksynapse (Kolb and Famiglietti, 1974; Famiglietti and Kolb, 1975).Therefore, the two postsynaptic partners at bipolar cell dyadsrepresent different pathways and have different functions; oneis more involved with the transfer of the light signal, whereasthe other one plays a modulatory role (Bloomfield and Dacheux,2001).

Recent investigations of the transmitter receptors and postsynaptic density proteins expressed at the dyads have revealedmolecular differences between the two pathways. The first hintcame from the localization of the NMDA receptor NR2A subunit (Hartveitet al., 1994), which was expressed in only one partner of conebipolar cell dyads, most likely the ganglion cell dendrite. Later,it was shown that the metabotropic glutamate receptor mGluR7 isexpressed in only one postsynaptic member of the cone bipolarcell dyad and is not expressed postsynaptically at RB cells (Brandstätteret al., 1996). Similarly, mGluR2 and mGluR4 were restricted toone postsynaptic member of the dyad; however, they were associatedwith both cone and rod bipolar cells (Koulen et al., 1996). Kainatereceptors were also selectively expressed in only one member ofthe dyad, both in cone and rod bipolar cells (Brandstätter etal., 1997; Qin and Pourcho, 2001). AMPA receptors were expressedalso in only one postsynaptic dendrite, both in cone and rod bipolarcells (Qin and Pourcho, 1999a,b). In the case of the synapse-associatedproteins PSD-95 and SAP102, localization was also restricted toone postsynaptic dendrite of cone and rod bipolar cells (Koulenet al., 1998a,b). All of this suggests that the two pathways postsynapticto cone and rod bipolar cell dyads express different receptorsto glutamate and that this molecular dichotomy results in differentfunctional roles. The results also show that there is a differencebetween the cone bipolar cell and the rod bipolar cell pathwaysas the NMDA receptor subunits NR1, NR2A, NR2B, and mGluR7 arenot expressed at the RB cell dyads (Brandstätter et al., 1996;Fletcher et al., 2000).

In this study, we have presented further evidence for the role of the dyad as a synapse that initiates two functionally andmolecularly different pathways. The studies mentioned above analyzedthe dyads primarily by pre-embedding immunocytochemistry and electronmicroscopy. In such studies, one has to worry about the tissuepenetration of the antibodies and that only a few synapses canbe observed. Hence, one can never be sure whether the labelingof only one postsynaptic partner of the dyad is because of technicallimitations or whether it represents a real functional difference.In this study, we used confocal light microscopy and triple-labelingimmunocytochemistry, and thus we were able to observe many moresynapses and positively identify the postsynaptic partners. Thisanalysis showed convincingly not only that AI and AII cells expressdifferent sets of GluRs but also that different postsynaptic densityproteins are involved in clustering the receptors in the postsynapticdensities.

The AII cell pathway

We could show by labeling the RB cell synaptic ribbons for kinesin and by confocal light microscopy that the AMPA receptorsubunits GluR2/3 and GluR4, as well as PSD-95, are aggregatedin postsynaptic densities at every individual dyad. Additionallabeling of AII amacrine cells for calretinin demonstrated thatthese AMPA-PSD-95 clusters are expressed at the arboreal dendritesof AII amacrine cells. This result confirms and extends an EMstudy of the cat retina (Qin and Pourcho, 1999a,b) showing thatAII amacrine cells, at their contacts with RB cells, express theGluR2/3 and GluR4 subunits. Also in agreement with studies inthe cat retina (Qin and Pourcho, 1999a), we found no expressionof GluR1 at RB cell dyads (Fig. 1C,D). However, in contrast toBrandstätter et al. (1997, their Fig. 7A), we conclude that the $delta$ 1/2 subunits are not expressed by AII cells. Recent electrophysiologicalrecordings from AII amacrine cells in a slice preparation of therabbit retina (Zhou and Dacheux, 2001) showed that activationof NMDA receptors did not elicit a current response. Kainate-AMPAreceptor-mediated responses could be blocked by CNQX and GYKI52466,suggesting that they are mediated only by AMPAreceptors.

