Massive Autaptic Self-Innervation of GABAergic Neurons in Cat Visual Cortex

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Volume 17, Number 16, Issue of August 15, 1997 pp. 6352-6364
Copyright ©1997 Society for Neuroscience

Massive Autaptic Self-Innervation of GABAergic Neurons in Cat Visual Cortex

Gábor Tamás¹^,², Eberhard H. Buhl¹, and Peter Somogyi¹
¹ Medical Research Council, Anatomical Neuropharmacology Unit, Department of Pharmacology, University of Oxford, Oxford OX1 3TH, United Kingdom, and ² Department of Comparative Physiology, József Attila University, Szeged, Hungary H-6726

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Autapses are transmitter release sites made by the axon of a neuron on its own dendrites. We determined the numbers and precisesubcellular position of autapses on different spiny and smoothdendritic cell types using intracellular biocytin filling in slicesof adult neocortex.
Potential self-innervation was light microscopically assessed on 10 pyramidal cells, 7 spiny stellate cells, and 41 smoothdendritic neurons from cortical layers II-V. Putative autapsesoccurred on each smooth dendritic neuron and on seven pyramids,but not on spiny stellate cells. However, electron microscopicexamination of all light microscopically predicted sites on pyramids(n = 28) showed only one case of self-innervation with two autapseson dendritic spines. Interneurons were classified by postsynaptictarget distribution (Tamás et al., 1997) and all putative autapsesof seven basket, three dendrite-targeting, and three double bouquetcells were scrutinized. All basket and dendrite-targeting cellsestablished self-innervation, the number of autapses being 12± 7 and 22 ± 12 (mean ± SD), respectively; only one of the doublebouquet cells formed autapses (n = 3). Basket cell autapses (n= 74) were closer to the soma (12.2 ± 22.3 µm) than autapses establishedby dendrite-targeting cells (51.8 ± 49.9 µm; n = 66).
The degree of self-innervation is cell type-specific. Unlike on spiny cells, autapses are abundant on GABAergic basket anddendrite-targeting interneurons, with subcellular location similarto that of synapses formed by the parent cell on other neurons.The extensive self-innervation may modulate integrative propertiesand/or the firing rhythm of the neuron in a manner temporallycorrelated with its own activity.
Key words: autapse; interneuron; neocortex; inhibition; pyramidal cell; feedback

INTRODUCTION

Van der Loos and Glaser (1972) proposed the word "autapse" to describe a transmitter release site made by the axon of a neuronand its own somatodendritic domain. In addition to their originalGolgi study in rabbit neocortex predicting the existence of autapses,possible autaptic contacts have been described in dog (Shkol'nik-Yarros,1971) and rat (Peters and Proskauer, 1980; Preston et al., 1980)cerebral cortex, monkey neostriatum (DiFiglia et al., 1976), andcat spinal cord (Scheibel and Scheibel, 1971). Using intracellularmarkers, several groups also detected apparent self-innervatingconnections from various brain regions, such as substantia nigra(Karabelas and Purpura, 1980) and striatum (Park et al., 1980;Preston et al., 1980), but the above studies were based on lightmicroscopic observations. Peters and Proskauer (1980) verifiedan autapse on a multipolar stellate cell by electron microscopy(EM), and more recently autapses were found on layer V pyramidsin developing neocortex (Lübke et al., 1996), on a fast-spikingneocortical interneuron (Thomson et al., 1996), and on a hippocampalGABAergic basket cell (Cobb et al., 1997). Although autapses formedin cell cultures have been used extensively to study the physiologyof synaptic mechanisms (Segal, 1991; Pan et al., 1993; Shi andRayport, 1994), few proposals have been made for the functionalsignificance of inhibitory autaptic innervation in vivo (neostriatum,Park et al., 1980; Aplysia buccal ganglia, White and Gardner,1981).

Neocortical GABAergic cells generally have smooth dendrites and receive input from both pyramidal and nonpyramidal cells aswell as from subcortical afferents (Kisvárday, 1992). In a seriesof experiments (Buhl et al., 1997; Tamás et al., 1997), we labeledsynaptically coupled pairs of neurons from slices of the cat visualcortex. During the anatomical analysis of such biocytin-filledcell pairs, we found that a significant portion of the connections,as detected by light and electron microscopy, was formed betweenaxons and the soma and dendrites of the same cell. We confirmedthe results with preparations containing only one filled neuron.Using intracellular biocytin labeling and correlated light microscopy(LM) and EM, we determined the exact number of autapses on severalneocortical cell types. The filling of synaptically coupled cellpairs also allowed the comparison of the number and position ofsynaptic junctions on a given postsynaptic cell with that of autapsesestablished by the same presynaptic neuron.

Preliminary results have been published in abstract form (Tamás et al., 1995).

