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The Journal of Neuroscience, June 1, 1998, 18(11):4255-4270
Differentially Interconnected Networks of GABAergic Interneurons
in the Visual Cortex of the Cat
Gábor
Tamás1, 2,
Peter
Somogyi1, and
Eberhard H.
Buhl1
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,
H-6726, Hungary
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ABSTRACT |
Networks of GABAergic neurons have been implicated in neuronal
population synchronization. To define the extent of cellular interconnections, we determined the effect, number, and subcellular distribution of synapses between putative GABAergic neurons in layers
II-IV of the cat visual cortex using paired intracellular recordings
in vitro followed by correlated light and electron microscopy. All neurons having interneuronal electrophysiological properties were classified by their postsynaptic target profile and
were identified as basket (BC; n = 6),
dendrite-targeting (DTC; n = 1), and double bouquet
(DBC; n = 2) cells. In four out of five
anatomically fully recovered and reconstructed cell pairs, synaptic
connections were found to be reciprocal. Generally BCs established
synaptic junctions closer (21 ± 20 µm) to postsynaptic somata
than did DBCs (43 ± 19 µm; p < 0.01). The
unitary number of synapses (n values, 10, 7, and 20) in
each of three BC-to-BC pairs was higher than that in three BC-to-DBC
(n values, 1, 2, and 2) and three DBC-to-BC
(n values, 1, 4, and 4) connections (p < 0.05). A BC innervated a DTC through
two synaptic junctions. Unitary postsynaptic effects mediated by five
BCs could be recorded in two BCs, two DBCs, and a DTC. The BCs elicited
short-duration fast IPSPs, similar to those mediated by
GABAA receptors. At a membrane potential of  55.0 ± 6.4 mV, unitary IPSPs (n = 5) had a mean amplitude
of 919 ± 863 µV. Postsynaptic response failures were absent
when an IPSP was mediated by several release sites. Thus, distinct
GABAergic interneurons form reciprocally interconnected networks. The
strength of innervation and the proximal placement of synapses suggest
a prominent role for BCs in governing the activity of intracortical
GABAergic networks in layers II-IV.
Key words:
cerebral cortex; interneuron; inhibition; IPSP; GABA; synapse
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INTRODUCTION |
Local-circuit GABAergic neurons
modulate the operation of excitatory neurons in cortical networks. They
govern the generation and backpropagation of action potentials
(Andersen et al., 1963 ; Miles and Wong, 1987; Buhl et al., 1995;
Buzsaki et al., 1996; Tsubokawa and Ross, 1996) dendritic calcium
electrogenesis (Traub et al., 1994; Miles et al., 1996) and play a role
in synchronizing population activity (Cobb et al., 1995; Whittington et
al., 1995; Bush and Sejnowski, 1996; Freund and Buzsaki, 1996).
Analysis of inhibitory unitary interactions between identified
interneurons and principal cells revealed that distinct classes of
GABAergic neurons terminate on different subcellular domains and elicit fast IPSPs (Buhl et al., 1994; Miles et al., 1996; Thomson et al.,
1996; Tamas et al., 1997a).
Cortical interneurons themselves are also under GABAergic control,
because they receive GABAergic afferents from both subcortical and
cortical sources. In the neocortex, the main extrinsic source of
inhibitory innervation is the basal forebrain, and this pathway terminates predominantly on GABAergic neurons (Freund and Meskenaite, 1992). Cortical GABAergic afferents arise either from smooth dendritic interneurons exclusively innervating other GABAergic cells, as recently
demonstrated in the hippocampus (Acsady et al., 1996; Gulyas et al.,
1996), or from GABAergic neurons divergently innervating both principal
and GABAergic neurons (Somogyi et al., 1983; Kisvarday et al., 1985,
1993; Freund et al., 1986; Cobb et al., 1997; Meskenaite, 1997).
Moreover, in cat visual cortex, large GABAergic basket cells form an
interconnected network linking columns with different orientation
preferences (Kisvarday et al., 1993, 1994).
Regarding the functional effect of GABAergic interneurons, the same
presynaptic GABAergic cell evoked qualitatively similar fast IPSPs in
both postsynaptic interneurons and pyramidal cells (Cobb et al., 1997).
Modeling studies indicate that such fast IPSPs can synchronize a
network of mutually connected interneurons that, in turn, generates a
coherent oscillatory output to principal neurons (Traub et al., 1996;
Wang and Buzsaki, 1996). Indeed, recent in vitro experiments
show that cortical inhibitory neurons can generate oscillatory network
activity in the gamma frequency range (Whittington et al., 1995). Such
oscillations occur in the neocortex of behaving animals in response to
visual stimulation, and they may be of major importance in the cortical
representation of objects, the so-called binding phenomenon [for
review, see Singer and Gray (1995)]. Computational simulations of
gamma frequency network oscillations require an appreciable degree of
mutual connectivity between interneurons and a critical minimum of
synaptic connectedness to induce and maintain rhythmic population
activity (Traub et al., 1996; Wang and Buzsaki, 1996), but there is
little experimental information on the degree of GABAergic
interconnections.
This study addresses the extent and mode of
synaptic interactions between GABAergic neurons innervating both spiny
and smooth dendritic cells by using in vitro paired
intracellular recordings and light and electron microscopy. Below, we
not only determine the degree of reciprocity between interneurons, but
we also investigate their domain-specific efferent connectivity and
specific differences in the strength of unitary connections.
Parts of this paper have been published previously (Tamas et al., 1995,
1997a).
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MATERIALS AND METHODS |
Slice preparation. Adult female cats weighing
2.6-3.2 kg were deeply anesthetized with an intramuscular injection of
a mixture of ketamine (30 mg/kg) and xylazine (10 mg/kg). After the
cessation of noxious reflexes (pedal withdrawal and/or tail pinch
reflex), a craniotomy was performed over the occipital cortex, leaving the dura intact. After ensuring adequate levels of anesthesia by
ascertaining the loss of pain reflexes (see above), we perfused the
animals with ~1.5 l of modified (see below) artificial CSF (ACSF)
that had been chilled and oxygenated. Then the dura was opened, and a
5-8 mm block of occipital cortex was excised from one of the
hemispheres and immersed in chilled ACSF. The tissue was sectioned on a
vibroslice (Campden Instruments, Loughborough, UK) in the frontal plane
at 400 µm thickness. The slices were trimmed, keeping primarily the
crest of the lateral gyrus, including portions of areas 17 and 18, and
then transferred to a recording chamber, where they were maintained at
34-35°C on a nylon mesh at the interface between oxygenated ACSF and
a humidified atmosphere saturated with 95% O2/5%
CO2. The normal ACSF was composed of (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). The slices remained in the sucrose solution for 30 min
before the perfusion medium was changed to normal ACSF.
