Cholinergic Septal Afferent Terminals Preferentially Contact Neuropeptide Y-Containing Interneurons Compared to Parvalbumin-Containing Interneurons in the Rat Dentate Gyrus

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The Journal of Neuroscience, November 15, 1999, 19(22):10140-10152

Cholinergic Septal Afferent Terminals Preferentially Contact Neuropeptide Y-Containing Interneurons Compared to Parvalbumin-Containing Interneurons in the Rat Dentate Gyrus
Karen D. Dougherty² and Teresa A. Milner¹
¹ Department of Neurology and Neuroscience, Weill Medical College of Cornell University, New York, New York 10021, and ² Department of Neuroscience and Cell Biology, University of Medicine and Dentistry, Robert Wood Johnson Medical School, Piscataway, New Jersey 08854

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Septal cholinergic neurons may affect hippocampal memory encoding and retrieval by differentially targeting parvalbumin (PARV)-containingbasket cells and neuropeptide Y (NPY) interneurons. Thus, thecellular associations of cholinergic efferents, identified bythe low-affinity, p75 neurotrophin receptor (p75^NTR), with interneurons containing either PARV or NPY in the hilusof the rat dentate gyrus were examined in single sections usingdual labeling immunoelectron microscopy. Most profiles immunoreactive(IR) for PARV and NPY were perikaryal and dendritic and foundwithin the infragranular and central hilar regions, respectively,whereas most profiles with p75^NTR-labeling were unmyelinated axons and axon terminals. AlthoughPARV-labeled profiles were more numerous, p75^NTR-labeled axons and terminals contacted few PARV-IR profiles comparedto NPY-labeled profiles (2% of 561 for PARV vs 12% of 433 forNPY). Moreover, structures targeted by p75^NTR-IR axon terminals varied depending on the presence of PARV orNPY immunoreactivity. p75^NTR-IR terminals primarily contacted PARV-IR dendrites (87%) comparedto somata (13%); however, they contacted more NPY-IR somata (57%)than dendrites (43%). p75^NTR-labeled terminals formed exclusively symmetric (inhibitory-type)synapses with PARV-IR somata and dendrites; however, they formedmostly symmetric but also asymmetric (excitatory-type) synapseswith NPY-IR somata and dendrites. These results suggest that septalcholinergic efferents in the dentate gyrus: (1) preferentiallyinnervate NPY-containing interneurons compared to PARV-containingbasket cells; and (2) may provide a more powerful (i.e., somaticcontacts), yet functionally diverse (i.e., asymmetric and symmetricsynapses), modulation of NPY-containing interneurons. Moreover,they provide evidence that neurochemical subsets of hippocampalinterneurons can be distinguished by afferentinput.

Key words: neurotrophin receptors; septohippocampal pathway; nerve growth factor; electron microscopy; GABAergic nonprincipal cells; neuropeptide Y

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Neurons in the medial septum-diagonal band complex provide a major subcortical input to the hippocampal formation (HF) (Swansonand Cowan, 1979; Senut et al., 1989). Septohippocampal neuronsinclude cholinergic and noncholinergic populations, the lattermostly containing GABA (Köhler et al., 1984; Amaral and Kurz,1985; Freund and Antal, 1988). Cholinergic septohippocampal neuronsare believed to influence memory and attentional processing (Chibaet al., 1995; Baxter et al., 1997); moreover, loss of these neuronsis associated with age- and Alzheimer's-related memory declines(Muir, 1997).

Septal afferents are topographically arranged within the HF with many terminating in the hilus of the dentate gyrus (Swansonand Cowan, 1979; Milner et al., 1983). Although they contact principaland nonprincipal (GABAergic interneurons) hippocampal cells (Frotscher,1991; Dougherty and Milner, 1999), GABAergic and cholinergic septalaxons have different patterns of connectivity. GABAergic septohippocampalterminals preferentially contact GABAergic basket interneuronsand almost exclusively form symmetric synapses (Freund and Antal,1988). Many of these basket interneurons contain the calcium-bindingprotein parvalbumin (PARV) and are primarily in the infragranularhilus (Kosaka et al., 1987; Freund, 1989; Deller et al., 1994;Freund and Buzsáki, 1996). In contrast, cholinergic septohippocampalterminals are thought to form both asymmetric and symmetric synapsesindiscriminately with granule cells and hilar GABAergic interneurons(Clarke, 1985; Frotscher, 1991).