MATERIALS AND METHODS
Slice preparation. Adult female cats weighing 2.6-3.2 kg were deeply anesthetized with intramuscular injection of ketamine(30 mg/kg) and xylazine (1 mg/kg). When pain reflexes had ceased,a craniotomy was performed on each animal to expose the visualcortex. Subsequently, the animals were perfused with ~1500 mlof chilled and oxygenated artificial CSF (ACSF). After the removalof the dura, blocks of brain tissue including the dorsal and medialaspect of the lateral gyrus and containing areas 17 and 18 ofthe visual cortex were removed from both hemispheres, and thebiopsies were then immersed in chilled ACSF. No attempt was madeto locate the retinotopic position of labeled cells. Using a Vibroslice(Campden Instruments, Loughborough, UK), 400-µm-thick frontalslices were cut from the dissected visual areas and transferredto a recording chamber where they were maintained at 34-35°C onnylon mesh at the interface between oxygenated ACSF and a humidifiedatmosphere saturated with a mixture of 95% O₂ and 5% CO₂. TheACSF that was used for electrophysiological recordings was composedof (in mM) 126 NaCl, 3.0 KCl, 1.25 NaH₂PO₄, 24 NaHCO₃, 2.0 MgSO₄,2.0 CaCl₂, and 10 glucose. During perfusion, cutting, and preincubation,all NaCl was replaced with equiosmolar sucrose (252 mM) to preventpassive chloride entry, which has been suggested to be responsiblefor neurotoxicity during slice preparation (Aghajanian and Rasmussen,1989). The slices remained in the sucrose solution for 30 minbefore the perfusion medium was changed to normal ACSF.

Intracellular recordings. Recording electrodes were pulled from standard wall borosilicate tubing, filled with 2% biocytinin 1.5 M KCH₃SO₄, and beveled to a DC resistance of 80-150 M $Omega$ .Putative GABAergic neurons were identified by their physiologicalcharacteristics, for example, short-duration action potentialsfollowed by large amplitude, fast afterhyperpolarizing potentials(fAHPs) (McCormick et al., 1985). Once a stable recording hadbeen obtained, a search was made for cells displaying the electrophysiologicalproperties of pyramidal and spiny stellate neurons. Capacitivecoupling was eliminated on-line using a modified Axoprobe amplifier(Axon Instruments, Foster City, CA). Synaptic coupling was testedusing on-line spike-triggered averaging while eliciting firingin the interneuron with either depolarizing current pulses orconstant DC current injections. Recordings were obtained withan Axoprobe amplifier, which was operated in bridge mode. Experimentaldata were acquired using a PCM instrumentation recorder and storedon videotapes. Data analysis was then continued off-line by redigitizingthe data at 5-20 kHz using commercially available 12 bit analog-to-digitalboards (Computerscope, RC Electronics, Santa Barbara, CA; andLabmaster, National Instruments, Newbury, UK) in conjunction withthe Axograph (Axon Instruments), RC Electronics Computerscope,and Whole Cell Program (courtesy of Dr. J. Dempster, Universityof Strathclyde, Glasgow, UK) software packages.

Histological processing and anatomical evaluation. In most of the cases, depolarizing current pulses (0.1-0.5 nA) resultedin an adequate diffusion of biocytin, filling the recorded neurons.To avoid deformations, slices were sandwiched between two Millipore(Bedford, MA) filters and fixed in 2.5% paraformaldehyde, 1.25%(both w/v) glutaraldehyde, and 15% (v/v) saturated picric acidin 0.1 M phosphate buffer, pH 7.4, for 12-24 hr. The tissue processingwas based on previously described procedures (Han et al., 1993).Briefly, after gelatin embedding, the slices were resectionedat a 60 µm thickness, and the biocytin-filled cells were visualizedby the avidin-biotinylated horseradish peroxidase method withdiaminobenzidine as a chromogen. Sections were postfixed with1% OsO₄ and block-stained in 1% uranyl acetate.

After flat embedding into resin (Durcupan, Fluka, Buchs, Switzerland), recovered cells were reconstructed at 1250× magnificationfrom the entire slice using the 60-µm-thick serial sections withthe aid of a drawing tube attached to a light microscope. In general,axonal filling was of high quality, and a significant portionof the axon collateralization was contained within the slice (i.e.,there were no signs of partially filled axonal branches, becauseall collaterals ended in fine terminal segments with varicositiesor were cut at the surface of the slice). With the exception ofone basket cell, the location of the postsynaptic cells in thecentral portion of the slice enabled us to perform full, or nearlyfull, reconstructions of the dendritic arbors. The entire somatodendriticsurface of both presynaptic and postsynaptic cells was testedfor close appositions with filled axons, each of which was tracedback to the soma. Light micrographs at different focal depthswere taken from all such close appositions and from characteristicaxonal and dendritic patterns.