Intracellular recordings and data analysis. Recording
electrodes were pulled from standard wall borosilicate tubing, filled with 2% biocytin in 1.5 M potassium methyl sulfate, and
beveled to a DC resistance of 80-150 M . Putative GABAergic neurons
were identified by their physiological characteristics, such as
short-duration action potentials (APs) followed by large-amplitude fast
afterhyperpolarizing potentials (fAHPs) (see Figs.
1Ea, 2Ga) (McCormick et al., 1985). After
a stable recording had been obtained, a search was made for cells
displaying similar electrophysiological properties (e.g., see Fig.
2J). Capacitive coupling was eliminated on-line
using a modified (Mason et al., 1991) Axoprobe amplifier that was
operated in bridge mode (Axon Instruments, Foster City, CA). Synaptic
coupling was tested using on-line spike-triggered averaging while
eliciting firing in the interneuron with depolarizing current pulses.
Firing rates in the interneurons were adjusted by varying the current intensity and, depending on the particular protocol, ranged between 0.3 and >100 Hz. Experimental data were acquired using a pulse code
modulation (PCM) instrumentation recorder and were stored on
videotapes. Data analysis was continued off-line by (re)digitizing the
data at 5-20 kHz using commercially available 12 bit analog-to-digital boards (RC Electronics, Santa Barbara, CA, and National Instruments Labmaster, Newbury, UK) in conjunction with Axograph (Axon
Instruments), RC Electronics Computerscope (RC Electronics), and
whole-cell program (courtesy of Dr. J. Dempster, University of
Strathclyde, UK) software packages.
Resting membrane potentials were determined after electrode withdrawal
and are given as the difference between surface DC potential and the
most negative steady state membrane potential without bias current
injection. Membrane time constants were obtained from the decay of
small-amplitude hyperpolarizing current pulses and could be well fitted
with a single exponential function in all cells. Likewise, input
resistance was determined from measuring the maximal deflection of
averaged small-amplitude hyperpolarizing current pulses. Spike
amplitudes were taken from baseline to the peak of the action
potential; spike duration was measured at half-amplitude. Unitary IPSP
amplitudes were measured from baseline to peak. The corresponding noise
levels were determined for the same time interval from baseline to
baseline, using the pre-event interval of the same traces.
Distributions of measured IPSP and noise amplitudes showed no
significant differences relative to ideal normal distributions (Kolmogorov-Smirnov normality tests; p > 0.516). Data
for amplitude histograms were used only from epochs in which the
postsynaptic responses remained stationary, defined as epochs during
which (1) the mean amplitude of 50 consecutive IPSPs remained
within ± 1 SD of the mean amplitude of the first 50 IPSPs of the
epoch and (2) no significant change of either IPSP or noise amplitudes was noted over time (Pearson correlation; p > 0.08).
To assess paired-pulse modulation of unitary IPSPs, we elicited
consecutive action potentials in the presynaptic cells
(n = 2) by injecting either a single current pulse of
100-200 msec duration evoking two action potentials or two brief
consecutive current pulses with one action potential each. Both cells
were activated at a rate of 1 Hz. All synaptic events (see Figs. 1, 2,
in which n is 25 or 217 in cell pairs, respectively) were
aligned on the rising phase of the first presynaptic action potential and subsequently, because of variations of the interspike intervals, realigned on the rising phase of the successive second action potential. Then, the respective voltage traces of the postsynaptic cell
were averaged over each of four equal-length periods, with those used
for noise and IPSP measurements separated by equal intervals. Average
voltages for the first two periods preceding the synaptic event were
calculated for each sweep, and their respective differences provided
the noise sample distribution. Likewise, IPSP peak amplitude
measurements were obtained from the set of differences between the
average voltage of a period preceding the IPSP and the time window
encompassing the peak of the IPSP. Because of some relatively brief
interspike intervals (<70 msec) that were used to evoke paired-pulse
modulation of unitary IPSPs, the ongoing decay of the first,
conditioning IPSPs could significantly overlap with the rise of the
successive event, essentially arising from a sloping baseline and
therefore affecting the measurements of the second IPSP. Assuming
linear summation of the recorded voltage, we corrected the amplitude
measurements that were obtained for the second IPSP (all events  2 × SD of noise) for the extrapolated decay of the preceding
IPSP, taking into account the respective interspike interval as well as
the peak amplitude and monoexponential decay kinetics of the
conditioning event.
Histological processing and anatomical evaluation. In most
of the cases, diffusion, presumably aided by current pulses (0.1-0.5 nA) used during recording, resulted in an adequate filling of neurons
with biocytin. Slices were sandwiched between two Millipore filters to
avoid deformations and were fixed in 2.5% paraformaldehyde, 1.25%
glutaraldehyde, and 15% (v/v) saturated picric acid in 0.1 M phosphate buffer, pH 7.4, for 12-24 hr. The tissue
processing was based on previously described procedures (Han et al.,
1993; Buhl et al., 1994). Briefly, after gelatin embedding, the slices were resectioned at 60 µm thickness, and the biocytin-filled cells were visualized by the avidin-biotinylated horseradish peroxidase method with diaminobenzidine as the chromogen. Sections were post-fixed with 1% OsO4, block-stained in 1% uranyl acetate,
dehydrated, and embedded into epoxy resin (Durcupan; Fluka, Buchs,
Switzerland) on glass slides.
Recovered cells were reconstructed at 1250× magnification from the
serial, 60-µm-thick sections of the entire slice using a light
microscope and a drawing tube. Although cells can be filled completely,
the reagents used for visualizing biocytin do not penetrate well into
the myelinated segments of axons, which often remain faint.
Nevertheless, the axons can be followed accurately along the Ranvier
nodes that are stained and easily recognized in osmium-treated
material. The total number of axonal varicosities in the slice, some of
them shown by subsequent electron microscopy to
correspond to synaptic boutons, was counted during the drawing procedure. Although in some cases the axons of different types of
interneuron within the same slice could be differentiated based on
anatomical criteria alone (see Results), each axonal branch presented
in the reconstructions was followed back to the parent soma. Within a
specimen, the average proportion of filled axonal varicosities that
could not be traced back to the axon initial segments was 8.5 ± 3.7%. However, in the presented cases, all axonal branches that formed
a putative contact site on a filled soma or dendrite could be followed
back to the parent soma. Because of the location of pre- and
postsynaptic cells in the central portion of the slice, we could obtain
nearly complete reconstructions of the dendritic arbors in each case.
The entire somatodendritic surface of both recorded cells was
investigated for close appositions with filled axons, each of which
could be traced back to the respective parent soma. Light micrographs
at different focal depths were taken from all such close appositions
and from characteristic axonal and dendritic patterns.
