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The Journal of Neuroscience, May 1, 1998, 18(9):3386-3403
NOTE: In this article, the following sentence
"The estimated ratio of interneurons versus principal
cell targets of the mossy fiber is 1:4 to 1:6," should read, "The estimated
ratio of interneurons versus principle cell targets of the mossy fiber is
4:1 to 6:1." A printed correction will appear in a later issue of the journal.
GABAergic Cells Are the Major Postsynaptic Targets of Mossy
Fibers in the Rat Hippocampus
László
Acsády1, 2,
Anita
Kamondi1,
Attila
Sík2,
Tamás
Freund2, and
György
Buzsáki1
1 Center for Molecular and Behavioral Neuroscience,
Rutgers, The State University of New Jersey, Newark, New Jersey 07102, and 2 Institute of Experimental Medicine, Hungarian Academy
of Sciences, H-1450 Budapest, Hungary
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ABSTRACT |
Dentate granule cells communicate with their postsynaptic targets
by three distinct terminal types. These include the large mossy
terminals, filopodial extensions of the mossy terminals, and smaller
en passant synaptic varicosities. We examined the postsynaptic targets of mossy fibers by combining in
vivo intracellular labeling of granule cells,
immunocytochemistry, and electron microscopy. Single granule cells
formed large, complex "mossy" synapses on 11-15 CA3 pyramidal
cells and 7-12 hilar mossy cells. In contrast, GABAergic interneurons,
identified with immunostaining for substance P-receptor, parvalbumin,
and mGluR1a-receptor, were selectively innervated by very thin
(filopodial) extensions of the mossy terminals and by small en
passant boutons in both the hilar and CA3 regions. These
terminals formed single, often perforated, asymmetric synapses on the
cell bodies, dendrites, and spines of GABAergic interneurons. The
number of filopodial extensions and small terminals was 10 times larger
than the number of mossy terminals. These findings show that in
contrast to cortical pyramidal neurons, (1) granule cells developed
distinct types of terminals to affect interneurons and pyramidal cells
and (2) they innervated more inhibitory than excitatory cells. These
findings may explain the physiological observations that increased
activity of granule cells suppresses the overall excitability of the
CA3 recurrent system and may form the structural basis of the
target-dependent regulation of glutamate release in the mossy fiber
system.
Key words:
granule cell; mossy fiber; interneuron; spine; dentate
gyrus; in vivo
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INTRODUCTION |
A unique neuron type of cortical
structures is the dentate granule cell of the archicortex. Granule
cells receive most of their extrinsic input from layer II neurons of
the entorhinal cortex and convey neocortical representations to the
recurrent system of the hippocampal CA3 region by way of their axons,
known as mossy fibers (Ramón y Cajal, 1911 ; Steward and Scoville,
1976; Claiborne et al., 1986). Collaterals of the same
entorhinal afferents also directly innervate the distal dendrites of
CA3 pyramidal cells (Steward and Scoville, 1976). The entorhinal
projections to both granule cells and CA3 cells are very divergent. In
contrast, a single granule cell contacts only a few dozen hilar mossy
cells and CA3 pyramidal cells, and the convergence of granule cells on
their principal cell targets is similarly limited (Amaral et al.,
1990). The target mossy cells and CA3 pyramidal cells provide a highly
divergent feedback excitation to the granule cells (Li et al., 1994;
Scharfman, 1994; Soriano and Frotscher, 1994; Buckmaster et al., 1996).
Despite these excitatory loops, activation of the entorhinal-granule
cell network appears to exert an overall suppressive effect on CA3
pyramidal neurons (Bragin et al., 1995a,b; Penttonen et al., 1997) as
opposed to the overall excitatory effect of the CA3 recurrent network
on all other regions of the hippocampal formation (Chrobak and
Buzsáki, 1996; Penttonen et al., 1997). The possible anatomical
basis of this functional suppression might be a strong feed-forward
activation of inhibitory interneurons by granule cells (Frotscher,
1985, 1989; Gulyás et al., 1992; Deller et al., 1994).
The physiological effects of granule cells on interneurons are
different from those on principal cells (Miles, 1990; Scharfman et al.,
1990; Livsey and Vicini, 1992; Jonas et al., 1993; Geiger et al., 1997;
Maccaferri et al., 1998). Whether this difference is reflected in the
structure of excitatory terminals or in the number of release sites on
different postsynaptic cell types has yet to be demonstrated.
Interestingly, Ramón y Cajal (1911) noted a unique feature of
mossy fibers: that unlike any other cortical principal cell, granule
cells have more than one terminal type along their axons. In addition
to the well known mossy terminals, which form intricate multiple
contacts with principal cells (Blackstad and Kjaerheim, 1961; Chicurel
and Harris, 1992), small terminals and filopodial extensions of the
mossy terminals have also been described (Ramón y Cajal, 1911).
More recently, these various smaller extensions of the mossy fibers
were also identified as presynaptic terminals (Amaral, 1979; Claiborne
et al., 1986). Although the small terminals may outnumber the well
characterized large mossy terminals, identification of their
postsynaptic targets has not been attempted to date.
In the present study, we combined in vivo intracellular
labeling of granule cells with immunocytochemistry and electron
microscopy to answer the following questions. Are the different types
of axon terminals associated with different postsynaptic neuronal populations? Is the proportion of principal cells versus inhibitory interneurons innervated by a single granule cell similar to or different from that in other cortical networks? What kind of
interneurons are innervated by the granule cells? Do neighboring
granule cells share common principal and interneuron targets? Are the
number of neurotransmitter release sites similar on the different
neuronal targets? We attempted to answer these questions quantitatively within the limits afforded by the single cell labeling and
immunocytochemical methods.
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MATERIALS AND METHODS |
Surgery and recording. Twenty-one rats of the Sprague
Dawley strain (250-350 gm) were anesthetized with urethane (1.3-1.5 gm/kg) and placed in a stereotaxic apparatus. The body temperature of
the rat was kept constant by a thermoregulation device. The scalp was
removed and a small (1.2 × 0.8 mm) bone window was drilled above
the hippocampus (anteromedial edge at anterioposterior =  3.3;
lateral = 2.2 mm from bregma) for extra- and intracellular recordings. Details of surgery and electrode placement have been published previously (Penttonen et al., 1997). Briefly, glass micropipettes for intracellular labeling were pulled from 2.0 mm
capillary glass. They were filled with 1 M
K+-acetate in 50 mM Tris buffer, pH 7.2, also containing 2% biocytin for intracellular labeling. After the
recording pipette was inserted into the brain, the bone window was
covered by a mixture of paraffin and paraffin oil to prevent drying of
the brain and to decrease pulsation. Once a stable intracellular
recording was obtained, evoked and passive physiological properties of
the cell were determined (Axoclamp-2B; Axon Instruments, Foster City,
CA). After the completion of the physiological data collection
(Penttonen et al., 1997), biocytin was injected through a
bridge circuit using 500 msec depolarizing pulses at 0.4-0.7 nA at 1 Hz for 10-60 min. Neuronal activity was followed throughout the
procedure, and the current was reduced if the electrode was blocked and
the condition of the neuron had deteriorated. In some cases small
spikelets were recorded in addition to the regular large amplitude
action potentials. In all of these cases histological analysis revealed
multiple labeling of granule cells (two or three neurons). These
artificially labeled cells were also included in this study, because
they provided an opportunity to examine the topography and convergence
of mossy fibers of nearby granule cells.