However, we recently reexamined the ultrastructural distribution of cholinergic septal terminals in the dentate gyrus usingp75 neurotrophin receptor (p75^NTR) immunoreactivity, which is not detected in GABAergic septalneurons (Koliatsos et al., 1994). This study revealed that p75^NTR-immunoreactive (IR) axons and axon terminals were more numerousin the central hilus, suggesting that they preferentially contactedinterneurons rather than granule cells (Dougherty and Milner,1999). Previous studies support this notion and further suggestthat GABAergic interneurons targeted by septal cholinergic terminalsmay contain neuropeptide Y (NPY). First, septal afferents, morphologicallysimilar to cholinergic terminals, form numerous contacts on hilarNPY-containing interneurons (Milner and Veznedaroglu, 1993). Second,cholinergic septal deafferentation using 192 IgG-saporin leadsto rapid and selective decreases in the number of NPY-containinghilar interneurons (Milner et al., 1997). This NPY-labeled interneuronloss is restricted to a subset located primarily in the centralhilus and distinct from infragranular GABAergic basket cells (Milneret al., 1997, 1999). However, whether septal cholinergic neuronspreferentially contact subpopulations of GABAergic interneuronsin the dentate gyrus remains to bedemonstrated.

Understanding the targeting specificity of septal cholinergic afferents with subpopulations of GABAergic interneurons couldhave important implications for hippocampal function. In particular,growing evidence indicates that functionally and morphologicallydistinct interneuron subtypes might modulate selective types ofhippocampal-dependent memory processes (Han et al., 1993; Halasyand Somogyi, 1993; Klapstein and Colmers, 1997; Sik et al., 1997;Paulsen and Moser, 1998). Thus, the present study sought to determinewhether septal cholinergic afferent terminals differentially innervatesubpopulations of GABAergic interneurons containing NPY or PARVin the dentate gyrus. For this, the proportion of cholinergicaxon terminals (identified with p75^NTR immunoreactivity) that contacted hilar NPY- or PARV-IR perikaryaand dendrites was compared using electronmicroscopy.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Section preparation. Nine naive male Sprague Dawley rats (250-300 gm; Taconic, Germantown, NY) were used in these studies.All methods were approved by the Weill Medical College of CornellUniversity Institutional Animal Care and Use Committee and conformto National Institutes of Health guidelines. Rats were anesthetizedwith Nembutal (150 mg/kg, i.p.), and their brains were fixed byascending aortic arch perfusion sequentially with solutions of:(1) 10-15 ml of normal saline (0.9%) containing 1000 U/ml of heparin,(2) 50 ml of 3.75% acrolein (Polysciences, Warrington, PA) and2% paraformaldehyde in 0.1 M phosphate buffer (PB; pH 7.4), and(3) 200 ml of 2% paraformaldehyde in PB. For the immunogold-silverprocedure, all rats were injected with the zinc chelator DEDTC(1 mg/kg, i.p.) 15 min before perfusion to reduce nonspecificsilver labeling of mossy fibers (Milner and Veznedaroglu, 1993).The region of the forebrain containing the HF was removed, cutinto a 5-mm-thick coronal block and placed in the latter fixative(30 min). The brains then were sectioned (40-µm-thick) on a vibratingmicrotome (Vibratome) and collected in PB. Before immunocytochemicalprocessing, sections were placed into 1% sodium borohydride inPB (30min).

Antibodies. For immunohistochemical localization of the p75^NTR, two antibodies were used. In a previous investigation, we foundthat both of these antibodies labeled the same cellular profileswith the same subcellular distribution (Dougherty and Milner,1999). Specificity of both antibodies has been tested previously(Chandler et al., 1984; Dobrowsky et al., 1994). The polyclonalantibody raised in rabbit (Promega, Madison, WI), which recognizesthe cytoplasmic domain of the p75^NTR, was used in double-labeling experiments with antibodies forPARV. The monoclonal antibody derived from mouse 192 IgG, whichrecognizes the extracellular domain of the p75^NTR (Boehringer Mannheim, Indianapolis, IN) was used in double-labelingexperiments with antiserum for NPY. A polyclonal antiserum raisedin rabbits against NPY (Peninsula, Belmont, CA) and a monoclonalantibody raised in mice to PARV (Sigma, St. Louis, MO) (both diluted1:2000) have been previously tested for specificity to their respectivepeptides, using both preadsorption and immunodot blot techniques(Sloviter and Nilavier, 1987; Milner and Veznedaroglu, 1992).

Dual immunocytochemical labeling. To reduce variability attributable to differences in fixation and solutions between thedual-labeling conditions, tissue collected from each rat was labeledusing both conditions on the same day. For dual immunocytochemicallocalization of p75^NTR and PARV or NPY, prepared sections through the HF were processedby using a combined immunoperoxidase and immunogold-silver labelingtechnique (Chan et al., 1990). Sections were incubated for 48hr at 4°C in a 0.1% bovine serum albumin (BSA) and a Tris-bufferedsaline (TBS, pH = 7.6) solution containing either: (1) rabbitpolyclonal antiserum for p75^NTR at 1:2000 dilution and mouse monoclonal antibody for PARV at1:1000 dilution, or (2) mouse monoclonal antibody for p75^NTR at 1:300 dilution and rabbit polyclonal antiserum for NPY at1:2000 dilution. After incubation with these primary antisera,sections were dually labeled for either of the two antibody combinationsusing immunoperoxidase followed by immunogold-silverdetection.

