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The Journal of Neuroscience, January 28, 2004, 24(4):853-864; doi:10.1523/JNEUROSCI.1619-03.2004
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Neurobiology of Disease
Translamellar Disinhibition in the Rat Hippocampal Dentate Gyrus after Seizure-Induced Degeneration of Vulnerable Hilar Neurons
Colin A. Zappone andRobert S. Sloviter Departments of Pharmacology and Neurology, and the Graduate Program in Neuroscience, University of Arizona College of Medicine, Tucson, Arizona 85724
Abstract
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Abstract
Introduction
Longitudinally restricted axonal projections of hippocampal granule cells suggest that transverse segments of the granule cell layer may operate independently (the "lamellar" hypothesis). Longitudinal projections of excitatory hilar mossy cells could be viewed as antithetical to lamellar function, but only if longitudinal impulse flow effectively excites distant granule cells. We, therefore, determined the effect of focal granule cell discharges on granule cells located >2 mm along the longitudinal axis. During perforant pathway stimulation in urethane-anesthetized rats, passive diffusion of the GABAA receptor antagonist bicuculline methiodide from the tip of a glass recording electrode evoked granule cell discharges and c-Fos expression in granule cells, mossy cells, and inhibitory interneurons, within a400 µm radius. This focally evoked activity powerfully suppressed distant granule cell-evoked responses recorded simultaneously
Key words: lamellar hypothesis; inhibitory interneurons; hippocampus; epilepsy; c-Fos; lateral inhibition
Introduction
Despite decades of study, the nature of the three-dimensional functional organization of the mammalian hippocampus remains controversial. The lamellar hypothesis posits a system in which focal excitation is conveyed sequentially to target neurons within functionally separated slices or "lamellae" (Andersen et al., 1971, 2000
In this study, we have determined for the first time the nature of the influence of focal granule cell discharges on distant granule cells located
Materials and Methods
Male Sprague Dawley rats (250–400 gm) were treated in accordance with guidelines set by the National Institutes of Health for the humane treatment of animals and approved by the University of Arizona Institutional Animal Care and Use Committee.KA SE and PP stimulation. Rats were anesthetized briefly with ether, a small incision was made in the skin overlying the saphenous vein, and KA (9–12 mg/kg; 10 mg/ml saline; Ocean Produce International, Shelburne, Canada) or saline was injected intravenously. After the end of SE, animals were given saline periodically by subcutaneous injection, and apple slices were provided as a source of food and water in a combined, digestible form. Four saline-treated rats and 14 rats that survived KA-induced SE lasting 3–6 hr were subsequently evaluated as described below. Intermittent PP stimulation for 24 hr was performed in six urethane-anesthetized rats to produce extensive hilar neuron loss throughout the dorsal hippocampus, as described previously (Sloviter et al., 2003
Assessment of translamellar influences. Normal (n = 23), KA-treated (n = 14), saline-treated (n = 4), and PP-stimulated (n = 6) rats were anesthetized with urethane (1.25 gm/kg, s.c.) 3 d after saline or KA injection, or 3 d after the end of 24 hr intermittent PP stimulation, and placed in a stereotaxic apparatus. The rectal temperature was maintained at 37.0 ± 0.2°C. A bipolar-stimulating electrode (NE-200; Rhodes Medical Instruments, Summerland, CA) was placed in the left angular bundle of the PP (
Translamellar influences were assessed by first lowering a saline-filled recording electrode into the hippocampus (
Retrograde transport of FG. The retrograde tracer FG (Fluorochrome, Englewood, CO) (Schmued and Fallon, 1986
Perfusion fixation and tissue treatment. After 1 hr of BMI-induced granule cell discharges at the posterior recording site, all electrodes were removed, and the distance between the BMI and saline electrode tips was measured. In 11 additional rats, electrodes were removed after 7 hr of BMI-induced discharges, a duration used to determine whether prolonged discharges would evoke c-Fos expression in distant target cells. All animals were perfused with saline for 2 min, then 4% paraformaldehyde in 0.1 M phosphate buffer, pH 7.4, for 10 min. After storage of the intact rat overnight at 4°C, brains were removed from the skull and placed in perfusate. Coronal sections, 40 µm thick, were cut on a Vibratome in 0.1 M Tris buffer, pH 7.6. Sections were mounted on gelatin- and chrom alum-coated slides for subsequent Nissl (cresyl violet) staining or for staining acutely degenerating neurons with Fluoro-Jade B (Schmued and Hopkins, 2000