Histological analysis. Two to twelve hours after the
biocytin injection, the animals were given an overdose of urethane and then perfused intracardially with physiological saline followed by 400 ml fixative containing 4% paraformaldehyde dissolved in 0.1 M phosphate buffer (PB), pH 7.4 (fixative A). In four
cases, after the saline the animals were perfused with 60 ml fixative containing 3.75% acrolein and 2% paraformaldehyde (5 min) in 0.1 M PB and then with 300 ml 2% paraformaldehyde in 0.1 M PB (fixative B). The brains were then removed and stored
in the fixative solution overnight. Coronal sections (40 or 60 µm
thick) were cut from the hippocampus on a Vibroslice, washed,
cryoprotected in 30% sucrose in 0.1 M PB overnight, and
freeze-thawed in aluminum foil boats over liquid nitrogen. The sections
were treated with 1% sodium borohydride when fixative B was used.
After extensive washes first in PB and then in Tris-buffered saline
(TBS), pH 7.4, the sections were incubated in avidin-biotin
horseradish peroxidase complex (ABC, Vector Laboratories, Burlingame,
CA) (1.5 hr, 1:150). Biocytin labeling was visualized by
nickel-intensified 3,3'-diaminobenzidine-4HCl (DAB) (Sigma, St. Louis,
MO) as a chromogen, which resulted in a black reaction product. The DAB
solution contained ammonium chloride (0.4%) to reduce background. The
sections were then treated with 1% OsO4 in 0.1 M PB for 45 min, dehydrated in ethanol and propylene oxide,
and embedded in Durcupan (ACM, Fluka; Neu Ulm, Germany).
Three-dimensional reconstruction of the main axons was accomplished in
four cases using motorized microscope stage and the program NeuroLucida
(MicroBrightfield, Colchester, VT) or in another three cases using the
program Arbor (S. Pomaházi and A. I. Gulyás, Budapest,
Hungary). The latter creates a pseudo three-dimensional image from
camera lucida drawings. After the reconstruction of the axon, its
length and the distances between mossy terminals in the
three-dimensional space were determined. Long mossy fiber segments,
parallel to the surface, were selected and re-embedded for further
electron microscopic examination. Serial ultrathin sections were cut
with a Reichert ultramicrotome and examined with a Philips CM 10 or
Hitachi 7100 electron microscope.
Immunostaining procedure. For the examination of the axonal
targets of the filled granule cells, the sections were not dehydrated after the first ABC reaction but were processed with additional antibodies. To reduce nonspecific staining, the sections were incubated
with 10% normal goat serum (Vector Laboratories) for 40 min. Rabbit
anti-substance-P (SPR) (1:3000; gift of Dr. R. Shigemoto; four cases)
(Shigemoto et al., 1993;), rabbit anti-parvalbumin (1:2000; gift of Dr.
K. G. Baimbridge; two cases) (Baimbridge and Miller, 1982), rabbit
anti-calretinin (1:5000; gift of Dr. J. H. Rogers; one case)
(Rogers, 1989), or mouse anti-metabotropic glutamate receptor 1a
(mGluR1a 1:10; gift of Dr. T. Görcs; one case) was used as
primary antisera for 2 d. The second layer was biotinylated
anti-rabbit IgG made in goat or biotinylated anti-mouse IgG made in
horse (Vector Laboratories) (1:200; 6 hr) followed by ABC (Vector
Laboratories) (overnight; 1:200). All washes and dilutions of antisera
were performed in 0.05 M Tris-buffered saline (TBS), pH
7.4. The immunoperoxidase reaction was developed with DAB as a
chromogen, resulting in a brown reaction product. Replacement of the
primary antisera with normal sera of the animals, in which the primary
antisera were raised, resulted in lack of immunostaining. Next, the
sections were treated with 1% OsO4 (containing 7% glucose to preserve color difference) in 0.1 M PB for 45 min,
dehydrated in ethanol and propylene oxide, and embedded in Durcupan
(ACM, Fluka, Buchs, Switzerland). The axon terminals of the granule cells and their close appositions with a flat surface toward a target
soma, dendrite, or spine (i.e., putative synapses) were examined under
a 100× oil immersion objective. In several cases, the dendritic tree
of the putative postsynaptic target(s) was also reconstructed to
determine the number of contacts with a single postsynaptic neuron and
to measure the distance of the contact from the soma. Correlated light
and electron microscopy were used in 42 cases to verify the synaptic
specialization between the labeled profiles.
The size of presynaptic terminals of granule cells on their GABAergic
target neurons was examined by pre-embedding gold immunostaining for
dynorphin (a marker of mossy fibers and terminals) (McLean et al.,
1987; Drake et al., 1994) combined with pre-embedding DAB reaction for
SPR (p = 3 rats). Sections were incubated first with rabbit anti-dynorphin antibody (1:8000; Peninsula Labs) followed by anti-rabbit antiserum conjugated to 1 nm gold particles (1:40; overnight) (Amersham, Little Chalfont, UK). The colloidal gold was
visualized by IntenS EM Silver Enhancement Kit (Amersham), and the
reaction was terminated by 1% sodium thiosulfate and fixed with 1%
glutaraldehyde for 10 min. The sections were processed further for SPR
immunocytochemistry as described above. In the electron microscope, the
end product of the pre-embedding immunostaining appeared as
high-contrast electron-dense granules, whereas the reaction product of
DAB was less electron dense and homogeneously filled the profiles.
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RESULTS |
The passive and synaptic properties of the intracellularly
recorded granule cells have been reported previously (Ylinen et al.,
1995; Penttonen et al., 1997). Figure 1
illustrates the dendritic arbor of a biocytin-filled granule cell and
its local axon collaterals in the hilar region. Both large mossy
terminals and various small terminals could be visualized as described
before in Golgi preparations (Ramón y Cajal, 1911) and in
vitro studies (Claiborne et al., 1986). The terminology of Lorente
de Nó (1934) and Amaral (1978) is used in this paper. Axon
trajectories, terminal specializations, and postsynaptic targets of
labeled granule cells will be described first in the CA3 region,
followed by a similar description in the hilus.
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Figure 1.
Granule cell filled with biocytin in
vivo. The cell was first developed for biocytin and
photographed, and the image was fused with the cresyl violet-stained
image of the same section. Arrow indicates mossy fiber;
white arrowheads indicate local collaterals in the hilar
region. m, Molecular layer; g, granule
cell layer; h, hilus; CA3, pyramidal
layer of CA3c. Top inset, Current-voltage responses of
the granule cell to hyperpolarizing (0.8, 0.6, and 0.4 nA) and
depolarizing (0.7 and 0.8 nA) current steps. Bottom
inset, High magnification of a mossy terminal
(arrow) in the hilar region. Double
arrowhead indicates filopodial extension; white
arrowheads indicate small en passant and
drumstick-like boutons. Scale bar, 10 µm.