For immunoperoxidase labeling, sections were incubated in either biotinylated donkey anti-rabbit (for detection of p75^NTR immunoreactivity in combination with PARV labeling) or rat anti-mouseIgG (for detection of p75^NTR immunoreactivity in combination with NPY labeling) (Vector Laboratories,Burlingame, CA; 1:400 in 0.1% BSA-TBS) for 30 min. After rinseswith TBS, sections were incubated in avidin-biotin-peroxidasecomplex (Vectastain Elite kit; Vector Laboratories; 1:100 in TBS)for 30 min. Bound peroxidase was visualized by 6 min incubationin 0.022% 3,3'-diaminobenzidine (DAB; Aldrich, Milwaukee, WI)and 0.003% hydrogen peroxide inTBS.

For immunogold-silver labeling, sections were rinsed in 0.01 M PBS, pH 7.4, blocked in 0.8% BSA and 0.1% gelatin in PBS for10 min, then incubated in either goat anti-mouse (for detectionof PARV immunoreactivity) or goat anti-rabbit (for detection ofNPY immunoreactivity) IgG conjugated to 1 nm gold particles (AuroProbe;Amersham, Arlington Heights, IL; 1:50 in BSA-gelatin blockingsolution) for 2 hr. Sections were rinsed in PBS and post-fixedin 2% glutaraldehyde in PBS for 10 min. To obtain optimal visualizationof immunogold labeling, gold particles bound to the sections weresilver-enhanced for 6-7 min (IntenSE kit;Amersham).

For electron microscopy, labeled sections were fixed for 1 hr in 2% osmium tetroxide in 0.1 M PB and embedded in EMBed (ElectronMicroscopy Sciences, Fort Washington, PA) between two sheets ofAclar plastic as described previously (Milner and Veznedaroglu,1992). Sections through the dentate gyrus were mounted onto EMBedblocks, and ultrathin sections (70-nm-thick) from the tissue-plasticinterface of each section were cut with a diamond knife, collectedon 400 mesh copper grids, and counterstained with uranyl acetateand Reynolds lead citrate. Final preparations were examined witha Philips 201 electron microscope. Final illustrations were generatedfrom scanned photographic prints with a Power Macintosh 8500/120(Apple Computer, Cupertino, CA) using Adobe Photoshop 4.0 (AdobeSystems, Mountain View, CA) and Quark X-Press 3.32 (Quark, Denver,CO).

Electron microscopic analysis. Electron microscopic analysis of dual immunocytochemical labeling was conducted on those sixrats in which ultrathin sections collected from the dentate gyrusdisplayed optimal morphological preservation and robust immunolabelingof the p75^NTR and either PARV or NPY. The hippocampal nomenclature used inthis study is that reviewed in Patton and McNaughton (1995). Theterm "infragranular hilus" denotes that region of the hilus ~55µm below the granule celllayer.

Ultrastructural nomenclature was in agreement with Peters et al. (1991). Neuronal perikarya were identified by the presenceof a nucleus. Dendrites contained endoplasmic reticulum, wereusually postsynaptic to axon terminals, and ranged from 0.5-4.5µm in diameter. Axons were defined as those profiles containingfilaments but few synaptic vesicles and having a cross-sectionaldiameter of 0.1-0.2 µm. Axon terminals were defined as those profileswith a cross-sectional diameter of $>=$ 0.3 µm in which small synapticvesicles could clearly be seen. Those immunoreactive profilesthat could not be identified because of distorted or compromisedmorphology were categorized as "undefined." Asymmetric synapsescontained thick postsynaptic densities, whereas symmetric synapseshad thin postsynaptic densities. Appositions were defined as thosecontacts between profiles in which no interposing glial processeswere found but which lacked any recognizable synaptic specializations.A profile was defined as immunogold-silver-labeled when two ormore particles were seen in large profiles or a single particlein small profiles, such as small unmyelinated axons and dendriticspines that could be traced in serial sections. Immunoperoxidase-labeledprofiles were identified as those containing denseprecipitate.

A total of 10 coronal vibratome sections were examined in this study. The final quantitative analysis is based on data obtainedfrom two blocks of tissue from each of three rats. For each laminaof the dentate gyrus, three grid squares were analyzed (with totalarea of 9075 µm²). Four laminae were examined [central hilus (CNH), infragranularhilus (IGH), granule cell layer (GCL), and inner molecular layer(IML)] for a total of 36,300 µm² of tissue analyzed per block of tissue, for each dual labelingcondition. Only fields adjacent to the plastic-tissue interfacewere selected. For this, all immunogold-silver labeled profileswere counted, categorized (e.g., perikarya, dendrites, axons andterminals, glia) and described in terms of their laminar location.For each block of tissue examined, the total number of immunogold-silver-labeledprofiles was determined, from which the percentage of those ineach profile category and each lamina contacted by p75^NTR-labeled axons and axon terminals was calculated. The data areexpressed as either mean percent ± SEM or percentage of totalobserved. The types of contact relationships were identified andclassified as defined above. $chi$ ² analysis and factorial ANOVAs were used to compare the data obtainedfrom PARV- and NPY-immunolabeled tissuesections.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Light microscopic examination of p75^NTR-, PARV-, and NPY-IR