After light microscopic analysis, axon-rich areas, including all layers
covered by the axonal field, were re-embedded for ultrathin sectioning.
Serial sections were cut and mounted on single-slot Formvar-coated
copper grids and contrasted with lead citrate. The sections were
scanned in the electron microscope, and all biocytin-filled axonal
profiles were followed until they formed synaptic contacts. Because all
profiles were followed and the plane of the section randomly cuts
through the axonal branches, the above procedure ensured a random
sample of postsynaptic targets. Each presynaptic terminal under
scrutiny was completely examined in serial sections to establish the
number of synapses it formed. The tracing of serial sections was also
useful to distinguish between dendritic spines and small caliber
dendritic shafts as postsynaptic elements. In some cases, when the
tracing was not feasible, small diameter postsynaptic profiles
containing mitochondria and/or microtubules were classified as
dendritic shafts, although infrequently spines may also contain
mitochondria (Anderson et al., 1994; G. Tamás, E. H. Buhl, and P. Somogyi, unpublished observations). Subsequently, all light
microscopically detected sites of close appositions between filled
axons and labeled somata or dendrites were followed in serial electron
microscopic sections. Although in some cases the identification of the
postsynaptic membrane specialization was not possible because of the
electron-opaque reaction endproduct, we verified synaptic junctions
based on the following criteria: (1) vesicle accumulation at the
junctional site in the presynaptic axonal varicosity and (2) rigid
membrane apposition between the pre- and postsynaptic element with a
characteristic widening of the extracellular space. When the plane of
the section was not perpendicular to the junctional membranes, the
synaptic cleft could be recognized by tilting the section using the
goniometer of the electron microscope. Direct membrane apposition alone
did not predict the presence of a synaptic junction. Moreover, all filled somata were serially sectioned completely for electron microscopic analysis to check for the presence of axonal branches that
may have been obscured by the opaque cell bodies. The distances of
synaptic junctions from the respective soma were measured along the
dendrites on two-dimensional reconstructions.
Statistics. The nonparametric Mann-Whitney U
test was applied to compare the properties of the different cell types.
Unless indicated otherwise, results are given as the mean ± SD.
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RESULTS |
A total of nine smooth dendritic interneurons were studied,
resulting in the analysis of 10 paired unitary interactions. They were
comprised of three synaptically coupled pairs of interneurons and a
network of three reciprocally interconnected GABAergic cells. During
physiological recordings, neurons were tentatively identified according
to their firing characteristics. Despite differences in the properties
of distinct cell types, it was not possible to discriminate reliably
between interneurons on physiological grounds; therefore anatomical
identification of cell types was considered to be essential. Because
the primary aim of our study was the definition of synaptic
interactions between different types of smooth dendritic cells, we used
a well-established classification scheme according to which cells are
grouped with respect to their differential innervation of postsynaptic
membrane domains (Szentagothai and Arbib, 1974; Somogyi, 1989; Tamas et
al., 1997b). The GABAergic nature of basket cells is well established
(Somogyi and Soltesz, 1986). Dendrite-targeting cells, a class of cell
defined recently on the basis of the placement of their synaptic
terminals on proximal dendrites (Tamas et al., 1997b), make synaptic
junctions (type II; Gray, 1959) and evoke postsynaptic responses
similar to those of basket cells (Tamas et al., 1997b) and therefore
are also likely to be GABAergic, but this has not been demonstrated
directly. Double bouquet cells also establish Gray's type II synapses
and elicit fast IPSPs with a reversal potential close to the chloride equilibrium potential (Tamas et al., 1997b); therefore they are very
likely to use GABA as a transmitter.
Distinct categories of GABAergic interneurons
Based on random samples of postsynaptic target elements
(n = 75), five smooth dendritic cells were identified
as "basket cells" (BCs) innervating mainly somata (52.8 ± 12.8%) and dendritic shafts (44.3 ± 11.5%) and, on occasion,
dendritic spines and axon initial segments [1.3 ± 3.0 and
4.4 ± 9.9%; n = 26 synapses in this study; synaptic target data for three cells have been reported by Tamas et al.
(1997a)]. Sampling of the target elements could not be performed
randomly from the postsynaptic cell of cell pair 1412941 (Fig.
1) because only the main axonal trunks
and three bouton-forming collaterals were recovered from the axon. The
recovered boutons made synapses with three somata (43%), three
dendritic shafts (43%), and one dendritic spine (14%); therefore this
neuron was also classified as a BC. All BCs were characterized by
nonspiny, prominently beaded dendrites that bifurcated near the soma
into secondary and tertiary branches. With the exception of cell
0609964, which innervated mainly layer IVb, thus corresponding to
previously described clutch cells (Kisvarday et al., 1985), BCs
distributed their axons predominantly in layers II-III and sent
descending collaterals to layers V and VI. Detailed descriptions of the
morphological characteristics of BCs have been published (Gilbert and
Wiesel, 1979; Martin et al., 1983; Somogyi et al., 1983; Kisvarday et al., 1985; Tamas et al., 1997b). The BCs had a mean resting membrane potential of 63.0 ± 11.4 mV (n = 6) and an
input resistance of 41.7 ± 14.2 M (n = 4) and
fired APs with amplitudes of 48.1 ± 14.6 mV (n = 6).
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Figure 1.
Reconstruction and synaptic effect of a BC-to-BC
pair in layers II-III of area 18. A, B,
Axonal (A) and dendritic
(B) arborization of the presynaptic
(black) and the postsynaptic
(gray) BCs is shown. The axon of the postsynaptic
cell was only partially recovered. C, The route of the
presynaptic axon (black) to synaptic boutons on the
postsynaptic cell (gray) is shown. Branch points
are indicated by asterisks. D, The
locations of electron microscopically verified synaptic junctions
between the two BCs are indicated. Four synapses were found on the
soma, and six synapses were on proximal dendrites. Three boutons
established two distinct synaptic release sites each
(grouped numbers). Ea, In response
to (Figure legend continues).
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Based on light microscopic appearance and its characteristic
postsynaptic target profile (85% on dendritic shafts; 15% on dendritic spines; n = 13 synapses), one neuron was
identified as a "dendrite-targeting cell" (DTC; Fig.
2). The description of other examples of
this cell type is given by Tamas et al. (1997a). The beaded dendrites
of this cell formed a radially elongated dendritic field (Fig.
2A), and its axonal cloud was composed of radially
running main trunks and thick, necklace-like collaterals that were
studded with large boutons that followed mainly arcadic or radial
routes. The DTC had a resting membrane potential of 64 mV and an
input resistance of 80 M and fired overshooting APs with a mean
amplitude of 81.8 mV.