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Axonal trajectory of the main mossy fiber
A total of 28 granule cells with significant axonal labeling were
included in this study. In 14 cases the axon arbor was judged as
complete. Criteria for complete axonal labeling were twofold: the
appearance of (1) sharp endings of all side branches without fading
within the section and (2) terminal-like swelling (bouton) at the end
of each axon branch. The average three-dimensional length of the main
axon of granule cells, the "mossy" fiber, was 3236 ± 72 µm
(SE; n = >7 cells), of which 802 ± 21 µm was
in CA3c (hilar), 1051 ± 15 µm was in CA3b (ventricular), and
1396 ± 91 µm was in CA3a (fimbrial). Regardless of the position
of the parent cell body (dorsal blade, ventral blade, tip or crest of
the granule cell layer), the main axon trunk traveled septally in the
CA3c and CA3b subregions, turned caudally at the distal end of CA3b, and followed a caudal route in CA3a (Fig.
2), as suggested by previous bulk
injections and Golgi-staining studies (Ramón y Cajal, 1911;
Swanson et al., 1978; Amaral and Witter, 1989). The septotemporal span of the main axon in the coronal plane was 1.1 ± 0.5 mm (n = 12; 0.9 ± 0.05 mm septal
and 0.2 ± 0.05 mm caudal to the cell body). The largest septal
extension (1.3 mm) was measured in a granule cell with its cell body
sitting in the crest region. In contrast, the axon trunk of granule
cells situated at the tip of the dorsal blade had the shortest septal
route and terminated most caudally. In general, mossy fibers followed
the transversal axis of the hippocampus in the CA3c-b regions but ran
along the longitudinal axis in area CA3a (Fig. 2). Thus, the mossy
fiber system could be considered "lamellar" (Amaral and Witter,
1989) only in the CA3c-b regions. In area CA3a the mossy axons ran
perpendicular to the "lamellae."
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Figure 2.
Topography of the mossy fibers in the CA3 region.
A, Camera lucida drawing of mossy fibers of three
adjacent (multiple-labeled) granule cells. Note numerous filopodial
extensions of the large mossy terminals in A
(arrowheads) and thin stalks of large mossy terminals
(arrows). Boxed area in
inset in A shows the position of the
fibers at the CA3c-CA3b border. B, NeuroLucida
reconstruction of the same three axons shown in A
(diamonds, triangles, and squares label
mossy terminals) and an additional mossy fiber of a fourth granule cell
(circles) located posterior to the triple-labeled
neurons. The original coronal images are rotated to emphasize the
spatial characteristics of the fibers. In the transversal view
(left), fibers are visible only in CA3c
and CA3b, because in CA3a they run
perpendicular to this plane. In the dorsal view (right),
the entire semicircular route of the mossy fibers can be followed. Note
the parallel organization of the fibers. Insets show the
angles of view (arrows) on a coronal block.
D, Dorsal; A, anterior; L,
lateral. C, Wire diagram of the three mossy fibers shown
in A (two of them are considered as complete) depicting
the distribution of mossy terminals. Note that shorter interbouton
distances prevail in the CA3c subregion. Scale bars: A,
50 µm; B, 400 µm; C, 200 µm.
str.luc., Stratum lucidum; str.pyr.,
stratum pyramidale.
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Most mossy fibers ran in stratum lucidum and only occasionally
penetrated the CA3c pyramidal layer. Apart from one occasional side
branch in CA3c, which joined the hilar plexus (see below) and short,
thin stalks with a mossy terminal (Fig. 2A), mossy fibers did not have branchpoints along their length. When neighboring granule cells were labeled, their axons followed a relatively parallel
route (Fig. 2). The distance between the axons of neighboring granule
cells varied between 50 and 300 µm. Adjacent or nearby mossy boutons
(< 50 µm) from two or more axons were never observed (p = 58 boutons). Given the diameter of the the
apical dendrite of CA3 pyramidal cells (p < 10 µm), these findings indicated that the probability that adjacent
granule cells innervate the same or nearby pyramidal cells is low.
Mossy fibers have different terminal types
Three basic types of terminals were encountered along the main
axon of granule cells: large mossy terminals (4-10 µm), filopodial extensions of mossy boutons (0.5-2.0 µm), and small en
passant varicosities (0.5-2.0 µm). The latter two will be
referred to as "small" terminals (Fig.
3). These small terminals of granule cells were somewhat larger than the varicosities of CA3 pyramidal neurons (Fig. 3; see Figs. 5, 6) (Sík et al.,
1993).
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Figure 3.
Electron micrographs of different terminal types
along the mossy fibers in the CA3 region
(A-C, E) and of a CA3
pyramidal cell terminal (D). All electron
micrographs have the same magnification to help comparison of the
relative size of the terminals. A, B, A
small en passant terminal establishes a single
asymmetrical synapse on a dendritic shaft with long perforated
postsynaptic density (arrows). C, A
filopodial extension of a mossy terminal forms a synapse
(arrow) with an SPR-immunoreactive interneuron.
D, The postsynaptic target of a pyramidal cell terminal
is a simple spine of a CA1 pyramidal neuron. Compare this spine with
the spines of GABAergic interneurons (Fig. 10). E, A
large, double-headed mossy terminal forms multiple contacts
(arrows) with thorny excrescences of a CA3 pyramidal
cell. The individual release sites are short. Scale bars:
A-D, 0.5 µm; E, 1 µm.
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Mossy terminals varied greatly in shape and size. In addition to the
frequent, large single-headed terminals, double-headed and elongated
mossy terminals consisting of three to five bulbous expansions were
also found. Mossy terminals were either in en passant
position or they were connected to the parent axon by a small side
branch (1-30 µm long) (Fig. 2A). The total number of mossy terminals along the main axon in the CA3 region varied from 10 to 18 (average, 12.3 ± 0.9). They were distributed equally in the
three subregions (CA3c, 3.3 ± 0.25; CA3b, 4.1 ± 0.31; CA3a, 4.1 ± 0.4). However, the interval between mossy terminals
increased significantly in the CA3c to CA3a direction (CA3c, 162 ± 12.6 µm; CA3b, 223 ± 19.0 µm; CA3a, 345 ± 27.5 µm), as indicated by ANOVA (F(2,68) = 18.17;
p < 0.001). These findings suggest that the divergence
increases in the CA3c-CA3a axis, provided that the density of
pyramidal cells in the different subregions is similar (Fig.
2C).
The electron microscopic appearance of mossy terminals (Fig.