In agreement with previous reports (Pioro and Cuello, 1990; Dougherty and Milner, 1999), p75^NTR-IR was found in fine varicose processes and puncta throughoutthe dentate gyrus. Dense p75^NTR-IR was clustered in the supragranular and infragranular regions,whereas diffuse p75^NTR-IR was observed throughout the remaining dentate laminae (Fig.1A). Distribution patterns of immunocytochemical labeling of PARVand NPY in neuronal cell bodies and fibers also were similar tothose previously reported (Fukuda et al., 1996; Milner et al.,1997). Most PARV-IR neuronal perikarya and dendrites were locatedin the infragranular region of the hilus (Fig. 1B). Occasionally,PARV-IR perikarya and dendrites were seen in the central hilusand molecular layer (Fig. 1B). NPY-IR neurons and dendritic processeswere seen primarily in the hilus (Fig. 1C). Although a few NPY-labeledperikarya were observed in the infragranular region of the hilus,the majority were in the central portion.

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Figure 1. p75^NTR-IR processes have an overlapping distribution with both PARV- and NPY-containing neuronal profiles in the dentate gyrus. A, p75^NTR-labeled puncta and fine varicose fibers are densest in supragranular and infragranular cell layer (GCL) (arrows) and more diffuse in the central portions of the hilus (HIL) (arrowhead) and molecular layer (ML). B, Most PARV-IR somata and dendrites are in the infragranular region of the hilus (arrows), whereas PARV-IR fibers and puncta are dense in the granule cell layer. Scattered processes and somata with PARV immunoreactivity are seen within the molecular layer and central hilus. C, Numerous NPY-IR perikarya and dendrites are located within the central regions of the hilus (arrows). NPY-IR fibers are also visible in the hilus (arrowhead) Scale bars: A-C, 400 µm.

Electron microscopy

p75^NTR immunoreactivity is primarily presynaptic
In agreement with our previous reports (Dougherty and Milner, 1998, 1999), the majority of p75^NTR immunoreactivity was found in axons and axon terminals (Figs.2-4). Less frequently, glial processes, dendritic shafts, anddendritic spines contained p75^NTR immunolabeling (data not shown). In the present investigation,the distribution and morphological characteristics of the p75^NTR-IR axonal profiles within the dentate gyrus were identical wheneither the monoclonal antibody 192 IgG or the polyclonal antiserumraised in rabbit for the p75^NTR was used. p75^NTR-IR profiles were most numerous within the inner molecular layer,infragranular hilus, and central hilus. p75^NTR immunoreactivity was found predominantly within small (0.1-0.3µm in diameter) unmyelinated axons and small to medium (0.3-0.8µm diameter) axon terminal profiles (Fig. 2). p75^NTR-IR axon terminals contained many small synaptic vesicles andmitochondria, but no dense core vesicles.

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Figure 2. The majority of p75^NTR-IR axons and axon terminals do not contact PARV-labeled perikarya and dendrites. A, In the infragranular layer, a p75^NTR-IR axon terminal (p75-T) is near but does not contact a PARV-IR soma (PARV-SO), which contains many gold-silver particles (arrowheads) within its cytoplasm. Numerous unlabeled axon terminals (UT) synapse on the PARV-labeled soma (arrows). B, A p75^NTR-IR axon (p75-Ax) is in the vicinity of a PARV immunogold-silver-labeled dendrite (PARV-D) in the hilus. Many unlabeled axon terminals (UT) form asymmetric synapses (curved arrows) with this dendrite. SSV, Small synaptic vesicles. Scale bars: A, B, 0.5 µm.

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Figure 3. Occasionally, p75^NTR-IR axon terminals contact PARV-labeled dendrites. A, In the infragranular hilus, a p75^NTR-IR axon terminal (p75-T) forms a symmetric synapse (curved arrow) with a large PARV-IR dendrite (PARV-D). An unlabeled axon terminal (UT) forms a symmetric synapse (curved open arrow) with the same dendrite. B, In the infragranular hilus, a large p75^NTR-IR axon terminal (p75-T) contacts (curved arrow) a small, PARV-IR dendrite (PARV-D). C, In the infragranular hilus, a large p75^NTR-IR axon terminal (p75-T) forms a symmetric synapse (curved arrow) with a large PARV-IR dendrite (PARV-D). Scale bars: A, 0.65 µm; B, C, 0.5 µm.

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Figure 4. Rarely, p75^NTR-labeled terminals are associated with PARV-containing terminals. A, A somata in the granule cell layer is contacted (curved arrow and arrowhead, respectively) by both a PARV-IR axon terminal (PARV-T) and a p75^NTR-IR axon terminal (p75-T). B, In the supragranular portions of the molecular layer, a p75^NTR-IR axon terminal (p75-T) abuts (curved arrow) a PARV-IR axon terminal (PARV-T) labeled with gold-silver particles (arrowheads). C, An axon terminal in the supragranular layer contains both p75^NTR-IR and PARV-IR gold-silver particles (arrowheads). A single-labeled, p75^NTR-IR axon terminal (p75-T) nearby forms a symmetric synapse (curved arrow) with an unlabeled dendrite. Scale bars: A, 1.0 µm; B, C, 0.5 µm.