For immunocytochemistry, sections were mounted on Superfrost Plus slides, air dried for 15 min, placed in 0.1 M Tris buffer, pH 7.6, and processed as described in detail previously (Sloviter et al., 2003
To determine the extent of hilar neuron loss at the BMI site in KA-treated and PP-stimulated rats, we selected three nonconsecutive Nissl-stained sections from within the c-Fos-positive region of the BMI electrode. The numbers of surviving hilar neurons were counted in three sections from each animal and expressed as means ± SEMs. Although hilar cell loss or survival was relatively uniform throughout the dorsal hippocampus, only sections at the BMI electrode site were assessed quantitatively for hilar neuron loss or survival, because the primary assumption of the experimental design was that it was the activated neurons at the BMI electrode site that mediated the distant effects of the focal granule cell discharges. Statistical comparisons of spike suppression and hilar cell number were made using a Mann–Whitney U test.
Results
Translamellar influences in the normal rat dentate gyrus
In normal (n = 12) and saline-treated (n = 4) control rats, paired-pulse stimulation of the PP (Fig. 1, drawing) at 0.3 Hz and an interpulse interval of 60 msec evoked large amplitude population spikes at the saline-filled recording electrode that exhibited potentiation [i.e., the amplitude of the second of two evoked population spikes was larger than the amplitude of the first population spike (Fig. 1A2)]. While we continuously recorded these potentials at the saline electrode site, and without changing the stimulus parameters, the BMI-filled recording electrode was lowered into the granule cell layer
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Figure 1. Translamellar inhibition in the normal rat dentate gyrus under urethane anesthesia. The influence of focal granule cell discharges evoked at a BMI-filled recording electrode in response to slow (0.3 Hz) PP stimulation (PP stim) was assessed simultaneously at a distant segment of the granule cell layer via a saline-filled recording electrode. A1, A2, Before passive leakage of BMI from the tip of a glass recording electrode, PP stimulation at 0.3 Hz simultaneously evoked single population spikes at both the BMI-filled (A1; pre, pre-diffusion of BMI) and saline-filled (A2) recording electrodes, which were separated
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Figure 2. Progressive and reversible translamellar inhibition in the normal rat dentate gyrus. In this series of simultaneously recorded evoked responses to 0.3 Hz PP stimulation, diffusion of BMI from one recording electrode produced gradually increasing responses (multiple granule cell population spikes) to the same slow afferent stimuli. Coincident with these focal discharges recorded at the BMI-filled electrode (left shaded box), responses recorded simultaneously exhibited selective and progressive suppression of the second population spike and the fEPSP amplitudes (right shaded box). This selective inhibition of the second of two evoked responses at the saline-filled electrode was presumably initiated by the first of two discharges at the BMI-filled electrode, which required the interpulse interval to manifest its longitudinal influence. Note also that neither of the two multiple granule cell discharges at the BMI electrode evoked any detectable excitatory response after the second response recorded at the saline electrode site (arrowed line in trace 7). That is, no distant longitudinal excitatory influences of focal granule cell discharges were detected. Granule cell responses to PP stimulation recorded during the 10 min period after removal of the BMI-filled electrode from the granule cell layer (left trace 8) showed the decline of translamellar inhibition at the saline electrode (right trace 8), apparently reflecting recovery from the influence of the distant BMI-induced discharges as BMI was cleared from the tissue. Calibration, 5 mV and 10 msec.