3E) was similar to that described previously (Blackstad and
Kjaerheim, 1961; Amaral and Dent, 1981; Chicurel and Harris,
1992). They were packed with a large number of round vesicles and a
small number of dense core vesicles and formed intricate multiple
asymmetric synaptic contacts with the thorny excrescences of pyramidal
cells, which were embedded in the body of the terminal. In a fully
reconstructed mossy terminal from 41 ultrathin sections, we found 31 synapses. The lengths of the individual postsynaptic densities were
short. Mossy terminals also contacted the proximal apical shaft of the pyramidal cell with rows of punctum adherens-like specializations (Amaral, 1979). Previous research indicated that a single mossy terminal innervates thorny excrescences pertaining to the same pyramidal cell (Chicurel and Harris, 1992). Because double-headed mossy
terminals were also encountered, we examined their postsynaptic targets. Two double-headed boutons were reconstructed from 41 and 54 serial electron microscopic sections, respectively (the second
reconstruction was still partial). In both cases, both heads of the
mossy terminals converged to thorny excrescences of the same pyramidal
cell (Fig. 3E).
Filopodial extensions of the mossy terminals have been described
previously in Golgi material (Amaral, 1979). In our study, many mossy
terminals had varying numbers of hair-like extensions, often with
bulbous endings (Figs. 1-3; see Figs. 4-6). The mean number of
filopodial extensions with a bulbous ending (2.25/mossy terminal; n = 171) indicated that an average granule cell has
25-35 filopodial extensions. Electron microscopic examination of 15 filopodial extensions with a bulbous ending showed that all of them
established synapses. The varicosities of filopodial terminals were
packed with round vesicles and, in most cases, made only one synaptic specialization, often of the perforated type (Fig. 3). The postsynaptic densities were longer than those of the individual synapses of the
mossy terminals or the terminals of CA3 pyramidal cells (Fig. 3; see
Figs. 5, 6). The terminals also contained dense-core vesicles. Filopodial extensions did not form punctum adherens-like
specializations even when unfilled terminals were examined (see below).
The necks of the filopodia (2-50 µm long) were very thin, followed a
tortuous route, and did not form synapses.
The terminals belonging to the third type were small en
passant boutons along the mossy fibers (Fig. 3; see Fig. 6), as
also seen in earlier studies (Gulyás et al., 1992; Soriano and
Frotscher, 1993). These en passant varicosities were much
smaller (0.5-1.5 µm) than the mossy terminals. At the light
microscopic level they appeared as a fusiform thickening of the main
axon. The incidence of varicosities showed great variation among
individual granule cells. To determine whether all of these
varicosities represented conventional synapses, long segments of mossy
fibers (total of 750 µm in the CA3b region) were re-embedded and
serially sectioned for electron microscopic reconstruction. The labeled
mossy fibers were found embedded in the bundles of unstained mossy
fibers. The electron microscopic examination revealed that many of the small varicosities were clumps of mitochondria or filling artifacts, and only a portion of them represented synapses. Serial reconstruction revealed that the average interval between en passant
synaptic terminals was 250 µm, thus comparable to the distances of
the large mossy terminals. Therefore, a single granule cell may give rise to ~12-17 small en passant synaptic terminals in the
CA3 region. This figure should be considered an underestimation because the dark biocytin immunoprecipitate of the well filled main axon probably masked some synapses associated with the preterminal axon
segment (Gulyás et al., 1992; Soriano and Frotscher, 1993). The
ultrastructure of the small varicosities was similar to the bulbous
endings of the filopodial extensions. The terminals were packed with
round vesicles and formed mostly simple but occasionally perforated
synapses with long postsynaptic thickenings. One of them, reconstructed
from 15 ultrathin sections, showed that all postsynaptic
specializations are indeed linked and form one long perforated synapse
(Fig. 3A,B). The en passant synapses did not have
punctum adherens-like specialization. Dense-core vesicles were also
present in this terminal type.
Target specificity of different mossy fiber terminals in the
CA3 region
Various neurochemical markers known to label distinct
GABAergic neuron populations were used to examine the postsynaptic
targets of the different terminal types. Substance P receptor (SPR)
antibody was selected as a marker because it visualizes most GABAergic interneurons of various subtypes in the CA3 region in their entirety, including their distal dendrites and spines (Acsády et al.,
1997). Other markers used in this study included parvalbumin, which
labels a well characterized perisomatic inhibitory cell
population, and calretinin, which is present in interneurons
specialized to innervate other interneurons (Gulyás et al.,
1996).
As discussed above, mossy terminals contacted the proximal dendrites of
CA3 pyramidal neurons. Interneurons, however, were rarely among their
postsynaptic elements. After systematic screening of 24 mossy terminals
belonging to four granule cells, only one was found to form a putative
contact with an SPR-immunoreactive cell (Fig.
4A). Correlated
electron microscopy of this contact revealed that the mossy terminal
made a conventional asymmetrical contact with a spine of an
SPR-immunoreactive neuron.
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Figure 4.
GABAergic interneurons are innervated by small
terminals. Mossy fibers of two adjacent granule cells in CA3c.
A, Large mossy terminals only exceptionally innervate
SPR-immunoreactive neurons (arrow). B,
Thirteen other SPR-immunoreactive interneurons (only 7 shown here) were
contacted by either filopodial extensions or en passant
terminals of the same two mossy fibers shown in A.
Twelve of the 13 contacts were verified by electron microscopy (shown
in Figs. 5, 6). All subtypes of SPR-immunoreactive cells were
innervated by mossy fibers. The postsynaptic structures were somata
(neurons 4 and 5) or proximal
(1 and 7) or distal dendrites
(2, 3, and 6). All
contacts were single. Inset in A shows
the position of the reconstructed fibers in the CA3c subregion. Scale
bar, 50 µm. str.luc., Stratum lucidum;
str.pyr., stratum pyramidale; str.gran.,
stratum granulare.
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In contrast, filopodial extensions of the large mossy terminals and
small en passant terminals were often found to be in close apposition to SPR-immunoreactive neurons. Of 74 small terminals examined along the same mossy fibers at the light microscopic level, 35 made putative contacts on SPR-positive cells (Fig.
4B). This figure is probably an underestimation
because contacts on distal dendrites and especially on spines were
often hard to discern. In these experiments several of the postsynaptic
SPR-positive cells were reconstructed by camera lucida to examine the
number of synaptic contacts on single cells from a single mossy fiber and to identify the target neuron types. A single mossy terminal often
emitted several filopodial extensions. These extensions typically
innervated different SPR-immunoreactive neurons with only a single
contact. Multiple contacts (two to three) were encountered in only four
cases. Correlated electron microscopy was performed in 21 cases
(including one of the multiple contacts). Of the putative contacts, 18 of 21 were verified to form conventional asymmetric synapses (Figs.