PARV immunoreactivity is in basket cells
PARV immunogold-silver-labeled neuronal profiles observed in the present investigation closely resembled those described inprevious reports in which immunoperoxidase labeling was used (Ribaket al., 1990; Deller et al., 1994). Briefly, PARV-IR neuronalprofiles had the morphological characteristics of basket cells:(1) small (6-12 µm in diameter) and aspinous perikarya, (2) nucleiwith Nissl bodies, intranuclear rods, and nuclear infoldings (datanot shown), (3) aspinous dendrites that received numerous contactsfrom terminals forming both asymmetric and symmetric synapses(Figs. 2B, 3), and (4) axon terminals that form symmetric synapseswith granule cell bodies, dendrites, and axon initial segments(data notshown).
In agreement with the pattern of PARV-IR observed at the light microscopic level, the types of PARV-IR profiles observed (n= 581) varied significantly between the lamina. Most PARV-labeledsomal profiles (n = 43) occurred within the infragranular hilusand the central hilus (58 and 18%, respectively). PARV-labeleddendritic profiles (n = 382) also occurred more frequently inthe infragranular and central hilus (34% each) than in the granulecell layer and inner molecular layer, whereas PARV-labeled axonterminal profiles (n = 156) were found primarily in the granulecell layer (59%).

NPY immunoreactivity is in morphologically distinct subtypes of interneurons
NPY-IR neuronal profiles in the current experiment were similar to those described in previous investigations using immunoperoxidaselabeling (Deller and Leranth, 1990; Milner and Veznedaroglu, 1992,1993; Milner et al., 1997, 1999). NPY-labeled somal profiles wereeither elongated or round and ranged from small (6-12 µm diameter)to medium (12-18 µm in diameter) (Figs. 5, 6; see Fig. 8). NPY-labeledsomata contained immunogold-silver particles that were commonlyobserved near rough endoplasmic reticulum or within Golgi complexsaccules and multivesicular bodies (Fig. 5A,B). At least two morphologicallydistinct types of NPY-labeled somata were observed: (1) thosecontacted by few axons and axon terminals and covered by numerousglial processes (Fig. 5) and (2) those contacted by several axonsand axon terminals with very little glial coverage of their plasmalemmalsurface (Fig. 6). NPY-IR dendritic profiles ranged from 1.5-5µm in diameter and primarily contained mitochondria, smooth endoplasmicreticulum, and microtubules (Figs. 7, 8B). NPY-IR perikarya anddendrites often were contacted by many axon terminals (Fig. 7).NPY-labeled axon terminals were predominantly small (<0.8 µm indiameter) and contained many small synaptic vesicles and few mitochondria(data not shown).

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Figure 5. p75^NTR-labeled terminals commonly contact NPY-labeled perikarya with sparse inputs. A, In the hilus, a p75^NTR-IR axon terminal (p75-T) forms a symmetric synapse (curved arrow) with an NPY-IR soma (NPY-SO). This soma is contacted by few axon terminals, and its plasmalemmal surface is covered by glial profiles (asterisk). B, In the infragranular hilus, a p75^NTR-IR axon terminal (p75-T) forms an asymmetric synapse (curved arrow) with an NPY-IR soma (NPY-SO) that contains gold-silver particles (arrowheads). Glial processes (asterisk) are apposed to adjacent regions of the plasmalemma. C, In the central hilus, much of the plasmalemmal surface of an NPY-IR soma is apposed by glial processes (asterisk). A p75^NTR-IR axon terminal forms a symmetric synapse (curved arrow) with this perikaryon, whereas a nearby unlabeled axon terminal (UT) forms an asymmetric synapse (open curved arrow). Mvb, Multivesicular body; ER, endoplasmic reticulum. Scale bars: A, B, 0.5 µm; C, 0.65 µm.

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Figure 6. NPY-labeled perikarya with heavy inputs also commonly receive contacts from p75^NTR-labeled terminals. A, In the infragranular hilus, a p75^NTR-IR axon terminal (p75-T) establishes an asymmetric synapse (curved arrow) with an NPY-IR soma (NPY-SO). Many unlabeled axon terminals (UT) also synapse on this perikaryon (open curved arrows). B, Higher magnification view of a portion of an NPY-labeled perikaryon contacted by a p75^NTR-IR axon terminal (p75-T) and numerous unlabeled terminals (UT) (solid curved arrows and open curved arrows, respectively). Scale bars: A, 1.0 µm; B, 0.5 µm.