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Figure 2.
Physiologically and anatomically identified
BC-to-DTC connection in area 17. The sketch and
numbers on the top of the figure
represent the synaptic and autaptic connectivity (straight
arrow, synaptic connection; round arrows,
autaptic connections) in the cell pair. A, Axonal
pattern of the presynaptic BC (black) and the dendritic
arbor of the postsynaptic DTC (gray) that was
located at the margin of the presynaptic axonal arbor are shown.
B, The axonal arbor of the postsynaptic DTC
(gray) did not overlap with the dendritic tree of
the presynaptic BC (black). C,
(Figure legend continues).
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The characteristic axonal arborization of two neurons spanned all
cortical layers in a horsetail-like manner (see Figs. 3, 5). Therefore,
these cells were identified as "double bouquet cells" (DBCs) (Ramon
y Cajal, 1894; Somogyi and Cowey, 1981; Tamas et al., 1997b). The
samples of postsynaptic target elements and the presence or absence of
autapses on the two cells were reported earlier (Tamas et al.,
1997b,c). In the present study, we deal with their connections with
other GABAergic cells, which have been analyzed since the previous
publications. Although both cells were classified as DBCs, they showed
a number of dissimilar characteristics and may thus represent subtypes
of the DBC class. The dendrites of cell 2402934 (see Figs. 5, 6) were
thin and unbeaded and had branching points relatively distal (up to
~100 µm) from the soma. In addition, the proximal dendrites
received characteristic invaginated asymmetrical synapses with a wide,
nonsynaptic membrane apposition between the dendrite and the
presynaptic terminals. The axon had small, thorn-like varicosities with
thin interbouton segments and targeted preferentially dendritic spines
and less frequently dendritic shafts [67.7 and 32.3%, respectively;
n = 31; data from Tamas et al. (1997a)]. In contrast,
the dendrites of the DBC 0812945 (Fig. 3)
were strongly beaded; they branched in the proximity of the soma and
did not receive invaginated type I synapses. Furthermore, the axon of
this cell formed larger terminals and thicker interbouton segments, and
dendritic shafts were more frequent in the target element sample than
in spines [62.5 and 37.5%, n = 24; data from Tamas et
al. (1997b)]. The DBCs 0812945 and 2402934 had resting membrane
potentials of 65 and 81 mV, respectively; the input resistance of
cell 0812945 was 30 M; and they fired APs with amplitudes of 66.5 and 88.2 mV, respectively.
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Figure 3.
Reciprocally connected BC-to-DBC pair in area 17. The sketch and numbers on the
top of the figure represent the synaptic and autaptic
connectivity (arrows) in the cell pair.
A, B, Axonal (A)
and dendritic (B) arborization of the presynaptic
BC (blue) and the postsynaptic DBC (red)
is shown. C, The route of axonal branches of the BC and
DBC to boutons establishing synaptic and autaptic junctions, all of
which were verified by electron microscopy, is shown. The BC innervated
the DBC through a single synapse (b-db) and formed eight
autaptic junctions (blue; a1-a8). One of
the autaptic terminals formed two separate synaptic junctions
(a2,3). The DBC established one synaptic junction on the
BC (db-b) and innervated itself via three autapses
(red; a1-a3). Note that when the release
sites formed by the BC are compared with those established by the DBC,
the former targeted proximal parts, whereas the latter innervated more
distal regions of the cell. D-F, Synaptic coupling
could be tested electrophysiologically from the BC to the DBC.
D, Action potentials (~1 Hz) of the BC
(Da) resulted in a short-latency IPSP
(Db) with a mean amplitude of 0.13 ± 0.53 mV
with the DBC being depolarized to a membrane potential of 57 mV.
E, Amplitude distributions of IPSPs and baseline noise
in the DBC show a slight shift of the IPSP distribution relative
to the noise. F, Brief trains of presynaptic APs
(Fa) elicited a summated response in the DBC
(Fb) at a membrane potential of 57 mV.
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Anatomical analysis of unitary interactions
Ten unitary connections were fully analyzed with correlated light
and electron microscopy. All of the synaptic links involved BCs, with
the latter innervating other BCs (n = 3 connections), DBCs (n = 3), and a DTC. In addition, we studied three
DBC-to-BC connections. In four out of five cell pairs, having fully
recovered axons and dendrites of both neurons, synaptic connections
were reciprocal. A total of 53 synaptic junctions could be verified between the recorded neurons, with the average number of release sites
per unitary connection being 5.3 ± 5.9. However, significant differences emerge when comparing the number and location of unitary synapses between particular directions of synaptic links (Table 1). The subcellular domain preference of
the presynaptic GABAergic cells was reflected in the differential
placement of unitary terminals on individual postsynaptic neurons.
Moreover, the autaptic self-innervation reported earlier (Tamas et al.,
1997c) is illustrated for several of the analyzed interactions (see
schematic presentation in Fig. 2 and illustrations in Figs. 3, 6); for
a more comprehensive description, see Tamas et al. (1997b).
BC-to-BC connections
A BC-to-BC pair (1412941; Figs. 1,
4) and the connectivity between two BCs
of a trineuronal network (2402934; Figs.
5-7)
provided evidence of monosynaptic interactions of neighboring
(~40-130 µm) BCs in the neocortex, as reported earlier for BCs at
larger lateral distances (Kisvarday et al., 1993). Reciprocity could be
tested and ascertained in only one of the cell pairs (2402934) because
of the inadequate axonal labeling of the postsynaptic BC of cell pair
1412941. Consistently, BC-to-BC (n = 3) interactions were the strongest of the cortical unitary interneuron-interneuron connections analyzed in this study. The number of synapses (Table 1)
between BCs was significantly higher than that in BC-to-DBC and/or
DBC-to-BC connections (p < 0.05 for both;
Mann-Whitney U test). The electron microscopically verified
synaptic junctions mediating BC-to-BC interactions were located either
on somata (n = 15) or on dendrites (n = 22), with their overall subcellular placement being significantly
closer to the soma than that in DBC-to-BC connections
(p < 0.0005; Mann-Whitney U test;
Table 1). In one instance (pair 1412941), four axonal branches
originated from the same 10th order collateral and innervated the
postsynaptic BC (Fig. 1C,D). Three presynaptic boutons
established four synapses on the soma (Figs. 1D;
numbers 1; 2,3; 4;
4Aa), four secondary dendrites were targeted by three
en passant boutons forming five synapses (Fig. 1D;
numbers 5,6; 7; 8,9), and one en
termineaux bouton formed a single synaptic junction (Figs.
1D; number 10; 4Ab). The
presynaptic terminals in the BC1-to-BC2 connection of the trineuronal
network were formed by 4th to 10th order axonal branches (Fig.