5, 6). All
postsynaptic targets that were examined showed the characteristics of
interneurons, including invaginated nuclei, numerous mitochondria and
other cytoplasmic organelles in the cell body, and a large number of
asymmetrical synapses along the dendrites. The ultrastructure of
SPR-immunoreactive spines showed pronounced differences from both the
simple spines and the thorny excrescences of the pyramidal cells
(Gulyás et al., 1992). Dendritic spines of interneurons were long
and thin (up to 5 µm) and had no separate head region. The entire
spine was covered with several asymmetrical synapses (see Fig. 10), in contrast to spines of pyramidal cells, which had a simple short neck
and a mushroom-shaped head with usually a single synapse. Thorny
excrescences of pyramidal cells, embedded in the large mossy terminals,
were also easily distinguishable. Interneuron spines were not embedded
in the large mossy boutons.
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Figure 5.
Correlated light and electron micrographs of a
contact between a filopodial extension and an SPR-positive interneuron.
A, High-power light micrograph of an intracellularly
labeled mossy terminal (mt) showing one of its
filopodial extensions (arrowhead, f) in close
apposition to an SPR-positive interneuron (sSPR)
in the CA3c region. B, Camera lucida reconstruction of
the contacted SPR-containing cell, together with the afferent mossy
fiber segment (neuron 4 in Fig. 4). C,
Low-power electron micrograph. Note that the mossy terminal
(mt) contacts the thorny excrescenses of a pyramidal
cell dendrite (dP), whereas the terminal bulb of
the filopodium (f) is attached to the soma
of the SPR-positive interneuron (sSPR).
D, High-power electron micrograph of the asymmetrical
synapse (arrow) established by the filopodium
(f) on the soma of the SPR-containing
interneuron (sSPR). Scale bars:
B, 25 µm; C, 1 µm; D,
0.5 µm.
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Figure 6.
Convergence of adjacent granule cells to a spiny
SPR-immunoreactive cell (A-F) and innervation of
a parvalbumin-positive interneuron by a granule cell
(G-H). A, Camera lucida drawing
of an SPR-positive spiny neuron in the CA3c subregion (neuron
3 in Fig. 4B). The same tertiary
dendrite is contacted by mossy fibers of two neighboring granule cells
(arrowheads). The left contact is formed by a small
en passant terminal (st), whereas the
right contact is formed by a filopodial extension
(f). B, C,
High-power light micrographs of the mossy terminal (mt),
terminal bulb of the filopodial extension (arrowhead,
f in B), and the small en
passant terminal (arrowhead, st
in C). D-F, Correlated electron
micrographs of mossy terminal (mt), filopodia
(f), and small terminal
(st), respectively. Arrows indicate
synapses. G, High-power light micrograph of a small
en passant terminal in close apposition to a
parvalbumin-positive dendrite (arrowhead).
H, Electron micrograph showing two separate release
sites (arrows), a rare case for small terminals.
Open arrow indicates unlabeled small terminal;
arrowhead indicates dense-core vesicle.
dPV, Parvalbumin-positive dendrite Scale bars:
A, 50 µm; B, C, G, 10 µm;
D, 1 µm; E, F, 0.3 µm;
H, 0.5 µm.
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Every type of SPR-positive interneuron was represented among the
postsynaptic targets of filopodial extensions and small terminals (Fig.
4B). Spiny SPR-positive neurons (Acsády et al.,
1997), with dendrites parallel to the mossy fibers, were innervated
more frequently. The postsynaptic structures included somata, proximal or distal dendritic shafts, and spines. Given the restricted course of
granule cell axons, the location of synapses depended primarily on the
type of structure present in the stratum lucidum without any preference
for somata, proximal, or distal dendrites.
To determine whether filopodial extensions establish synaptic contacts
with pyramidal neurons, the postsynaptic targets of four filopodia,
which did not contact SPR-immunoreactive elements, were examined under
the electron microscope. All four terminals innervated distal dendrites
with ultrastructural characteristics of GABAergic cells, which were
clearly distinguishable from the thick primary dendrites and thorny
excrescences of pyramidal cells in stratum lucidum. Furthermore,
examination in serial ultrathin sections of the 18 terminals that
established synapses on the SPR-positive cells revealed only single
release sites on the SPR-positive interneurons. No additional release
sites were found for potential contacts with the surrounding pyramidal
cells.
Convergence of granule cells on interneurons was examined in one case
in which two adjacent granule cells were intracellularly labeled. From
the 18 SPR-immunoreactive neurons innervated by the filopodial
extensions and small en passant terminals of the two granule
cells, one spiny SPR-positive cell was found to receive synaptic
contacts from both granule cells (Fig. 6).
Analysis of parvalbumin- and calretinin-immunoreactive postsynaptic
targets of the various terminal types confirmed and extended the above
observations that interneurons were innervated by filopodial extensions
and small en passant terminals (Fig.
6G,H). A segment of a parvalbumin-immunoreactive
dendrite in the stratum lucidum was reconstructed from 45 electron
microscopic sections, and all afferent synaptic boutons were
photographed. In addition to the single synapse established by the
biocytin-labeled terminal, 19 unlabeled boutons forming asymmetrical
synapses were identified. All of these showed ultrastructural
characteristics of small terminals. Their diameter was <1.5 µm, and
they formed single, usually perforated synapses with long postsynaptic
thickening. Puncta adherentia were not present. Many of the small
terminals contained dense-core vesicles, indicating granule cell
origin. These observations support the suggestion that excitatory
inputs of granule cells to CA3 interneurons are established by small
en passant or filopodial terminals and not by large mossy
boutons.
To summarize, our analysis of postsynaptic targets of granule cells in
the CA3 region indicates that (1) mossy terminals innervate pyramidal
cells, whereas filopodial extensions and small en passant terminals contact primarily interneurons, and (2) small terminals and
filopodial extensions outnumber mossy terminals; therefore granule
cells innervate substantially more GABAergic interneurons than
pyramidal cells.
Terminal types of granule cells in the hilar area
Nearly the entire local axon arbor of the labeled granule cells
was within the border of the hilar region as visualized by SPR and
mGluR1a immunostaining (p = 6 cells) (see
below), confirming previous Golgi and single cell labeling studies
(Ramón y Cajal, 1911; Claiborne et al., 1986). The main axon of
the granule cell emitted five to eight thinner side branches in the
hilus, which occasionally bifurcated and gave rise to secondary
branches. The side branches followed a tortuous route usually parallel
to stratum granulosum. A recurrent collateral penetrating into stratum
granulosum was observed only in a single case. The total septotemporal
extension of the hilar plexus was 600 µm. However, 90% of the hilar
collaterals was within a 400 µm lamella. The transversal extent of
the hilar axon arbor depended on the location of the soma and varied
from 400 to 700 µm.
The terminal types in the hilus were similar to those described in the
CA3 region (Fig. 7). However, small
terminals along the side branches were much more numerous than in area
CA3. Many of the small terminals were situated on a short stalk and
formed "drumstick" rather than en passant boutons. Each
side branch had one or two large mossy terminals and associated
filopodial extensions. Not all mossy boutons were in the terminal
position. A single granule cell had 7-12 mossy boutons and 102-147
small terminals (p = 5 cells). Correlated light
and electron microscopy of 26 terminals verified synapse in each case.