After light microscopy, axon-rich areas including all layers covered by the axonal field were reembedded for ultrathin sectioning.Serial sections (~80 nm thick) were cut and mounted on single-slotButvar- or Formvar-coated copper grids, contrasted with lead citrate,and used to test synaptic output connections of the identifiedneurons by EM. After determination of the distribution of unlabeledpostsynaptic target elements, such as soma, dendritic shafts,or spines (for details, see Tamás et al., 1997), all light microscopicallydetected sites of close appositions between filled axons and labeledsomata, dendrites, and spines were tested in serial electron microscopicsections. Although in some cases the identification of the postsynapticmembrane specialization was not feasible, owing to the electronopaque reaction end product, we identified synaptic and autapticjunctions based on the following criteria: (1) vesicle accumulationin the presynaptic axonal varicosity, and (2) rigid membrane appositionbetween the presynaptic and postsynaptic element with a characteristicwidening of the extracellular space. With one exception (see Results),the synaptic or autaptic cleft could be recognized by tiltingthe sections with the goniometer of the electron microscope. Membraneapposition alone, even at the electron microscopic level, didnot necessarily reflect the presence of a synaptic junction (seeFig. 2C). Moreover, to avoid underestimation of the number ofsomatic synapses or autapses, all filled somata were completelysectioned serially for electron microscopic analysis to tracethe axonal branches, which may have been obscured by the opaquecell bodies. The dendritic distance of autapses from the somawas measured on two-dimensionally projected reconstructions ofthe cells, thus underestimating the real three-dimensional distancesalong the dendrites.
Fig. 2. Electron microscopic demonstration of autaptic connections established by BCs. A, Two self-innervating boutons (a1, a2) onthe soma (s) of the BC shown in Figure 1A-C. Ai, Aii, The autapticjunctions were identified by the rigid membrane apposition andthe widening of extracellular space (between arrows) and the clusteringof vesicles. Numbering is the same as in Figure 1C. B, CorrelatedLM (Bi) and EM of a self-innervating bouton (a2) targeting thesoma (s) of the parent BC 1102941. The autaptic junction is shownbetween arrows (Bii). C, A bouton (b) of BC 0812942 forms a membraneapposition (star) with its own axon initial segment (ais) withoutautaptic specialization. In a serial section (Ci), the same boutonestablishes a synaptic junction on an unlabeled soma (s). Scalebars: A, Ai, Aii, Bii, C, Ci, 0.2 µm; Ai, Aii, Bii, same magnification;C, Ci, same magnification; B, 2 µm; Bi, 10 µm.
[View Larger Version of this Image (179K GIF file)]

Statistical methods. Fisher's exact test and Pearson's $chi$ ² test for heterogeneity were applied to determine whether the cellgroups defined were homogeneous and/or overlapping (S-Plus, StatisticalSciences, Seattle, WA). The results obtained by the two testswere similar, although the p values were consistently greaterusing Fisher's test; therefore, we give the p values determinedby that test. The nonparametric Mann-Whitney U test was appliedto compare the properties of the different cell types. Unlessindicated otherwise, results are given as mean ± SD.

RESULTS
Putative self-innervation was light microscopically assessed on 58 biocytin-filled neocortical cells, including 41 aspinyinterneurons from layers II-V and 17 spiny cells from layers II-IVof the visual cortex (Table 1). Apparent self-innervation couldbe observed on each smooth dendritic neuron and on the majorityof pyramidal cells, but spiny stellate cells did not have axonterminals apposed to their own somatodendritic surface. Interneuronswere classified by electron microscopic examination of their unlabeledpostsynaptic targets. All putative autapses of 13 smooth dendriticneurons, selected to represent different degrees of overlap betweenthe dendritic and axonal arborization from each class, and allthe possible autaptic junctions on pyramidal cells were subjectto serial sectioning and EM. Altogether 172 light microscopicallyobserved close appositions were tested by EM, and 145 autapsescould be verified. In eight cases we observed membrane appositionswithout autaptic junctions.

Table 1. The extent of self-innervation in cortical neurons

Cell type

Basket Dendrite-targeting Double bouquet Pyramidal Spiny stellate

No. of tested cells 7 3 3 10 7

No. of putative self-innervating cells (LM) 7 3 3 7 0

No. of close process appositions (LM) 57 61 26 28 0

No. of self-innervating cells (EM) 7 3 1 1 0

No. of autaptic junctions (EM) 74 66 3 2 0

No. of autapses per cell (mean ± SD) 12 ± 7 22 ± 12 1 ± 1.73 0.2 ± 0.6 0

No. of autapses per cell (range) 3-23 9-32      0-3      0-2 0

Distance from the soma (2D^a; µm; mean ± SD) 12.2 ± 22.3 51.8 ± 49.9 68.5 ± 35.7 80 -

The complete dendritic arborization of all cells was checked in the LM. All light microscopically observed close appositionsof neural processes were scrutinised in EM in serial ultrathinsections. Because of the irregular outline of the spiny dendritesof pyramidal cells and small, thorn-like boutons of double bouquetcells, light microscopic predictions were highly unreliable. Allneocortical basket and dendrite-targeting cells formed autapses.Basket cell autapses were significantly (p < 0.0001) closer tothe cell body than autaptic junctions established by dendrite-targetingcells. Double bouquet cells with and without autapses might representdifferent subtypes of smooth dendritic neurons with columnar axonalbundles. ^a Measured as two-dimensional projected distance.