Focal granule cell discharges generated at the BMI electrode did not increase population spike amplitudes at the saline electrode in any animal tested (n = 16), nor did they evoke any detectable positive-going field potentials indicative of longitudinal excitation that was in any way comparable with even weak PP stimulation. That is, if the second of two multiple discharges recorded at the BMI-filled electrode produced a synchronous depolarization or discharge of the distant granule cells being simultaneously monitored at the saline electrode site, an evoked potential would presumably be detectable after the second evoked potential, during the period marked by the arrowed line in Figure 2, trace 7. Or, translamellar excitation would be expected to increase the amplitude of the population spike, or produce multiple spikes, which are effects we never observed.In a comparison of second spike suppression in control animals at different distances between the BMI- and saline-filled electrodes, no statistically significant difference in second spike suppression was observed between six controls, in which the mean distance between the electrodes was 4.03 mm (range, 3.60–4.89), and four other controls, in which the mean distance was 2.79 mm (range, 2.52–3.24). In these two groups, second spike suppression was 67.60 ± 4.24% in the larger separation group and 73.90 ± 10.13% in the smaller separation group. Thus, the magnitude of second spike suppression in control animals was not significantly different over the range of distances evaluated.
c-Fos expression in normal rats after BMI-induced focal discharges
c-Fos expression was assessed immunocytochemically to determine the extent of focal neuronal activation evoked at the BMI-filled recording electrode. BMI diffusion during slow (0.3 Hz) afferent stimulation consistently evoked c-Fos expression within a radius ofc-Fos expression in dentate hilar neurons and presumed basket cells of the granule cell layer was consistently evident longitudinally, beyond the region of focal granule cell activation (Fig. 3A1). That is, at relatively short longitudinal distances from the outer limit of c-Fos-positive granule cells (
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Figure 3. c-Fos expression beyond the region of focal granule cell activation evoked by BMI diffusion. A1, In sections
Translamellar disinhibition in KA-treated and PP-stimulated rats
Translamellar inhibition was assessed in 14 KA-treated rats, 3 d after all 14 had exhibited prolonged SE lasting at least 3 hr. This was done to determine whether prior hilar neuron loss would abolish BMI-induced translamellar inhibition. Analysis of each KA-treated animal, which was blinded in the sense that the extent of hilar neuron loss could not be known during the electrophysiological assessment, revealed two distinct responses to BMI diffusion. In 10 of the 14 KA-treated rats, BMI-induced granule cell discharges evoked relatively normal suppression of both the population spike and the fEPSPs recorded at the saline electrode (type 1 response) (Fig. 4A4; Table 1). However, in 4 of the 14 identically KA-treated rats, BMI-induced granule cell discharges produced minimal or no distant inhibition at the saline-filled electrode despite similar BMI-induced granule cell discharges (type 2 response) (Fig. 4B4; Table 1). Thus, the loss of translamellar inhibition in KA-treated rats seemed to be a relatively "all-or-none" phenomenon, with 10 KA-treated rats, appearing similar to normal animals, and 4 identically KA-treated rats nearly devoid of translamellar inhibition.
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Figure 4. Translamellar inhibition or disinhibition 3 d after KA-induced SE or 24 hr intermittent PP stimulation. A, KA type 1 response. Rats subsequently found to have an average of 20% fewer hilar neurons compared with controls (Fig. 5E) exhibited intact translamellar inhibition of the evoked granule cell population spike (A4, asterisk; n = 10). B, KA type 2 response. In rats subsequently found to have an average of 85% fewer hilar cells than controls (Fig. 5E; n = 4), BMI-induced discharges (B3) evoked minimal translamellar inhibition (B4, asterisk). C, Similar failure of translamellar inhibition in PP-stimulated rats (C4, asterisk), which exhibited an average of 93% fewer hilar cells (range, 89–95%; n = 6) than controls (Fig. 5E). Calibration, 10 mV and 10 msec.
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Table 1. Translamellar granule inhibition 3 d after KA-induced SE or 24 hr intermittent PP stimulation
Histological analysis (Fig. 5) revealed that, in KA type 1 rats (translamellar inhibition preserved), the number of hilar neurons counted in sections at the BMI electrode site was 20% lower, on average, than controls (saline-treated controls, 62.8 ± 12.0 hilar neurons per section; n = 4; KA type 1, 50.0 ± 3.5 neurons per section; range, 10–38% fewer neurons; n = 10; p > 0.05), which was not statistically significant. In contrast, KA type 2 animals (translamellar inhibition abolished) exhibited an average hilar cell loss of 85%, which was significantly different from type 1 rats and controls (9.5 ± 3.7 neurons per section; range, 68–94% fewer hilar neurons; n = 4; p < 0.05). Although the extent of hilar cell loss in the dorsal hippocampus was highly variable among identically treated KA rats, extensive CA3 pyramidal cell layer damage, ventral hippocampal hilar cell loss, and temporal cortex damage were present in both KA groups. Thus, only extensive dorsal hippocampal hilar neuron loss was consistently associated with a failure of BMI-induced granule cell discharges to evoke translamellar granule cell inhibition (Fig. 5E).