6Aa), and they targeted the soma (Fig.
6Ab; b6,7) and a secondary
(b5) and three tertiary (b1; b2,3;
b4) dendrites. In the reverse direction, sixth to
ninth order axon collaterals of BC2 (Fig. 6Ba)
terminated on the soma (Fig. 6Bb; b7-b15)
and on two primary (b1; b16), a secondary
(b4; b5), and four tertiary (b2,3;
b17; b18,19; b20) dendrites. The
analysis of BC-to-BC pairs underlined the importance of electron
microscopic (EM) examination of the connections. Without the complete
EM assessment of postsynaptic somata, the overall number of somatic
synapses would have been underestimated (p < 0.07). Light microscopic predictions of putative synaptic contacts
sites on dendrites were also unreliable (Table 1).
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Figure 4.
Electron microscopic evidence of synaptic
junctions between GABAergic neurons shown in Figures 1-3.
A, Synapses between the two BCs illustrated in Figure 1.
Aa, One of the two synaptic junctions
(arrow) established by a bouton (b2,3) of
the presynaptic BC on the soma (BCs) of the postsynaptic
BC is shown. Ab, An axonal terminal of the presynaptic
BC (b10) forms a synapse (arrow) on a
dendrite (BCd) of the postsynaptic BC. An unlabeled
terminal (t) also establishes a synaptic junction
(arrowhead). B, One of the two synaptic
junctions (arrow) formed by the same bouton
(b1,2) of the presynaptic BC on the soma of the
DTC illustrated in Figure 2. C, The two
synaptic junctions from the reciprocally connected BC-to-DBC pair shown
in Figure 3. Ca, A bouton (bc) of the BC
establishes a synapse (arrow) on a dendrite of the
DBC. Cb, In the reverse direction, a
bouton (dbc) of the DBC formed a synaptic junction
(arrow) on a dendrite of the BC. A
neighboring unlabeled terminal (t) also
established a synapse (arrowhead) on the postsynaptic
dendrite. The numbering of presynaptic boutons corresponds to that in
Figures 1D, 2D, and
3C, respectively. Scale bars, 0.2 µm, with
B and C at the same magnification.
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Figure 5.
Reciprocally interconnected network of two BCs and
a DBC in the medial bank of area 17. A, Light
microscopic reconstructions of the three interneurons [basket cell 1 (BC1), white soma and dendrites, green
axon; basket cell 2 (BC2), blue soma and dendrites,
pink axon; double bouquet cell, red soma
and dendrites, yellow axon] are shown.
Arrows indicate the identified directions of connections
(for details, see Figs. 6, 7); the numbers of synapses
are given in circles. Each cell was in reciprocal
connection with the other two, and the two BCs also innervated
themselves. For the display of overlapping axonal and dendritic
arborizations of the cells, layer III is shown expanded, maintaining
the position of layer I relative to the DBC and that of layers IV-VI
to the BCs. B, The topographically correct position of
dendritic trees is illustrated. C, D,
Functional synaptic coupling could be tested electrophysiologically in
only two directions. Action potentials (1-2 Hz) of BC1
(Ca) and BC2 (Da) resulted in
short-latency, fast IPSPs (Cb, Db) with
mean amplitudes of 0.59 and 0.70 mV in BC2 and DBC, respectively.
The latter were held at membrane potentials of 61 and 60 mV.
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Figure 6.
Route of axons to synaptic and autaptic boutons
and subcellular placement of synapses and autapses within the
trineuronal network established by two BCs and a DBC presented in
Figure 5. A-C, Within the network. a total of 70 synapses and autapses were identified with correlated light and
electron microscopy. Each panel shows a single
presynaptic axon and all dendritic branches innervated by the cell.
A, Synaptic and autaptic output of BC1.
Aa, The route of the axon to its identified targets is
shown (green). Ab, BC1 established
one somatic (white; a6) and seven
dendritic (a1-a5; a7,8) autapses,
innervated BC2 via seven synaptic junctions (blue; two
on the soma, b6,7; five on dendrites,
b1-b5), (Figure legend continues).
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Figure 7.
Examples of electron microscopically verified
synaptic and autaptic junctions within the trineuronal network of two
BCs and a DBC presented in Figures 5 and 6. A, Synaptic
and autaptic output of BC1. Aa, An axon terminal
(a7,8) of BC1 establishes two separate autaptic
junctions (arrows) on its own dendrite
(BC1). Ab, Two separate synaptic
junctions (arrows) between a bouton
(b6,7) of BC1 and the soma (BC2)
of BC2 are shown. Ac, A bouton (bd2) of
BC1 forms a synaptic junction (arrow) on a dendrite
(DBC) of the DBC. The convention of labeling presynaptic
boutons corresponds to that of Figure 6Ab.
B, Synaptic and autaptic output of BC2.
Ba, An axon terminal (a19) of BC2
establishes an autapse(Figure legend continues).
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The BC-to-DTC interneuron pair
The connection between the two layer IV neurons was found to be
unidirectional, both anatomically and physiologically. The postsynaptic
DTC was located at the margin of the BC axonal arborization, whereas
the axonal cloud of the DTC did not overlap with the dendritic arbor of
the BC (Fig. 2A,B). A single
terminal bouton formed by a 16th order collateral of the presynaptic
axon established two separate synaptic junctions on the basal pole of
the DTC soma (Figs. 2C,D,
4B).
BC-to-DBC interactions
The analysis of a BC-to-DBC pair (0812945; Figs. 3, 4) and the
connections from BC1 and BC2 to the DBC in the trineuronal network
(2402934; Figs. 5-7) showed that BCs innervate neighboring (~50-100
µm) DBCs. Reciprocity could be tested and verified for the three
BC-to-DBC cell pairs, all of which were located in layer III. As
indicated above, BC-to-DBC interactions were mediated by a
significantly smaller number of synaptic junctions than were BC-to-BC
connections (Table 1). Although all electron microscopically verified
synaptic junctions (n = 5) mediating BC-to-DBC
interactions were exclusively on dendrites, their distance, when
measured from the soma, was not significantly different from that of
BC-to-BC connections (p > 0.1; Table 1). In one
instance, an en passant bouton of a seventh order collateral of the
presynaptic BC (0812945; Fig. 3C) established a single
synaptic junction on a primary basal dendrite of the postsynaptic DBC
(Figs. 3C, 4). Both presynaptic terminals in the BC1-to-DBC
connection of the trineuronal chain were formed by an 11th order axonal
branch (Fig. 6Aa), and they targeted the same
secondary dendrite (Fig. 6Ab; bd1;
bd2). In the BC2-to-DBC connection of the trineuronal chain,
9th and 10th order axon collaterals of BC2 (Fig. 6Ba)
terminated on a tertiary and a secondary dendrite, respectively (Fig.