It is highly unlikely that autapses were formed during the slicing and incubation procedures, because the occurrence and frequencyof self-innervation was cell type-specific and did not dependon the density of axonal arborizations. Furthermore, some of theself-innervating axonal branches appeared to be specifically alignedwith the dendrites of the cell, forming multiple autaptic junctionsthrough large boutons that did not make synapses with other cells(see Figs. 3, 4).
Fig. 3. Exclusively dendritic self-innervation established by a DTC in area 18. A, Dendritic (red) and axonal (black) arborizationof the DTC. B, Location of electron microscopically verified (seeFig. 4) autaptic innervation by boutons. All autapses were ondendrites at various distances from the soma. One bouton establishedtwo separate autaptic junctions (10, 11). The cell showed a synaptictarget preference toward dendritic shafts (72.7%) and also innervatedspines (27.3%) of other neurons. Asterisks indicate axonal branchingpoints.
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Fig. 4. Correlated LM and EM of autaptic junctions established by the DTC shown in Figure 3. A, A myelinated axonal branch (ax) givesrise to six en terminaux boutons (a1-a5 and unlabeled arrows)apposed to a distal dendrite (d) of the parent cell. Unmarkedarrows indicate autaptic boutons not shown by EM on this figure.B, Three of the autaptic boutons shown in A are seen emergingfrom the myelinated axonal trunk (ax) and target successive dendriticbeads. Bi-Biii, The three autaptic junctions of B are illustratedat higher magnification. C, A self-innervating bouton targetingthe interbead segment of the parent dendrite is surrounded byunlabeled terminals (t) establishing synapses (between arrowheads).The numbering is identical to Figure 3B. Autaptic clefts are indicatedbetween arrows. Scale bars: A, 10 µm; B, 1 µm; Bi-Biii (same magnification),C, 0.3 µm.
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Light microscopic prediction of autapses proved unreliable; the degree of discrepancy between the LM estimates and electronmicroscopically verifiable autaptic junctions depended on thetype of neuron. In the case of basket cells (BCs) and dendrite-targetingcells (DTCs), having smooth dendrites and large axon terminals,68% (n = 28) and 87% (n = 47) of the boutons that appeared tocontact the dendrites were confirmed to make autaptic junctions(see Figs. 2, 4, 6). On somata, 93% (n = 13, BCs) and 84% (n =5, DTCs) of the predicted junctions could be verified (see Figs.2 and 6). The analysis of serial sections of dendritic sites revealedsix (17%, BCs) and seven (12%, DTCs) additional release sitesby boutons forming multiple autaptic junctions (see Fig. 6C).Moreover, 27 and 7 additional autapses were found on the somata(68 and 58% of all identified somatic autapses on BCs and DTCs),which could not be predicted, because the dense peroxidase productobscured boutons on and around the soma (see Fig. 6A). Althoughwe predicted two and one autapses on axon initial segments ofBCs and DTCs, none of these could be verified by EM (see Fig.2C). The spiny dendrites of pyramidal cells have an irregularoutline, and the dimensions of some of the spines are below theresolving power of the light microscope, hampering the predictionof contact with axons passing nearby. Consequently, 93% of predictedcontacts between spiny dendrites and the axon of the neuron werenot autapses when tested by EM (see Fig. 8). The characteristicsof the axon also influenced the predictability of autapses, becausethe potential contacts between the small, thorn-like axonal boutonsof double bouquet and pyramidal cells and their dendrites weredifficult to evaluate in the light microscope. Thus, our largeelectron microscopically tested sample has led to a conclusiondifferent from that of another correlated light and electron microscopicstudy based on eight electron microscopically tested autapticsites (Lübke et al., 1996), which suggested a high reliability(75%) of LM predictions.
Fig. 6. Examples of autaptic junctions established by the DTCs shown in Figure 5. A, B, Autapses on the DTC of Figure 5A. A, An autapticterminal (a,,17) targeting the soma (s) established threeseparate autaptic junctions, two of which (underlined numbers)are illustrated here. B, A bouton (a2) of the DTC forms an autapseon the dendrite of the cell. C, One (underlined number) of thetwo autapses established by a terminal (a,7) of the DTC shownin Figure 5B. A synapse (between arrowheads) formed by an unlabeledbouton (t) and the dendrite (d) of the DTC are indicated. Numberingis identical to Figure 5. Autaptic clefts are indicated betweenarrows. Scale bar for all panels, 0.2 µm.
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Fig. 8. The autaptic junctions established by the pyramidal cell shown in Figure 7. A, B, The axon of the pyramidal cell (ax) formedtwo closely located en terminaux autaptic boutons (a1, a2), whichinnervated two neighboring dendritic spines (s). Autaptic junctionsare indicated between arrows. Scale bar for both panels, 0.2 µm.
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Autapses of basket cells
BCs (n = 8) showed a postsynaptic target preference for somata (49.0 ± 11.8%) and dendritic shafts (47.4 ± 9.9%) and formedsynapses occasionally with dendritic spines (3.6 ± 4.5%; n = 135synapses; n = 26 obtained in this study) (data on six cells fromTamás et al., 1997). LM observations indicated 8.1 ± 3.7 (range,4-13) putative self-innervating contacts on the BCs. We determinedthe total number of autapses per cell on seven neurons from corticallayers II-IV showing similar dendritic trees but three types ofaxonal arborization and, therefore, different degrees of overlapbetween the axonal and dendritic tree. The dendrites of the remainingcell were not recovered, but we found four autapses on the soma,which was completely sectioned serially. Two neurons (1102943and 0812942) distributed their axons mainly in layers II and IIIand established nine and three autapses; four cells (1102941,2402942c1t2, 0812945b, and 2402942c1) sent collaterals to layersV and VI in addition to the extensive branching in layers II andIII and formed 8 (Figs. 1D, 2B), 8, 8, and 23 autaptic junctions.A large BC, with a patchy axon arbor in layers II-VI, established15 autapses, although its axonal cloud was very sparse in thevicinity of the soma (Figs. 1A-C, 2A). Overall, the number ofelectron microscopically verified autapses exceeded the LM predictions.The subcellular location of identified autapses was similar tothe synaptic target distribution on other innervated neurons,because 40 autapses were found on somata (5.7 ± 4.9 per cell;47.3 ± 33.1%), and 34 were found on proximal dendritic shafts(4.9 ± 4.1 per cell; 52.7 ± 33.1%; Fig. 1C,E). Moreover, althoughmembrane apposition could be detected electron microscopicallybetween a BC axon terminal and the initial segment of the axonof the cell, the bouton did not form an autaptic junction (Fig.2C), indicating autaptic target preference toward the somatodendriticdomain. This bouton formed a type II synapse on a neighboringcell body (Fig. 2C).