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Figure 7. p75^NTR-IR axon terminals commonly contact NPY-IR dendrites. A, A p75^NTR-IR axon terminal (p75-T) contacts (curved arrow) a large NPY-IR dendrite (NPY-D) in the hilus. Several unlabeled terminals (UT) also contact (open curved arrows) this dendrite. B, A large NPY-IR dendrite (NPY-D) in the infragranular hilus is contacted by a p75^NTR-IR axon terminal (p75-T) that forms a symmetric synapse (curved arrow). The NPY-labeled dendrite contains many gold-silver particles located at the plasmalemma (arrowheads) and is also contacted (open curved arrows) by an unlabeled terminal (UT) and an unlabeled mossy fiber terminal (mT). Scale bars: A, 1.0 µm; B, 0.5 µm.

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Figure 8. Often, more than one p75^NTR-IR terminal contacts an NPY-labeled perikaryon or dendrite. A, Two p75^NTR-labeled terminals (p75-T) form symmetric synapses (curved arrows) with the same NPY-containing soma (NPY-SO). This soma received few contacts from other terminals. B,. A large NPY-labeled dendrite is contacted (curved arrows) by two p75^NTR-IR terminals (p75-T). An unlabeled terminal (UT) also contacts (open arrow) the same dendrite as well as a neighboring NPY-IR soma. Scale bars, 0.5 µm.

Quantitative analysis of the DG revealed that the majority of NPY-IR profiles observed (n = 433) were located in the infragranularhilus (n = 135) and central hilus (n = 148). The majority of NPY-labeledprofiles in these regions comprised somata (n = 45) and dendrites(n = 178). Few NPY-containing terminals were seen (n = 58). NumerousNPY-labeled terminals were found in the outer molecular layer;however this region was not included in the quantitative analysisbecause few p75^NTR-IR profiles are found here (Dougherty and Milner, 1999). Significantlyfewer NPY-IR labeled profiles were found in the inner molecularlayer and granule cell layer (n = 94 and 56,respectively).

p75^NTR-IR axon terminal associations with NPY-IR and PARV-IR profiles
The relative frequency of immunogold-silver-labeled profiles observed in tissue labeled for PARV or NPY was not significantlydifferent (PARV, 116 profiles per section; NPY, 108 profiles persection). Despite nearly equal densities of immunogold-silverlabeling in each of these conditions, a significantly greaterproportion of NPY-IR profiles received contacts from p75^NTR-IR axon terminal profiles than did PARV-IR profiles ( $chi$ ² = 8.25; df = 3; p < 0.03). Of all NPY-IR profiles observed, 12%(n = 51) were contacted by one or more p75^NTR-IR axon terminal profiles. In contrast, only 2% (n = 12) of allPARV-IR profiles observed received suchcontacts.
Instances in which p75^NTR-IR axon terminals synapsed with NPY-IR perikarya and dendrites (n = 51) occurred primarily in the infragranularand central hilar regions (n = 21 and 23, respectively). Thesesynapses were predominantly symmetric (86%), but some were asymmetric(14%). p75^NTR-IR terminals synapsed more frequently with NPY-IR somata (57%)than with NPY-IR dendrites (43%) (Table 1, Figs. 5A,B, 6-8). SomeNPY-IR somata (n = 3) and dendrites (n = 2) were contacted bymore than one p75^NTR-IR axon terminal (Fig. 5B), which was never seen for PARV-IRprofiles. Moreover, NPY-IR somata that received contacts fromp75^NTR-IR axon terminals fell into both morphological subtypes (i.e.,those having have either very little or abundant axon terminalcoverage on the plasmalemmal surface) (Figs. 5A,B, 6, 7).


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Table 1. Relation of p75^NTR-IR axon terminals to PARV- and NPY-IR profiles

Target type tended to be dependent on peptide label. For instance, associations between p75^NTR-IR and PARV-IR profiles tended to be axodendritic rather thanaxosomatic. For associations between p75^NTR-IR and NPY-IR profiles, the reverse was true: the majority ofsynapses formed were axosomatic and fewer were axodendritic (Table1). Moreover, synaptic associations between p75^NTR-IR terminals and PARV-IR perikarya and dendrites were exclusivelysymmetric, whereas synaptic associations between p75^NTR-IR terminals and NPY-IR perikarya and dendrites were predominantlysymmetric, but also asymmetric (Table 1).
Unlike NPY-labeled profiles, which were almost exclusively perikarya and dendrites in the regions analyzed, a number of PARV-IRprofiles were axon terminals. Rarely, (n = 1) a p75^NTR-IR axon terminal and a PARV-IR axon terminal contacted the sameperikaryon (Fig. 4A). Equally rare was the identification of axoaxoniccontacts between a p75^NTR-IR axon terminal and a PARV-IR axon terminal (Fig. 4B). Moreover,a few axon terminal profiles (n = 4) contained immunoreactionproduct for both p75^NTR- and PARV-IR (Fig. 4C).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

These results suggest that septal cholinergic afferents to the dentate gyrus: (1) preferentially innervate NPY-containinginterneurons compared to those labeled with PARV and (2) may providea more powerful (i.e., somatic innervation), yet functionallydiverse (i.e., asymmetric and symmetric synapses) modulation ofNPY-containing interneurons. Moreover, they provide evidence thatneurochemical subsets of hippocampal interneurons can be distinguishedby afferentinput.