6Bb; bd1; bd2).
DBC-to-BC connectivity
The interconnectivity of the above DBC-to-BC pair (0812945; Figs.
3, 4) and the connections from the DBC to BC1 and BC2 in the
trineuronal network (2402934; Figs. 5-7) confirm that DBCs innervate smooth dendritic cells as well as pyramidal cells (Somogyi and Cowey,
1981) and indicate that DBCs and BCs are reciprocally connected. The
number of synaptic junctions mediating DBC-to-BC interactions was
significantly smaller than that for BC-to-BC connections (Table 1). In
addition, the electron microscopically verified synaptic junctions
(n = 9) mediating DBC-to-BC interactions were
exclusively on dendrites, and the distance of synapses, when measured
from the soma (two-dimensional projected distances), was significantly larger than that of release sites established by presynaptic basket cells (p < 0.0005; Table 1). In one instance,
an en passant bouton of a seventh order collateral of the DBC (0812945;
Fig. 3C) established a single synaptic junction on a fourth
order dendrite of the postsynaptic BC (Figs. 3C, 4), whereas
the presynaptic terminals in the DBC-to-BC1 connection of the
trineuronal chain were formed by fifth to ninth order axonal branches
(Fig. 6Ca), and they targeted three secondary dendrites
(Fig. 6Cb; white b1; b2;
b3-b4). Finally, six to ninth order axon collaterals of the
DBC (Fig. 6Ca) terminated on two secondary dendrites of BC2
(Fig. 6Cb; blue b1-b3; b4).
Physiological properties of the recorded interactions
From 10 of the anatomically reconstructed connections described
above, a total of five could be physiologically tested, and in each
case, action potentials evoked in the presynaptic interneuron evoked a
unitary IPSP in the postsynaptic cell. All of the synaptic effects were
elicited by presynaptic BCs (n = 5) and recorded in
postsynaptic interneurons, being comprised of two BCs (Figs. 1, 5), a
DTC (Fig. 2), and two DBCs (Figs. 3, 5).
Kinetics of unitary IPSPs
All presynaptic BCs elicited short-latency (<1.5 msec) IPSPs,
with fast rise and decay kinetics, regardless of the postsynaptic cell
type (Figs. 1E, 2E, 3D,
5C,D). Reversal potentials, indicating that
chloride was probably the major charge carrier, were 66.9 mV for a
postsynaptic BC (1412941; Fig. 1) and 72.9 mV for the DTC (Fig. 2),
as extrapolated from hyperpolarizing IPSPs measured at membrane
potentials ranging from 58 to 49 mV and 76 to 44 mV,
respectively. Apart from the IPSP elicited by the BC in the DBC (Fig.
3), the decay phase of unitary IPSPs (n = 4) could be adequately fitted with a single exponential function, with a mean time
constant of 5.6 ± 1.6 msec (range, 3.4-7.0 msec) being similar to the decay time constant of somatically injected current pulses (5.9 ± 3.4 msec; range, 3.6-11.6 msec; p = 0.46). Unitary mean IPSP conductances could be calculated for a
BC-to-BC (1412941; n = 10 synapses) and the BC-to-DBC
(n = 2 synapses) interaction and were 5.735 and 0.373 nS, respectively [for details, see Ginsborg (1973) and Benardo
(1994)]. Although we have not obtained pharmacological evidence, the
kinetics of unitary IPSPs evoked in both pyramidal (Tamas et al.,
1997b) and smooth dendritic neurons is compatible with the properties
of GABAA receptor-mediated synaptic responses (Avoli, 1986;
Connors et al., 1988; Benardo, 1994; Deuchars and Thomson, 1995).
Average IPSP amplitudes were 919 ± 863 µV (n = 5) and varied from 133 to 2397 µV at membrane potentials ranging
between 46 and 61 mV (mean ± SD, 55.0 ± 6.4 mV). The
IPSPs elicited in BCs and in DBCs had an average amplitude of 1522 and
419 µV, respectively (for individual measurements, see Figs. 1, 3,
5), and the mean amplitude of the IPSP in the DTC was 771 µV (Fig.
2). There was no significant correlation between the postsynaptic
membrane potential and the amplitude of the IPSPs (r = 0.60; p = 0.23; Spearman correlation). There was a
trend for unitary IPSP amplitudes to increase with the number of
synaptic release sites mediating the interaction, although the
correlation was not significant (r = 0.67;
p = 0.18; Spearman correlation). There were no obvious
differences for different types of connections in the rise and decay
kinetics of unitary IPSPs. Unitary IPSPs had a mean 10-90% rise time
of 1.51 ± 0.53 msec (range, 1.12-2.27 msec)
and, measured at half-amplitude, a duration of 6.66 ± 1.24 msec
(range, 5.03-8.00 msec).
Amplitude distribution of unitary IPSPs
At each interaction tested (n = 3), the amplitudes
of unitary IPSPs fluctuated to some degree, although a significant
portion of this variability may have been originating from the
recording noise (see below). Generally, the amplitude of individual
events fluctuated around the average of the postsynaptic response (Fig. 1Ec,d). For further analysis, amplitude histograms of
unitary IPSPs and the corresponding baseline noise were constructed for those cases in which the number of unitary IPSPs was higher than 100 and the postsynaptic response remained stationary (Figs.
1F, 2F, 3E). In those
three interactions, the mean ratio of IPSP amplitude and noise
variances was 1.9 ± 1.2, ranging from 0.9 to 3.3. The overlap
between the signal and noise distributions decreased with the
increasing number of synaptic junctions mediating the events, with the
absence of such overlap indicating the complete absence of transmission
failures in the connection mediated by 10 release sites between two BCs
(Fig. 1). Moreover, the absence of a distinct peak around the zero
amplitude level suggests few, if any, response failures in a connection
mediated by two synaptic junctions (Fig. 2, BC-to-DTC).
Response summation and use-dependent depression of
unitary IPSPs
Unitary IPSP summation and use-dependent depression could be
observed in the DTC when investigating the postsynaptic effect of
high-frequency trains of action potentials elicited in the presynaptic
BC (Fig. 2G). Summation of the initial two IPSPs increased the amplitude of single action potential-evoked events by 43%. Although the presynaptic firing frequency remained constant, the response gradually declined to a relatively stationary level ~53% of
the maximum of the summed response. In comparison with single action
potential-evoked events, the decay phase of a tetanically (17-18 APs)
evoked unitary IPSP was somewhat prolonged (decay time constant = 17.1 msec).