Fig. 1. Self-innervation by BCs. A-C, Light microscopic reconstructions of a large BC in layer III of area 17. The soma and dendritesare illustrated in red; axons are shown in black. Although theaxonal cloud is relatively sparse in the neighborhood of the soma,the parent cell body is heavily innervated by high-order axonalbranches. B, Route of the axon back to the parent soma. C, Allelectron microscopically verified autaptic junctions were locatedon, or very close to, the cell body. Three boutons establishedmore than one autaptic junction, as indicated by grouped numbers.D, Autaptic junctions of a different type of BC in layer III.The dendritic arborization is shown in red; the axonal branchesforming autapses are presented in black. The complete axonal arborizationis illustrated by Buhl et al. (1997, their Fig. 3). E, Subcellulardistribution of autaptic junctions. Both cells have higher autaptictarget preference toward their soma than in the overall synaptictarget distribution on other neurons. Asterisks indicate axonalbranching points.
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Self-innervation by dendrite-targeting cells
Based on their synaptic target preference (n = 145 synapses), six neurons were defined as DTCs (five cells from Tamás etal., 1997), innervating dendritic shafts predominantly (81.3 ±11.0%) and occasionally dendritic spines (14.9 ± 10.8%) and somata(3.8 ± 4.6%). One cell was reconstructed for this study (Fig.3). Each DTC appeared to be strongly self-innervated on the basisof LM assessment (17.1 ± 7.8 putative contacts; range, 6-26).To determine the total number of autapses on individual cells,a selection of three neurons had been made for EM from corticallayers II-IV, with different degrees of overlap between the dendriticand axonal trees. Regardless of the variability of the cell class,each dendrite-targeting interneuron massively innervated its somatodendriticdomain. Cell 1003953 spanned all cortical layers with straightaxonal branches giving rise to necklace-like terminal segmentsmainly around the border between layers III and IV. The axonalarbor had a horizontal extent of 1460 µm in the slice and established25 autapses (Figs. 3, 4). A different, columnar axonal arborizationwas formed by cell 1506935 (for full reconstruction, see Tamáset al., 1997, their Fig. 6), which made 32 autapses (Figs. 5A,6A,B). The third electron microscopically fully analyzed cell(1612941; for full reconstruction, see Buhl et al., 1997, theirFig. 1) had the bulk of its axonal terminals in layer IVa andestablished nine autaptic junctions (Figs. 5B, 6C). Autapses onDTCs were located predominantly on dendrites (n = 54; 18.0 ± 9.6per cell; 82.2 ± 16.1%), and autaptic junctions on the parentsomata were less frequent (n = 12; 4.0 ± 5.3 per cell; 17.8 ±16.1%), a result similar to the overall synaptic target preferenceof the three neurons (Figs. 4, 6). Dendrite-targeting interneuronshad a higher number of dendritic autapses than BCs (p < 0.05,Mann-Whitney U test), and, in addition, the distance of autapticjunctions from the soma, as measured in two-dimensional projection,was significantly greater (p < 0.0001; see Table 1).
Fig. 5. Comparison of synaptic and autaptic connections established by individual interneurons. A, Synaptic and autaptic connectionsof a layer IV DTC (soma and dendrites, red; axon, black) and aspiny stellate cell (soma and dendrites, green; axon not shown).The complete axonal and dendritic arborizations are shown by Tamáset al., (1997, their Fig. 6). The DTC innervated the spiny cellthrough three dendritic synapses (s1-s3) and established 32 autapses(a1-a32). Grouped numbers represent multiple autaptic junctionsformed by the same bouton. Ten autapses were found on the soma,a higher proportion than the somatic targets (10.7%) in the overallsynaptic target distribution. B, Synaptic and autaptic relationshipsbetween a layer IV DTC (soma and dendrites, red; axon, black)and a layer III-IV border pyramidal cell (soma and dendrites,green; axon, blue). The complete axonal and dendritic arborizationsare shown by Buhl et al., (1997, their Fig. 1). The cell pairwas in reciprocal synaptic connection, but only the effect ofthe pyramidal cell could be recorded. The DTC established nineautaptic junctions (a1-a9), innervated the pyramidal cell via17 synapses (i1-i17), and received five synapses from the pyramid(p1-p5). Note that the subcellular distribution of synaptic andautaptic junctions established by the interneuron was similaron both cells.
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Autapses on double bouquet cells
In the course of the experiments six double bouquet cells (DBCs) were recorded, but, despite extensive axonal filling, thedendrites were recovered from only three neurons. We then investigatedthe extent of self-innervation on the three fully recovered cells.Putative autapses were predicted by light microscopy on the dendritesof each DBC. On two cells, which had 8 and 12 suspected contactsites, none of the sites turned out to be autaptic junctions whentested by EM. On the third cell, three of six putative autapsescould be verified by EM, and the autaptic junctions were on relativelydistal dendrites (Table 1). It should be added that althoughthe three cells were classified as DBCs, based on their characteristicaxonal bundle traversing through all layers of the cortex (Somogyiand Cowey, 1981; Tamás et al., 1997), they showed a number ofdissimilar characteristics. The dendrites of the two cells withoutautapses were thin and unbeaded and had branching points relativelydistal (up to 100 µm) from the soma. In addition, the proximalregion of these dendrites received characteristic invaginatedasymmetrical synapses with a wide nonjunctional membrane appositionbetween the dendrite and the presynaptic terminals. The axonsof these cells, and of all DBCs without recovered dendrites (Tamáset al., 1997), had small, thorn- or mushroom-like varicositiesand thin interbouton segments and targeted preferentially dendriticspines (64.0 and 67.7%, respectively) and less frequently dendriticshafts (36.0 and 32.3%, respectively) (Tamás et al., 1997). Incontrast, the dendrites of the additional DBC (not illustrated)analyzed in this study were strongly beaded, branching in theproximity of the soma and not receiving invaginated type I synapses.The axon of this autapse-forming cell was also different in thatit had large, round terminals and thicker interbouton axon segmentsthan the other DBCs. The random sample taken from unlabeled postsynaptictargets (n = 24) of this DBC showed a preference toward dendriticshafts (62.5%) over dendritic spines (37.5%). The postsynaptictarget selectivity of the three DBCs tested here for autapseswas heterogeneous (Fisher's exact test for heterogeneity, p <0.05), but the two cells that formed no autapses were membersof a homogeneous class of cells (Tamás et al., 1997).