The AI cell pathway

As mentioned in Results, for several technical reasons we could not study the localization of the kainate receptor subunitsKA2 and GluR6/7 in the rabbit and macaque monkey retina. However,it has been shown before for the cat and rat retina that thesesubunits are expressed by only one postsynaptic member of thecone and rod bipolar cell dyad (Brandstätter et al., 1997; Qinand Pourcho, 2001). In this paper, by using confocal light microscopyand specific markers, we could show that the $delta$ 1/2 subunit is aggregatedat the RB cell dyads, most likely at their contacts with AI amacrinecells. We have also presented evidence that the synapse-associatedprotein GRIP is most likely aggregated at these AI cell contacts.Together, all of this evidence suggests a clear-cut moleculardifference between the AII contacts involving AMPA receptors andPSD-95 and the AI contacts involving the $delta$ 1/2 subunit and GRIP.We suggest that the subunits KA1/2, GluR6/7, and $delta$ 1/2 form heteromericchannels of the kainate type (Kohda et al., 2000) and that thesereceptors provide the signal transfer between RB cells and AIcells. However, because AI cells comprise several different types(Sandell and Masland, 1986; Sterling and Lampson, 1986; Vaneyet al., 1991), it is possible that kainate receptors with differentsubunit combinations are expressed by these different AI celltypes. This would create further diversity of the signal transferat the RB celldyads.

The glutamate receptors of AI amacrine cells have recently been studied by patch-clamp recordings from rat retina slices (Mengerand Wässle, 2000). It was found that non-NMDA receptors mediatethe responses to glutamate. A similar result has been reportedby Hartveit (1999). Although specific antagonists to distinguishAMPA and kainate receptors were not applied, it was noticed thatthe CNQX and NBQX, which usually block these receptors, reducedthe responses to only 64% of the controls. This suggests thata glutamate receptor with an unusual pharmacological profile isinvolved. On the basis of the present results, we suggest thatthis "unusual" receptor includes the $delta$ 1/2 subunits that so farhave escaped a pharmacological analysis (Wollmuth et al., 2000).

Signaling through AMPA and kainate receptors

It has been shown in both the nonmammalian and mammalian retina that the light signal from cone bipolar cells onto ganglioncells involves both AMPA and NMDA receptors (Mittman et al., 1990;Diamond and Copenhagen, 1993; Lukasiewicz et al., 1997; Cohen,2000). The AMPA receptors contribute fast EPSCs, whereas the NMDAreceptor-mediated EPSCs have slower rise and decay times. Thus,mainly the temporal characteristics of the signal transfer differs.However, there are also substantial pharmacological differencesbetween NMDA and AMPA receptors such as the voltage dependence,the Mg²⁺ block, and the Ca²⁺ permeability of NMDA receptors. Kainate receptors do not appearto be involved in the signal transfer from cone bipolar cellsonto ganglion cells (Lukasiewicz et al., 1997). However, becausekainate receptors are also present at the cone bipolar cell dyad(Brandstätter et al., 1997; Qin and Pourcho, 2001), they aremost likely expressed at the amacrine cell dendrites and not onthe ganglion cell dendrites (Shen and Slaughter, 2001). Only onestudy of the mammalian retina has so far pharmacologically dissectedcontributions of AMPA and kainate receptors to retinal signaling.DeVries (2000) studied the signal transfer from cones onto off-conebipolar cells in the ground squirrel and showed that b3 bipolarcells express kainate receptors, whereas b2 and b7 bipolar cellstransfer the light signal via AMPA receptors. The result of thispharmacological diversity is a more transient, short latency lightresponse in b2 and b7 bipolar cells and a more sustained, longerlatency light response in b3 bipolar cells. If the same differencewould also hold for the RB output synapse in the IPL, it wouldsuggest that the signal transfer into AII amacrine cells mediatedby AMPA receptor is "fast," whereas the signal transfer to AIcells is "slow." Such a difference in the temporal transfer characteristicswould be in agreement with the notion that AII amacrine cellsare through conducting neurons, whereas AI cells have a modulatoryrole (Masland, 1986).

  FOOTNOTES

Received July 10, 2001; revised Aug. 13, 2001; accepted Aug. 17, 2001.

This work was supported by the Deutsche Forschungsgemeinschaft (SFB 269/B4) and by a Fellowship of the A. V. Humboldt Foundationto K.K.G. We are grateful to Dr. B. Lee and Dr. P. Martin forproviding monkey eyes. We thank M. Dumbsky, W. Hofer, and G. S.Nam for excellent technical assistance; Dr. F. Priesnitz for hishelp with confocal microscopy; and I. Odenthal for typing thismanuscript.
Correspondence should be addressed to Dr. Heinz Wässle, Max-Planck-Institut für Hirnforschung, Abteilung Neuroanatomie,Deutschordenstrasse 46, D-60528 Frankfurt/Main, Germany. E-mail:Waessle{at}mpih-frankfurt.mpg.de.

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RESULTS
DISCUSSION
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