Thus, artifactual en passant varicosities, observed in the
CA3 region, were much less common in the hilar area. The intervals
between small terminals were highly variable.
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Figure 7.
Terminal types of mossy fibers in the hilus. All
electron micrographs have the same magnification. A,
Mossy terminal establishing four synapses (arrows) with
the shaft and the thorny excrescences of a mossy cell. Curved
arrows point to the filopodiae originating from this terminal.
B, A small en passant terminal with
single release site (arrow) contacts a dendritic shaft.
C, A drumstick-like small terminal forms a synapse on
the proximal part of an SPR-positive spine. Open arrows
in B and C label synapses formed by
unlabeled small terminals. D, E,
Intermediate terminal type contacting a distal SPR-positive dendritic
shaft (arrow in D) and on a neighboring
section forming two synapses (arrows in
E) on a putative mossy cell. Scale bars:
A, 1 µm; B-E, 0.5 µm.
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The ultrastructural features of small terminals and filopodial
extensions were identical to those described above for the terminals in
the CA3 region. In addition, 5-10% of the terminals showed
characteristics intermediate between the large mossy and small
terminals. These latter varicosities had a diameter of 2-3 µm,
displayed multiple release sites, and occasionally innervated a
GABAergic cell and the distal dendrite of a putative mossy cell at the
same time (Fig. 7D,E). These intermediate-size terminals therefore might be considered a variant of the mossy terminal.
Postsynaptic interneuron targets of the granule cells in
the hilus
SPR and mGluR1a immunostaining were used to study the postsynaptic
targets of granule cells. These antibodies were chosen because they
label a large fraction of GABAergic interneurons in the hilar region
and because the dendritic distribution of these cells clearly outlines
the border between the hilus and the CA3c region (Ramón y Cajal,
1911; Amaral, 1978), as indicated by two independent means. First, the
distal dendrites of in vivo filled CA3c pyramidal cells
always terminated outside the border of the densely immunoreactive
area. Second, all dendrites of an in vivo filled mossy cell
were confined to the hilar region, as outlined by SPR staining.
The postsynaptic interneuron targets of granule cells in the hilus were
examined by using antibodies against mGluR1a (p = 2 cells) and SPR (n = 4 cells). mGluR1a
immunoreactivity is present in all somatostatin-positive interneurons
(Baude et al., 1993), whereas 60% of somatostatin-immunoreactive cells
also contain SPR (Acsády et al., 1997). In addition, SPR is
present in other GABAergic cell types (Acsády et al., 1997).
Thus, the two markers label partially overlapping sets of GABAergic
interneurons in the hilus. All mGluR1a-immunoreactive neurons had large
fusiform or polygonal cell bodies and three to five primary dendrites, which were densely covered with long spines that had many branches. SPR
immunostaining labeled GABAergic neurons similar to those in the CA3
region.
The large mossy terminals did not contact mGluR1a-positive cells
(n = 11). In contrast, 52 of the 175 small terminals
and filopodiae that were examined (30%) innervated
mGluR1a-immunoreactive neurons (Fig. 8).
A representative sample of 22 contacts was identified by correlated
light and electron microscopy as a conventional asymmetrical synapse
(Fig. 10). The postsynaptic targets of four granule cells were examined
with SPR immunostaining. Of the small terminals examined, 44 of the 76 (58%) were in close apposition to SPR-immunoreactive somata,
dendrites, or spines. Four of these contacts were examined at the
electron microscopic level, and a single synapse was verified in each
case. The higher ratio of contacts in the case of SPR-positive cells
may reflect the higher percentage of interneurons labeled by this
marker in the hilar region. None of the markers used alone or in
combination label all hilar GABAergic cells. Nevertheless, the high
incidence of synaptic contacts observed with these markers indicates
that most of the small terminals innervate GABAergic cells in the hilar region.
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Figure 8.
GABAergic cells are major postsynaptic
targets of the small terminals of granule cells in the hilus. Shown are
hilar axon arbors of two adjacent granule cells
(gray and black) and their
mGluR1a-immunoreactive targets reconstructed from three neighboring
60-µm-thick sections. Fifty-two of the 175 small terminals and
filopodiae (arrowheads) innervated
mGluR1a-immunoreactive targets, whereas large mossy terminals contacted
none. A representative sample of 22 contacts was identified at the EM
level (illustrated in Fig. 10). Boxed area in the
inset shows the position of the axon arbor. Scale bar,
50 µm.
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To determine whether small en passant terminals had an
absolute target selectivity for interneurons in the hilar region,
presynaptic terminals impinging on the distal dendrites of an
intracellularly filled mossy cell were examined. Several terminals that
established synapses on distal dendritic shafts or spines of the mossy
cell bore the characteristics of small terminals of granule cells (data not shown). This observation therefore indicates that small terminals in the hilar region also can be presynaptic to mossy cells.
Nevertheless, the high ratio of contacts between the small terminals
and GABAergic interneurons in the dorsal hilus suggests a target
preference for interneurons.
The convergence and divergence of granule cells were studied with
mGluR1a immunostaining in a rat in which two granule cells were
labeled. The postsynaptic mGluR1a-immunoreactive neurons were
reconstructed with camera lucida from seven consecutive 60-µm-thick sections with the highest density of axon collaterals (Fig.
9). The seven reconstructed
mGluaR1a-immunoreactive neurons received 11 contacts, 6 of which were
identified under the electron microscope. Two of the seven cells
received convergent inputs from both granule cells. Most contacts
corresponded to single release sites. Double contacts were found in two
cases. These contacts were found on different dendritic branches in
both cases (Fig. 9). Postsynaptic targets included somata, proximal or
distal dendritic shafts, and spines (Fig.
10).
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Figure 9.
Convergence and divergence of granule cell
contacts on hilar mGluR1a-positive neurons. Camera lucida
reconstruction of three hilar mGluR1a-immunoreactive neurons from six
60-µm-thick sections, innervated by the two granule cells shown in
Figure 8. Neuron 1 received a single contact from one of
the granule cells (black arrowhead); both granule cells
converged onto neuron 2 with single contacts each
(black and gray arrowhead), whereas
neuron 3 was innervated by two terminals of the other
granule cell (gray arrowheads). Correlated
electron micrographs of the contacts are shown in Figure 10.
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Figure 10.
Small terminals of mossy fibers innervate
mGluR1a-containing GABAergic cells (dmGluR) in
the hilus. Correlated light (small insets) and electron
micrographs of three contacts shown in Figure 9. Neurons
1 and 2 are contacted
(arrows in A and C,
respectively) on their spines (s), whereas neuron
3 receives a synapse on a proximal dendrite
(B). Open arrows label synapses
formed by unlabeled small terminals. st, Small terminal.
Scale bars: A-C, 0.5 µm.