Comparison of synaptic and autaptic innervations established by the same interneurons
The number and location of autapses could be compared with those of identified synapses established by the same neuron. Oneof the DTCs (1506935) elicited fast IPSPs in a postsynaptic spinystellate cell through three dendritic release sites, which wereequidistant from the soma of the spiny stellate cell (see Tamáset al., 1997, their Fig. 6). The autaptic innervation was an orderof magnitude higher in terms of the number of release sites (n= 32). Autapses were scattered over the surface of the parentcell, varying from relatively distal dendrites (Fig. 5A, a14)to the soma (Fig. 6A,B). It should be added, however, that aswith DTC 1612941, all somatic autapses were formed by only oneaxon collateral, and the cell showed a moderate innervation ofthe somata of other neurons (10.5%).

All autaptic and synaptic (Tamás et al., 1997) junctions were also tested electron microscopically from cell pair 1612941,consisting of a reciprocally connected layer III-IV border pyramidalcell and a layer IV DTC (Fig. 5B). Only the EPSPs, elicited bythe pyramidal cell via five synapses, were measured in the DTC(for the recordings and complete axonal and dendritic arbors,see Buhl et al., 1997, their Fig. 1). The interneuron establishedmultiple synaptic junctions (n = 17) on the pyramidal cell andalso formed numerous autapses (n = 9); the subcellular locationof synaptic and autaptic junctions was similar. The pyramid wasinnervated by two synaptic clusters on two basal dendrites (i6-i10and i14-i17) and by a cluster on the soma near the origin of adendrite (i1-i5). Autapses on the parent cell formed a clusteron the soma (a3-a4), two clusters (a5-a7 and a8-a9), and two solitaryjunctions (a1 and a2) on dendrites (Figs. 5B, 6C).