Cholinergic septal afferent terminals form more contacts with NPY-IR neurons than PARV-IR neurons

In the present investigation, p75^NTR-IR axon terminals, presumably arising from cholinergic neurons in the septal complex (Doughertyand Milner, 1999), contacted a significantly greater proportionof NPY-IR profiles than PARV-IR profiles. Moreover, some NPY-IRtargets were contacted by two or more p75^NTR-IR axon terminals. According to their location and morphology,the majority of NPY-IR cells likely correspond to hilar perforantpath-associated (HIPP) cells (Han et al., 1993; Halasy and Somogyi,1993; Freund and Buzsáki, 1996; Sik et al., 1997). The axon terminalsof these cells, many of which also contain somatostatin, contactthe dendrites of granule cells, overlapping with the terminationzones of glutamatergic entorhinal afferent fibers (Deller andLeranth, 1990). These cells therefore are ideally situated toprovide spatial control of the ability of granule cell dendritesto support backpropagation and may be instrumental regulatorsof synaptic plasticity by modulating excitatory inputs to granulecells (Klapstein and Colmers, 1997; Paulsen and Moser, 1998).Conversely, PARV-IR neurons correspond to perisomatic inhibitoryinterneurons or basket cells, which contact granule cells andmediate both feedback and feedforward inhibition (Ribak et al.,1990; Han et al., 1993; Halasy and Somogyi, 1993; Fukuda et al.,1996).

Several different, but not mutually exclusive, mechanisms may account for selective targeting of NPY-IR structures by cholinergicaxon terminals. For example, cholinergic neurons in the adultrat septal complex are critically dependent on neurotrophins derivedfrom target structures for their survival. Recent reports suggestthat subpopulations of hippocampal interneurons produce uniquecombinations of neurotrophins (Pascual et al., 1999). Some cholinergicaxons may possibly target those structures that produce the necessaryneurotrophic combination. The large majority of both PARV-IR basketcells and NPY-IR interneurons in the dentate gyrus contain nervegrowth factor (NGF) mRNA and thus likely produce NGF; however,neurotrophin-3 (NT-3) is found within most NPY-IR interneuronsin the dentate gyrus, but only a small subset of PARV-IR interneurons(Pascual et al., 1999). The possibility that adult septal cholinergicaxons in the dentate gyrus are attracted toward and preferentiallysynapse with cells that produce both NGF and NT-3 may underliethe current findings. Moreover, hippocampal interneurons may alsodepend on neurotrophic support for survival (Ha et al., 1998),and recent reports (Cho et al., 1998; Milner et al., 1999) suggestthat they may derive a portion of this (especially NGF) from theirseptal cholinergicassociations.

Cholinergic septal afferents preferentially contact NPY-IR somata

Most associations between septal cholinergic afferents and NPY-IR neurons were axosomatic. In contrast, the majority of contactsbetween p75^NTR and PARV profiles were axodendritic. Perikaryal contacts mayexert a more rapid and potent effect on the cell than do dendriticinputs (Spruston et al., 1994; Milner et al., 1999). Moreover,somatic synapses regulate action potential firing whereas dendriticsynapses influence efficacy of specific types of afferent innervation(Paulsen and Moser, 1998). This differential pattern of connectivity,combined with the greater overall innervation of NPY-IR profilescompared to PARV-IR profiles, suggests that activation of septohippocampalcholinergic fibers is heavily weighted toward influencing NPY-IRrather than PARV-IRinterneurons.

p75^NTR-IR axon terminals formed synapses with both classes of NPY-IR somata: (1) those with sparse associations from axons andaxon terminals and a high degree of plasmalemmal astrocytic coverageand (2) those with dense associations from many axons and axonterminals and concomitantly less astrocytic coverage. These observationsadd to the growing body of evidence that functional and/or morphologicallydistinct subgroups of interneurons exist in the hippocampal formation(Freund and Buzsáki, 1996; McQuiston and Madison, 1999; Pascualet al., 1999; Svoboda et al., 1999). Our recent study (Milneret al., 1999) indicates that a subset of cholinergically targetedNPY interneurons located in the central hilus may depend on suchinput for survival. Further investigations are needed to examinewhether degree of terminal coverage compared to astrocytic coverageof the plasmalemma determines vulnerability of NPY interneuronsafter loss of cholinergic input. Moreover, the morphological variationsbetween NPY-IR perikarya we observed in the current investigation(i.e., many overall terminal contacts vs few terminal contacts)may be relevant to determining the functional consequences ofcholinergic activation among these somata; those cells havingfew contacts may be more potently modulated by cholinergic inputsthan those cells having many terminalcontacts.