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Dynorphin-SPR double immunostaining
Because mossy fibers contain the neuropeptide dynorphin (McLean et
al., 1987; Drake et al., 1994), immunostaining against this
neuropeptide allowed us to identify their terminals and investigate their postsynaptic elements using double immunostaining against dynorphin and SPR (pre-embeding gold and DAB, respectively; see Materials and Methods). Dynorphin immunoreactivity was present in the
mossy fiber system as a diffuse precipitate, as described previously
(McLean et al., 1987; Drake et al., 1994), but a few individual mossy
terminals showed very strong immunoreactivity. At the ultrastructural
level, gold particles indicated that dynorphin immunoreactivity was
distributed in synaptic terminals with characteristics of both large
and small terminal types (Fig. 11). In
addition to axonal staining in the hilar region, weak immunoreactivity
was present also in the dendrites of granule cells, as described
previously (Drake et al., 1994). The pattern of SPR immunostaining
remained unchanged after the pre-embedding gold staining procedure.
Examination of 21 dynorphin-positive terminals, establishing
asymmetrical synapses with SPR-positive profiles, demonstrated that all
of them showed the characteristics of small terminal types (Fig. 11).
The presynaptic terminals were 0.5-1.0 µm in diameter, formed single
release sites, and did not have punctum adherens-like specialization. These results confirmed that most excitatory input to GABAergic cells
from granule cells derives from small terminals.
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Figure 11.
Excitatory inputs from granule cells to GABAergic
cells are established by small terminals. Dynorphin (mossy fibers)-SPR
(interneurons) double immunostaining. Dynorphin and SPR were visualized
using pre-embedding gold immunostaining (dark, electron-dense particles
labeled by arrowheads) and DAB (diffuse precipitate),
respectively. A, B, Two neighboring
sections show that a dynorphin-positive terminal contacts
(arrows) a distal SPR-immunoreactive dendritic shaft
(dSPR). Note that the presynaptic terminal shows
the characteristics of small mossy fiber terminals (i.e., single, long
postsynaptic thickening, lack of punctum adherens). C,
D, The same type of terminals contact
(arrows) an SPR-positive spine (s in
C)and a proximal and a distal dendrite
(dSPR and d, respectively, in
D). E, A large dynorphin-positive
terminal forms multiple contacts on an SPR-negative mossy cell
dendrite (dM). Scale bars: A-E,
0.5 µm.
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DISCUSSION |
The main findings of the present study are that (1) granule
cells innervate their principal cell and interneuron targets
preferentially by large mossy boutons and small en passant
or filopodial terminals, respectively; (2) they innervate substantially
more inhibitory than excitatory cells; and (3) convergence of granule
cells to principal cells is very limited, whereas convergence on
interneurons may be high. At the cellular level, this synaptic
arrangement may allow for the target-dependent regulation of glutamate
release, whereas at the network level it may efficiently suppress
recurrent excitation in the CA3 collaterals but allow for the selective discharge of a few CA3 pyramidal cells.
Granule cells affect their targets by morphologically
different terminals
The present in vivo single cell labeling study
confirms and extends previous works using Golgi material and the
in vitro slice preparation regarding the topography of the
mossy fiber system (Swanson et al., 1978; Amaral and Witter,
1989; Tamamaki and Nojyo, 1991). Local collaterals of a single granule
cells in the dorsal hippocampus arborized in the hilus, whereas the
main axon coursed in the CA3 region. Most hilar branches and the main
axon in the CA3c and CA3b regions remained within a 400 µm
transversal lamella. However, in the CA3a region the mossy terminal
turned caudally and continued for up to 1 mm. The intervals of mossy
terminals increased in the CA3c to CA3a direction. This might reflect
the lower packing density of pyramidal cells in the distal CA3 region or increasing divergence.
Cortical pyramidal cells give rise to large numbers of axon collaterals
and innervate all postsynaptic targets with morphologically identical
boutons (Kisvárday et al., 1986; Gulyás et al., 1993; Sík et al., 1993; Li et al., 1994). In contrast, granule cells have very specialized synaptic terminals, including the large mossy
boutons, small en passant terminals, and filopodial
extensions of the mossy boutons (Ramón y Cajal, 1911; Amaral,
1979; Claiborne et al., 1986). These three terminal types were observed
in both the hilus and the CA3 region. Electron microscopic examination demonstrated ultrastructural similarities between filopodial extensions and the small en passant terminals and their differences
from the large mossy boutons. The large mossy terminals had as many as
31 release sites, confirming previous results (Chicurel and Harris,
1992). In addition, they contacted the pyramidal cells by rows of
puncta adherentia. In contrast, the small en passant terminals and filopodial extensions in most of the cases established a
single release site and did not have punctum adherens-like
specializations. A single granule cell gave rise to only 7-12 large
mossy boutons in the hilus and 11-18 boutons in the CA3 region. In
contrast, the number of small terminals (en passant and
filopodial) was considerably higher both in the hilus (120-150) and
the CA3 region (40-50). The number of small terminals is likely
underestimated because of technical factors, including incomplete
filling of thin filopodial extensions and biocytin "masking" of
en passant terminals.
Large mossy boutons and small terminals preferentially innervate
principal cells and interneurons, respectively
Cortical pyramidal neurons innervate their postsynaptic principal
and interneuron targets nonpreferentially, i.e., the incidence of the
targets is determined by the relative distribution of the neuron types
(Kisvárday et al., 1986; Gulyás et al., 1993; Sík et al., 1993). Our findings indicate that this is not the case with
granule cells. The GABAergic targets were preferentially innervated by
filopodial extensions and the small en passant terminals and
only exceptionally by the large mossy bouton. Some previous observations are in accordance with this conclusion (Amaral, 1978, his
Figs. 46, 75; Ribak and Seress, 1983, their Fig. 16; Gulyás et
al., 1992; Ribak, 1992; Soriano and Frotscher, 1993; Halasy and
Somogyi, 1993; Geiger et al., 1997). Two previous electron microscopic
studies indicated that the postsynaptic targets of small terminals were
smooth dendrites, a known characteristics of several GABAergic cell
types (Amaral, 1979; Claiborne et al., 1986). In contrast, other
studies suggested that the large mossy terminals contact GABAergic
cells both in the hilus and in the CA3 region of the rat (Frotscher,
1985; Ribak and Seress, 1988; Frotscher, 1989; Deller and
Léránth, 1990; Léránth et al., 1990; Nitsch et
al., 1990; Deller et al., 1994) and the monkey (Seress and
Léránth, 1996). This apparent controversy is likely attributable to the difficulty involved in the identification of
postsynaptic targets at the light microscopic level and the lack of a
reliable marker of presynaptic terminals in most of these studies.
Importantly, none of these investigations attempted to quantitatively
assess the regional distribution of the different terminal types and
their precise neuronal targets.