Rare self-innervation of pyramidal cells
We tested 10 cells from granular and supragranular layers, including one cell in layer IV, three in layers II and III, twosmall pyramids in layer II, and four layer III-IV border pyramidalcells. The local axonal arborizations varied from a narrow, columnar-typedistribution to a wider, fan-like arrangement, but in each casenumerous axonal branches passed through the dendritic arbor. Althoughon seven cells close appositions could be observed in the lightmicroscope between axons and the dendritic shafts (n = 17) andspines (n = 11) of the parent cell, only two autapses could beverified by EM on two neighboring spines of a layer III-IV borderpyramidal cell (Figs. 7, 8). In addition, a membrane appositionbetween the same axon collateral forming the verified autapsesand a basal dendritic shaft could not be evaluated reliably becauseof the almost parallel plane of the cutting and the potentialautaptic cleft. On two other pyramidal cells, 2 nonautaptic membraneappositions were found on dendritic shafts.
Fig. 7. Reconstruction of the only self-innervating pyramidal cell of 10 tested. A, Dendritic and axonal arborization of the pyramidalcell from area 17. B, Location of the two electron microscopicallyverified autaptic junctions on the pyramidal cell. Autapses wereformed by two neighboring boutons of a seventh order axon collateralon two adjacent dendritic spines on a fourth order dendrite. Forcorrelated EM of the connection, see Figure 8. Asterisks indicateaxonal branching points.
[View Larger Version of this Image (15K GIF file)]

DISCUSSION
The results demonstrate extensive self-innervation by at least two distinct classes of GABAergic cortical neurons, BCs andDTCs. We identified 32 autapses on a DTC, which represent thehighest number of transmitter release sites so far on a singlecortical cell originating from an individual axon of any origin(e.g., see Freund et al., 1985; Kisvárday et al., 1987; Deucharset al., 1994; Thomson et al., 1996; Buhl et al., 1997). The formationof autapses is both cell type-specific and selective with regardto the placement of autapses on specific subcellular domains.A high level of self-innervation in the two cell classes is incontrast with its absence or rare occurrence in spiny stellateand pyramidal cells as well as in other types of GABAergic neurons.By testing 172 predicted sites we found that in many cases LMpredictions for autapses are unreliable, and electron microscopicevaluation is essential to ascertain the presence of both directmembrane apposition and autaptic membrane specialization.

Autapses in the CNS
The existence of autapses has been reported primarily from cultures (Crain, 1971; Landis, 1976; Bekkers and Stevens, 1991;Segal, 1991), and their formation has been considered an artifactbecause of the lack of appropriate postsynaptic targets. Occasionalautapses on neurons have been reported in anatomical studies fromvarious brain regions (Held, 1897; Chan-Palay, 1971; Scheibeland Scheibel, 1971; Shkol'nik-Yarros, 1971; Van der Loos and Glaser,1972; DiFiglia et al., 1976; Karabelas and Purpura, 1980; Petersand Proskauer, 1980; Preston et al., 1980; Kuffler et al., 1987;Shi and Rayport, 1994; Lübke et al., 1996), but in view of ourdifficulty predicting the existence of autapses on the basis oflight microscopy, some of the previous predictions will requirereexamination, including EM or physiology. To our knowledge, electronmicroscopic studies have so far verified one autapse on a smoothdendritic stellate cell (Peters and Proskauer, 1980), six autapseson layer V pyramidal cells (Lübke et al., 1996), one autapticjunction on a fast-spiking interneuron (Thomson et al., 1996),and five autapses on a hippocampal basket cell (Cobb et al., 1997).

Self-innervation is cell type- and domain-specific
It is possible that autapses may result from the chance meeting of the axon of the neuron with its somatodendritic surface.However, several observations suggest that this is not the case.First, the number of autapses per BC or DTC is at least threetimes higher than the number of potential synapses originatingfrom a single interneuron on an individual postsynaptic cell,assuming that each cell in the axonal field receives an equalnumber of unitary synapses (Tamás et al., 1997). Second, thedegree of autaptic innervation greatly varies between differenttypes of cell, although there is a substantial overlap betweenthe dendritic and axonal arborizations in all cell types tested.Although within the dendritic tree the density of GABAergic boutonsoriginating from a single cell is higher than that of pyramidaland spiny stellate cells, this alone does not explain the highincidence of autapses, because axo-axonic cells do not form autapses(Somogyi et al., 1982; Freund et al., 1983), and DBCs only exceptionallyseem to establish self-innervation despite the high density oftheir axons. Third, the subcellular domain-specific innervationof a cell seems to be preserved in the autaptic innervation; "forbidden"cell regions are not targeted by autapses, even when membraneapposition provides an opportunity. Finally, cells with a sparseaxon cloud in their somatodendritic domain establish massive autapticinnervation.

Autapses on BCs are also placed close to their soma in the hippocampus of the rat (Cobb et al., 1997), and a multipolar stellatecell in the rat cortex, resembling BCs identified in this study,formed an autapse close to the soma (Peters and Proskauer, 1980).The DTC autapses were more distal than BC autapses, similar tothe more distal location of their efferent synapses. Pyramidalcells, when they form autapses, do so on dendritic shafts andspines (Lübke et al., 1996), where their efferent synapses arefound on other cortical cells (Kisvárday et al., 1986; Deucharset al., 1994). Target zone preference might also contribute tothe lack of autaptic innervation by some aspiny DBCs, which terminatepredominantly on dendritic spines and occasionally on shafts (Tamáset al., 1997). The preservation of subcellular specificity forthe placement of transmitter release sites suggests a similarfunctional role for the autapses and synapses of the cell.