The type of synapse formed by cholinergic septal afferents varies depending on the target

We found that the type of synapses formed by cholinergic hippocampal afferents is, at least in part, dependent on target type.In agreement with previous work (Dougherty and Milner, 1999),p75^NTR-IR axon terminals formed both symmetric and asymmetric synapticassociations with their NPY-IR targets. However, when contactingPARV-IR targets, such axon terminals formed exclusively symmetricsynapses. Under these circumstances, postsynaptic responses mayheavily depend on the presence of various classes of cholinergicreceptors, the neurochemical content of other afferents a giventarget receives, and/or the degree to which these inputs are active.Physiological studies have shown that diverse responses to cholinergicexcitation may be mediated by the activation of various classesof muscarinic and nicotinic cholinergic receptors on functionallydistinct subsets of hippocampal interneurons (Behrends and Bruggencate,1993; McQuiston and Madison, 1999). Moreover, anatomical studiesindicate that cholinergic receptors are not only differentiallydistributed within the cellular compartments of subsets hippocampalinterneurons, but that they are differentially regulated by cholinergicseptal input (Levey et al., 1995; Hájos et al., 1998). Together,these findings suggest that acetylcholine release may lead toeither inhibition or excitation within the same cell, as wellas among possibly distinct interneuronpopulations.

Cholinergic septal afferents have additional relationships with PARV-IR neurons

Occasional instances of other types of interactions between p75^NTR-IR axon terminals and PARV-IR neuronal profiles were observedin this study. In a few instances, p75^NTR-IR axon terminals and PARV-IR axon terminals were in close proximityor directly apposed, raising the possibility that PARV-IR axonterminals may modulate septal cholinergic hippocampal afferentsor vice versa. Some granule cell profiles were contacted by botha p75^NTR-IR axon terminal and a PARV-IR axon terminal, likely to originatefrom a basket cell in the infragranular region of the hilus (Ribaket al., 1990). This observation suggests that PARV-containingbasket cells and septal cholinergic afferents could modulate thesame populations of principal cells. In rare instances, PARV-IRand p75^NTR-IR were colocalized in the same neuronal profile, indicatingthat some PARV-IR hippocampal neurons and/or septal PARV-IR afferentsare responsive to one or more of the neurotrophins. The recentfinding that many PARV-IR hilar interneurons produce NGF (Pascualet al., 1999), together with our observation of the p75^NTR within these cells, provides further evidence suggesting thatin the adult, neurotrophin production may be regulated in an autocrinefashion, with local neurotrophin concentrations possibly actingas a component of a negative feedback loop (Zaremba and Dreyfus,1999).

Functional significance

Investigations of both humans and animals have implied indirectly the existence of an association between cholinergic septalafferents and NPY-containing interneurons. In humans with epilepsyand dementia and among experimental animals after seizure induction,both septal cholinergic cells and/or hippocampal NPY/SOM-containinginterneurons degenerate (Chan-Palay et al., 1986; Babb et al.,1989; Lehéricy et al., 1991; Freund et al., 1992; Sloviter, 1994).As presumptive modulators of hippocampal interneurons, any alterationin septohippocampal afferents may affect the cellular mechanismsthat underlie learning and memory. Hippocampal interneurons havebeen proposed to provide the spatial and temporal conditions necessaryfor synaptic modifications that may underlie hippocampal-dependentmemory encoding and retrieval (Paulsen and Moser, 1998). The currentfindings, together with previous evidence (Milner et al., 1997;Freund and Antal, 1988), suggest that septal afferents form synapticassociations with hippocampal interneurons in a transmitter-specificfashion, such that GABAergic septal afferents predominantly contactGABAergic basket cells and cholinergic septal afferents preferentiallytarget NPY-IR HIPP interneurons. Consequently, GABAergic and cholinergicseptal afferents may modulate inputs to hippocampal granule cellsvia separate interneuron populations. Each of these populationsmay be involved in synaptic plasticity: NPY-IR HIPP cells areideally situated to provide control of dendritic segments to supportbackpropagation, whereas basket and chandelier cells, which contactprincipal cell somata and axon initial segments, synchronize principalcell activity and mediate feedback inhibition (for review, seePaulsen and Moser, 1998). Basket and chandelier cells may alsoachieve temporal control of dendritic action potentials by phasingaction potential generation in the soma (Parra et al., 1998).Death of basal forebrain cholinergic neurons, such as that seenin Alzheimer's disease, therefore is likely to lead to a lossof cholinergic modulation of HIPP cells, whereas GABAergic inputonto basket cells remains intact. Functionally, this may leadto profound granule cell inhibition, as well as a desynchronizationof granule cellresponsiveness.

  FOOTNOTES

Received June 17, 1999; revised Aug. 19, 1999; accepted Sept. 3, 1999.

This work was supported by National Institutes of Health Grants MH42834, DA08259, and HL18974 (T.A.M.) and National Institutesof Health training Grant NS07384 (K.D.D.). We thank Ms. SabrinaPrince and Mr. Peter Chang for technical assistance. We also thankDrs. Carrie T. Drake and Joseph P. Pierce for their helpful commentson thismanuscript.
Correspondence should be addressed to Dr. Teresa A. Milner, Division of Neurobiology, Weill Medical College of Cornell University,411 East 69^th Street, New York, NY 10021. E-mail: tmilner{at}mail.med.cornell.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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