To investigate more systematically the effect of activity preceding
evoked responses, we applied a paired-pulse (PP) protocol by adjusting
the depolarizing current pulse in the presynaptic cell to eliciting two
action potentials only. Such data were obtained in two of the
connections (Figs. 1, BC-to-BC, 2, BC-to-DTC). Interspike intervals
were varied either by adjusting the current intensity or by delivering
two successive current pulses and ranged from 10-28 and 14-200 msec
in the BC-to-BC and BC-to-DTC connections, respectively. The mean
amplitudes of second IPSPs (IPSP2s) were 83 and 79% (mean = 81%)
of the corresponding conditioning first events, thus revealing
statistically significant PP depression of both connections
(p < 0.05) at mean interspike intervals of 15.0 ± 5.8 and 83.1 ± 63.7 msec, respectively. The overall
decrease of mean IPSP2 amplitudes was accompanied by an increase of the measured response variability, because the coefficient of variation (CV) of IPSP2s were 146 and 119% of the CV of the respective
conditioning events (IPSP1s). Amplitude histograms showed a general
shift of the distribution toward smaller amplitudes and a greater
overlap with the noise measurements, suggesting a larger proportion of postsynaptic response failures (Fig. 2I). When the
amplitudes of second IPSPs were plotted against those of the preceding
events (data not shown), a statistically significant negative
correlation was found in the BC-to-BC interaction (r = 0.49; p < 0.01; Pearson's r table); thus
large IPSP1s were followed more frequently by large IPSP2s and vice
versa (Fig. 1Gc,d). This trend was not apparent in the
BC-to-DTC connection (r = 0.06; p > 0.25; Fig. 2Ha). To assess the influence of the
magnitude of the conditioning IPSP, single traces were presorted
according to the amplitude IPSP1, separated into groups, and averaged.
Finally, for each of the groups, the corresponding PP ratio was
calculated, here taken as the ratio of averaged second IPSPs and the
mean conditioning IPSP (i.e., the average of all first IPSPs). A value
>1 would thus indicate the presence of PP facilitation, i.e., the
second IPSP amplitude exceeding that of the mean conditioning first
IPSP [for EPSPs, see Buhl et al. (1997)]. In the BC-to-BC connection, PP depression (PP ratio = 0.69) was apparent after IPSP1s smaller than 2 mV in amplitude (Fig. 1Gc) but not after IPSP1s
larger than 2 mV (PP ratio = 1.00; Fig. 1Gd), i.e.,
large conditioning events decreased the degree of PP depression. The
BC-to-DTC connection showed a similar trend, with PP ratios for
conditioning events that were either smaller than 1 or larger than 1.5 mV being 0.71 and 0.86, respectively (p < 0.02;
Fig. 2Ha). For this connection, individual trials
were also sorted with respect to the interspike interval and averaged.
At all intervals tested, presorted and averaged EPSP2s were compared
with the mean of the corresponding conditioning first events. It was
apparent that PP depression predominated and PP ratios were 0.74, 0.78, and 0.90 at intervals of 14-25, 100, and 200 msec (Fig.
2Hb). For each temporal increment, a prolongation of the
interspike intervals was associated with a statistically significant
increase of the PP ratio (p < 0.025).
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DISCUSSION |
This study demonstrates that neocortical GABAergic neurons receive
GABAergic input from several distinct local sources and that, in
addition to the innervation of spiny cell populations, individual
GABAergic cells direct their output toward several classes of smooth
dendritic cells. Intracolumnar reciprocal connections commonly occur
between GABAergic neurons with similar and dissimilar efferent
connectivity, and the intrinsic GABAergic interconnectivity is boosted
by a high incidence of autaptic self-innervation.
Interneuron-to-interneuron connections are heterogeneous, regarding
both the number and subcellular placement of unitary synapses. Synapses
between BCs are more numerous and located closer to the soma than are
synapses mediating BC-to-DBC or DBC-to-BC interactions. Regardless of
the postsynaptic target neuron, BCs evoke fast IPSPs in a reliable
manner, particularly when mediated by several release sites. These
results suggest a prominent role for BCs in governing the activity of
local GABAergic neuronal circuits and, because of
their divergent output, in linking excitatory and
GABAergic networks.
Differential patterns of interconnectivity in
GABAergic networks
We demonstrated that neocortical interneurons innervate other
GABAergic cells via 1-20 electron microscopically verified synaptic junctions. Although the present sample is relatively small, significant differences emerged regarding connections between interneurons with
distinct efferent target preferences; BCs innervated each other through
a number of unitary release sites that is among the highest in the
cortex, but BC-to-DBC and DBC-to-BC connections were mediated by a
smaller number of synapses. The interconnections among a subclass of
BCs was also noted from immunocytochemistry for cholecystokinin (Freund
et al., 1986). The high incidence of autapses on BCs and on DTCs (Tamas
et al., 1997c), the extensive interconnectivity between large BCs
(Kisvarday et al., 1993), and the perisomatic concentration of
symmetric synapses on layer IV basket cells (Freund et al., 1983; Ahmed
et al., 1997) suggest a powerful GABAergic influence on BCs.
Interactions between hippocampal BCs show a similar trend (Nunzi et
al., 1985; Sik et al., 1995; Cobb et al., 1997). Therefore, BC-to-BC
interactions probably constitute a special link in the cortical
network. Alternatively, the possibility may exist that there are
preferential interconnections among all interneurons of the same type.
Because of the large number of cell types that remain untested for
potential interconnections within a class, this scenario cannot be
excluded but seems unlikely.
If we assume that all neurons in the axonal field of an interneuron
(n = 1272 ± 414) are uniformly innervated, each
postsynaptic cell would receive on average 4.31 ± 1.28 unitary
GABAergic synapses, regardless of the presynaptic cell type (Tamas et
al., 1997b). This value is well below that obtained for BC-to-BC pairs
in this study and is in the upper range of the pooled BC-to-DBC and
DBC-to-BC data. Therefore, it seems that within their axonal field BCs
preferentially innervate other BCs. The overall degree of target cell
selectivity could be even higher for large BCs, having a large,
low-density axonal field (Somogyi et al., 1983; Kisvarday et al.,
1993). Because we anatomically scrutinized all possible interactions
for the number of synapses and detected physiologically connections
with one or two release sites, the possibility is unlikely that our recordings were strongly biased for sampling larger IPSPs.