Supragranular pyramidal cells in the adult cat cortex, with one exception, did not form autapses, in contrast to the reportedpresence of frequent autapses on layer V pyramids in the developingrat cortex (Lübke et al., 1996). Apart from the differences inspecies and the age of the animals, methodological factors mayalso explain the difference in conclusions, because in our studyLM examination alone would have also led to a higher incidenceof predicted autapses. However, pyramidal cells constitute manymorphological and physiological subtypes (Chagnac-Amitai et al.,1990; Larkman and Mason, 1990), and further studies may revealmore extensive autaptic innervation in some of the types not examinedhere.

Possible functional significance of autapses
In cultured excitatory and inhibitory neurons (Bekkers and Stevens, 1991; Segal, 1991; Shi and Rayport, 1994) the effect ofautapses is mediated by receptor mechanisms similar to those detectedat efferent synapses of the same cell class. Indeed, Park et al.,(1980) showed putative autaptic GABA_A receptor-mediated shuntingof evoked EPSPs after burst firing in GABAergic striatal mediumspiny neurons. What functional differences require self-innervationfor some GABAergic cells in the cortex, but not for others, remainsunclear. It is conceivable, however, that differences in the firingpattern of interneurons having or lacking autapses may be shapedby the autaptic outward currents in a certain frequency range.Inhibitory autapses can prolong the initial interspike intervalin Aplysia buccal ganglia (White and Gardner, 1981), maximizespike frequency, prevent burst firing, and contribute to spikeafterhyperpolarization in cultured nucleus accumbens neurons (Shiand Rayport, 1994).

In the neocortex, neither excitatory nor inhibitory autaptic effects have been recorded, but the cell type specificity andthe high number of autapses on some GABAergic cells predict effectsthat are functionally significant for the operation of these cells.It is not known how many synapses converge on a cortical GABAergiccell of any type, but in analogy with other cells a range of 1000-5000seems realistic (Anderson et al., 1994). Taking a value of 3000,the mean number of autapses being 13, it is apparent that 0.4%of all transmitter release sites could originate from the axonof the neuron. If the proportion of GABAergic synapses in theinput of BCs and DTCs is the same as in the overall population,then 17% of the synapses would be GABAergic (Beaulieu and Somogyi,1990). On average, autapses would then provide 2.5% (range, 0.6-6%)of the GABAergic input to BCs and DTCs. The amplitude of somaticallyrecorded unitary IPSPs elicited by self-innervating BCs and DTCsin postsynaptic pyramidal and spiny stellate cells was 1416 ±769 µV (Tamás et al., 1997). Assuming that autapses have functionalproperties similar to synapses made by the same cell, a fast GABAergiceffect could significantly influence local dendritic informationprocessing and possibly also the firing properties of the cell.

Recent results indicate that IPSPs evoked in dendrites can modulate spike back-propagation and associated changes in intracellularcalcium electrogenesis (Miles et al., 1996; Tsubokawa and Ross,1996). It is not known whether action potentials are activelypropagated in the dendrites of cortical GABAergic cells, but inGABAergic cells of the substantia nigra this might be the case(Häusser et al., 1995). Back-propagating action potentials andautaptic IPSPs would be tightly correlated and could arrive insynchrony at the dendrites. The relative timing would be influencedby the subcellular position of autapses and the length, myelination,and thickness of axonal branches connecting the autaptic terminals.Whether an interaction of possible back-propagating action potentialswith tightly correlated IPSPs is necessary for the function ofcertain GABAergic neurons remains to be established, but it couldbe relevant in regulating coincidence between postsynaptic potentialsand action potentials (Markram et al., 1997).

The generation of an IPSP of tens of milliseconds duration in the dendrites and soma of a neuron that fired an action potentialas a result of synaptic drive may not initially have much effect,owing to the considerably larger conductance of the action potentialand the fAHP, the latter being much shorter in BCs and DTCs thana conventional GABA_A receptor-mediated IPSP (Luhmann and Prince,1991). Therefore, the late phase of the IPSP could potentiallyinteract with other PSPs after the AHP. The effect of an increasein conductance during the autaptic IPSP may shorten EPSP duration,narrowing the window for summation and promoting coincidence detection(Softky, 1995; Buhl et al., 1997). Such a modulatory effect wouldbe linked to the firing activity of the neuron, and the high numberof autapses reported here could selectively influence the EPSPsthat arrive temporally correlated with the firing of the cell.

FOOTNOTES

Received April 2, 1997; revised June 3, 1997; accepted June 6, 1997.

This project was supported by the Wellcome Trust and by European Community Grant BIO4-CT96-0585. G.T. was supported by theOxford-Szeged Scholarship and the Blaschko Visiting Research Scholarship.E.H.B. holds a Medical Research Fellowship from Corpus ChristiCollege (Oxford, UK). We thank Mr. J. D. B. Roberts and Mr. F.Kennedy for technical and photographic assistance.

Correspondence should be addressed to Gábor Tamás, Medical Research Council Anatomical Neuropharmacology Unit, Universityof Oxford, Mansfield Road, Oxford OX1 3TH, UK.

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Massive Autaptic Self-Innervation of GABAergic Neurons in Cat Visual Cortex

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Volume 17, Number 16, Issue of August 15, 1997 pp. 6352-6364
Copyright ©1997 Society for Neuroscience