Several observations in our study suggest that small terminal types
form the majority of synaptic contacts between granule cells and
interneurons. First, examination of the intracellularly filled granule
cells showed that a large portion of their targets were GABAergic, as
indicated by the SPR, mGluR1a, calretinin, or parvalbumin
immunoreactivity of the innervated neurons. In the CA3 region, 47% of
the small terminals contacted SPR-containing cells, although
SPR-immunoreactive neurons make up <5% of the total neuronal
population in this region. In the hilus, 30 and 58% of small terminals
innervated mGluR1a- and SPR-immunoreactive cells, respectively, which
better matches the proportion of these interneurons within the
GABAergic population rather than within the entire neuron population of
the hilus. Clearly, not all GABAergic cells were labeled by these
markers. Most contacts made by a single granule cell with its
interneuron targets corresponded to a single release site. Second, we
found no indication that dendrites of pyramidal cells were contacted by
either the small en passant boutons or the filopodial
extensions, although in the hilar region, small terminals of assumed
granule cells innervated the distal dendrites of mossy cells.
Third, electron microscopic examination revealed that
dynorphin-immunostained presynaptic terminals on GABAergic dendrites in
the hilus and the CA3 region were always of small size (0.5-2.0
µm).
GABAergic cells form a morphologically and functionally diverse
neuronal population (Freund and Buzsáki, 1996). All GABAergic subgroups examined with antibodies against SPR, mGluR1a, parvalbumin, and calretinin were innervated by the small terminals of granule cells.
Spiny GABAergic cells with horizontal dendrites in the stratum lucidum
and their hilar counterparts, visualized with mGluR1a and SPR and
calretinin immunostainings, were innervated more frequently than the
other morphological categories. This may be because their dendrites are
restricted to the termination zone of mossy fibers and because their
dendritic surface is increased several-fold by a large number of
spines. These spiny cells also colocalize somatostatin and NPY (Baude
et al., 1993; Acsády et al., 1997), and their axons innervate the
distal dendritic region of principal cells, in association with the
entorhinal afferents (Han et al., 1993; Deller and Léránth,
1990; Léránth et al., 1990; Sík et al., 1997). This
inhibitory feed-back loop therefore may exert an effective control on
the entorhinal activation of granule cells.
The large mossy terminals contacted pyramidal cells and mossy cells, as
identified by their characteristic thorny excrescences. Synaptic
contact between a large mossy bouton and interneuron was observed only
in a single case. Serial sections of single- and double-headed large
mossy terminals indicated 30-40 release sites, all of which were
presynaptic to the same single postsynaptic pyramidal cell (Chicurel
and Harris, 1992) (this study).
On the basis of these observations, we conclude that granule cells
innervate their principal cell and interneuron targets via large mossy
boutons and small en passant or filopodial terminals, respectively (Fig. 12). Because each of
these terminals typically contacts a single neuron, the larger number
of small terminals indicates that granule cells innervate substantially
larger number of inhibitory interneurons than principal cells. The
estimated ratio of interneurons versus principal cell targets of the
mossy fibers is 1:4 to 1:6. Because this ratio is 1:10 to 1:20 for
cortical pyramidal cells (Kisvárday et al., 1986; Gulyás et
al., 1993; Sík et al., 1993; Douglas et al., 1995), we conclude
that, on average, granule cells contact GABAergic targets ~50 times
more frequently than other cortical principal cells.
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Figure 12.
Filopodial extensions of mossy terminals are
specialized to innervate GABAergic cells. Artistic rendition of two
mossy terminals, each with four filopodial extensions (large
arrowheads). All filopodial terminals contacted the dendrites
or spines of six GABAergic neurons. Four of them were identified by
their SPR-content and two of them by ultrastructural characteristics.
Five of the six postsynaptic interneurons were spiny cells. All
synapses were identified at the electron microscopic level (data not
shown). Arrows point to the main axons.
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Functional implications
Our anatomical examinations indicate that granule cells innervate
their postsynaptic pyramidal and GABAergic interneuron partners by
morphologically distinct presynaptic terminals. These terminal types
may not only exert differential effects on their postsynaptic targets
but may also have distinct mechanisms for transmitter reuptake and for
presynaptic control of transmitter release. In support of the latter
possibility, small presynaptic terminals innervating presumed
interneurons in stratum lucidum have recently been shown to express
presynaptic mGluR7b receptors, whereas the majority of large terminals
lacked this receptor (Shigemoto et al., 1997). The large and small
terminals may also express a different type of plasticity. Tetanic
stimulation of the mossy fibers is known to induce a presynaptic form
of long-term potentiation (LTP) in CA3 pyramidal cells (Jaffe and
Johnston, 1990; Zalutsky and Nicoll, 1990; Derrick and Martinez, 1996;
Urban et al., 1996). Recent works suggest that mossy fiber
stimulation-induced LTP may be absent in interneurons
(Maccaferri et al., 1998). The cause of this differential LTP
expression may be found in the different molecular compositions of the
large and small presynaptic boutons.
The granule cell to mossy cell and pyramidal cell excitatory
connectivity is characterized by a very limited convergence. In our
study, even neighboring granule cells failed to converge on common
pyramidal cell targets. In contrast, previous studies have already
indicated that hundreds or perhaps thousands of granule cells may
converge on the horizontal spiny interneurons of stratum lucidum
(Gulyás et al., 1992; Hsu and Buzsáki, 1993). Convergence of granule cells on interneurons was also common in our
experiments.
The low probability of principal cell innervation by granule cells can
also be contrasted with the higher probability of interneuron innervation in both the hilus and the CA3 region. This anatomical arrangement may explain why increased granule cell activity, in general, is associated with decreased excitability of CA3 pyramidal cells (Bragin et al., 1995a,b; Penttonen et al., 1997). Such a mechanism would insure that only a selected small group of pyramidal cells will be discharged by the dentate input. Threshold
depolarization, in principle, can be achieved by the coincident
activity of granule cells on a common pyramidal cell target. However,
the slow firing rate of granule cells (p < 0.5 Hz) (Jung and McNaughton, 1993), coupled with the extremely low
convergence of granule cells onto pyramidal cells and strong
feed-forward inhibition, suggests that the probability of such
coincident discharge is exceptionally low. These considerations suggest
that in the intact brain, transmission of information from the dentate
gyrus to the Ammon's horn may be provided by concerted release of the
neurotransmitter from a single mossy bouton (Henze et al., 1997). This
single granule cell-principal cell spike transmission may be
facilitated by subcortical neurotransmitters and by the direct, highly
divergent excitatory perforant path afferents.
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FOOTNOTES |
Received Dec. 19, 1997; revised Feb. 11, 1998; accepted Feb. 16, 1998.
This work was supported by the National Institute of Neurological
Diseases and Stroke (NS34994), the National Institute of Mental Health
(MH 54671), the OTKA (T16942), the Human Frontier Science Program, the
Whitehall Foundation, the Soros Foundation, and the Howard Hughes
Medical Institute. We thank M. Penttonen for performing some of the
intracellular experiments, L. Záborszky, Z. Nádasdy, E. Borók, H. Oliviera, and G. Goda for support, and T. Gorcs,
J. H. Rogers, and R. Shigemoto for the antibody gifts.
Correspondence should be addressed to György Buzsáki,
Center for Molecular and Behavioral Neuroscience, Rutgers University, 197 University Avenue, Newark, NJ 07102.
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Top
Abstract
Introduction