The BC-to-DTC pair also stresses the potential importance of the
relative position of connected cells, because the postsynaptic DTC was
located at the edge of the presynaptic axonal field, which may also
explain the relatively small number of synapses. However, we
demonstrated previously that pyramidal cells located at the periphery
of the presynaptic axonal cloud of BCs can receive a high number
(n = 15) of unitary synapses (Tamas et al., 1997b). In
addition, Kisvarday et al. (1993) found that long-range intercolumnar connections exist between large BCs and other BCs. They observed four
to six synapses formed by presynaptic large BCs on
parvalbumin-immunoreactive perikarya; thus, extrapolating from the
somatodendritic distribution ratio of synapses between BCs presented in
this study, the total number of unitary synapses established by large
BCs would be in the range of 10-14 on parvalbumin-positive cells, a
value that is close to the mean number of synapses between small BCs
presented above. Hence the degree of interconnectivity seems to be
governed by the identity of the postsynaptic cell and not by its
physical position within the presynaptic axonal field.
The relatively high number of transmitter release sites seems to
restrict the number of postsynaptic response failures. Thus, transmission at BC-to-BC connections remains reliable, even if the
release probability were relatively low. If we assume binomial release
statistics, an average of 12 release sites, and a uniform release
probability (p) of ~0.3 [inhibitory input onto
goldfish Mauthner cell (Korn et al., 1982)], the statistical
likelihood for all terminals failing to release transmitter would be
small (p ~ 0.01). If the same conditions were
to apply for BC-to-DBC or DBC-to-BC connections with a mean number of
unitary synapses in the range of two, the probability of failures would
be as high as 0.49. In view of the absence of a distinct failure peak
in the analyzed BC-to-DTC connection, the latter estimate seems to be
too high, and the release probability may thus be appreciably higher
than that in the case of the Mauthner cell. Hence a high probability of
release at cortical GABAergic synapses may serve to ensure a reliable
transmission within interneuronal networks.
Subcellular segregation of unitary synapses on
GABAergic neurons
Similar to BC-to-pyramid connections (Somogyi et al., 1983;
Kisvarday et al., 1985; Thomson et al., 1996; Tamas et al., 1997b), BCs
were found to establish synaptic junctions significantly closer to the
soma of postsynaptic GABAergic cells than to that of DBCs. Before the
current study, the only unitary interaction between two GABAergic
neurons that had been fully analyzed with electron microscopy also
demonstrated subcellular domain-specific innervation of a hippocampal
bistratified cell by a presynaptic basket cell (Cobb et al., 1997).
Moreover, autapses on BCs are also located more proximal to the soma
than are autapses established by DTCs (Tamas et al., 1997c). Such a
high degree of domain specificity implies functional differences
between synapses formed by perisomatically versus dendritically
terminating interneurons in controlling the activity of other GABAergic
cells. In pyramidal cells, perisomatic GABAergic synapses may control
the generation of APs (Buhl et al., 1995; Miles et al., 1996) and can
play a role in phasing neuronal activity (Cobb et al., 1995).
Conversely, GABAergic synapses on dendrites can prevent calcium spikes
(Traub et al., 1994; Miles et al., 1996) and have been proposed to
interact with backpropagating APs (Buzsaki et al., 1996; Tsubokawa and
Ross, 1996). An additional explanation for the spatial segregation of
GABAergic inputs may be their pairing with excitatory afferents as
found in the hippocampus (Gulyas et al., 1993; Halasy and Somogyi,
1993; Vida et al., 1998) and proposed for the neocortex (Kisvarday et
al., 1985; Tamas et al., 1997b).
A role for reciprocally interconnected GABAergic neurons to govern
oscillatory network activity
The high degree of reciprocity and the extent of differential
interconnectivity emphasize specificity as well as differentiation in
interneuronal networks of the cerebral cortex. In this web, mutually
connected interneurons may control spatial and temporal features of
inhibition. When linking two GABAergic neurons into a simple serial
circuit, this may result in a disinhibitory effect downstream. However,
such a simple formula is insufficient to explain the net effect of
reciprocally and widely interconnected GABAergic neurons. Recently, a
putative functional role for interneuronal interconnections emerged
from both experimental and modeling data, showing that, even in the
absence of fast glutamatergic neurotransmission, interconnected
GABAergic neurons can generate synchronous 40 Hz network oscillations,
provided the degree of synaptic interconnectivity/conductance between
cells is sufficiently high (Whittington et al., 1995; Traub et al.,
1996; Wang and Buzsaki, 1996). Our data confirm the results of
Kisvarday et al. (1993) and clearly favor the web of strongly
interconnected BCs to provide an adequate substrate for such
synchronous network activity. This notion is experimentally supported
by in vivo recordings from the rat hippocampus,
demonstrating BCs to discharge in short, theta-modulated bursts at
gamma frequencies (Ylinen et al., 1995). In addition, data presented
above show that BCs generate fast, presumably GABAA
receptor-mediated synaptic responses in other interneurons, which could
be sustained at relatively fast frequencies in the range of and above
the gamma frequency band. Such fast IPSPs may then, in turn, entrain a
network of tonically excited and mutually connected BCs at gamma
frequencies (Buzsaki and Chrobak, 1995; Jefferys et al., 1996). Indeed,
during visual stimulation, oscillatory synaptic membrane potential
changes have been noted in intracellularly recorded neurons of the cat visual cortex (Jagadeesh et al., 1992), although the spiking activity of putative BCs may not necessarily be periodic (Azouz et al., 1997).
Simulations of the coordinated firing of several neocortical GABAergic
neurons providing a perisomatic innervation pattern, namely BCs and
axoaxonic cells, indicated that they are well suited to entrain
principal cell activity in the gamma frequency range (Lytton and
Sejnowski, 1991). However, because axoaxonic cells do not innervate
other GABAergic neurons (see Somogyi, 1989), it thus seems that BCs,
because of their divergent innervation of both interneurons and
principal cells, are uniquely suited to correlate the activity pattern
of inhibitory and excitatory cortical neurons. Recordings of BCs and
their postsynaptic target neurons in an oscillating network will be
required to ascertain their role in the induction and maintenance of
cortical network oscillations.
| |
FOOTNOTES |
Received Dec. 16, 1997; revised March 12, 1998; accepted March 18, 1998.
This project was supported by European Community Grant BIO4-CT96-0585.
G.T. was supported by the Oxford-Szeged Scholarship of the Department
of Pharmacology, the European Blaschko Visiting Research Scholarship,
and the Z. Magyary Scholarship. E.H.B. also holds a Medical Research
Fellowship at Corpus Christi College, Oxford. We thank Drs. O. Paulsen
and Z. Nusser for critical comments on an earlier version of this
manuscript and P. Jays, F. Kennedy, and J. D. B. Roberts for
technical and photographic assistance.
Correspondence may be addressed to any of the authors. Reprint requests
should be addressed to Dr. Gábor Tamás, Medical Research
Council, Anatomical Neuropharmacology Unit, University of Oxford,
Mansfield Road, Oxford, OX1 3TH, UK.
| |
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Abstract
Introduction