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Figure 5. Hilar neuron loss and c-Fos expression 3 d after KA-induced SE or 24 hr intermittent PP stimulation. A1, NeuN immunoreactivity (a neuronal marker) in the dentate gyrus of a saline-treated control rat, illustrating the normal neuronal constituents of the dentate granule cell layer (sg, stratum granulosum), the hilus (h), and the adjacent end of the CA3c pyramidal cell layer (sp, stratum pyramidale). A2, c-Fos expression in the region of the BMI electrode, showing c-Fos-positive nuclei in cells of all dentate subregions. B1, B2, NeuN and c-Fos expression in a KA-treated rat that exhibited intact translamellar inhibition (type 1 response). Note the persistence of NeuN and c-Fos immunoreactivity in the hilus, which in 10 KA type 1 animals involved an average of 20% fewer hilar neurons counted (range, 10–38%) compared with controls. C1, C2, NeuN and c-Fos expression in an identically KA-treated rat that exhibited a loss of translamellar inhibition (type 2 response). Note extensive hilar neuron loss (an average of 85% hilar cell loss; n = 4; range, 68–94%). D1, D2, NeuN and c-Fos expression 3 d after 24 hr of PP stimulation, which resulted in a failure to evoke translamellar inhibition despite effective BMI-induced activation of granule cells (Fig. 4C3). In six PP-stimulated animals, the average hilar neuron loss was 93% (range, 89–95%). E, Graph showing the correlation between BMI-induced suppression of the second evoked population spike amplitude recorded at the saline electrode and the number of hilar neurons surviving at the septo-temporal level of the BMI electrode. The group means for cell number (*) and the degree of second spike suppression (+) in both the KA type 2 and PP stimulation groups were significantly different from the control and KA type 1 groups (p < 0.05); the latter were not significantly different from each other (p > 0.05). Scale bar, 100 µm. Magnification, 64x.
The close correlation between hilar neuron loss and translamellar disinhibition in KA-treated rats was also addressed in rats previously subjected to prolonged, unilateral PP stimulation, because this paradigm reliably produces extensive hilar cell loss throughout the dorsal hippocampus without involving behavioral SE or producing any significant extra-hippocampal damage (Sloviter, 1983Three days after the end of 24 hr of intermittent PP stimulation, BMI-induced granule cell discharges failed consistently to evoke distant inhibition (n = 6) (Fig. 4C2,C4; Table 1). Compared with controls (n = 4), previously PP-stimulated rats exhibited an average of 93% fewer hilar neurons (4.6 ± 0.7 hilar neurons per section; range, 89–95% fewer neurons; n = 6; p < 0.01) at the dorsal hippocampal BMI electrode site (Fig. 5D1,D2). Injury was also apparent in area CA3c of PP-stimulated animals (Fig. 6C1), but no obvious injury was detected in the temporal neocortex or in any other brain regions. Thus, unilateral 24 hr intermittent PP stimulation, which has been shown previously to produce primarily unilateral hilar neuron loss (Sloviter, 1991
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Figure 6. Loss or survival of dorsal hippocampal hilar neurons corresponds to loss or preservation of translamellar inhibition. A, In a rat subjected to prolonged PP stimulation 3 d before, distant translamellar inhibition evoked at the saline electrode by focal granule cell discharges was abolished (A1); top trace, before distant BMI-induced granule cell discharges; bottom trace, after BMI diffusion. Note selective and extensive loss of hilar neurons (A2, Nissl-stained sections) but survival of adjacent CA3 pyramidal cells (A3). B, In a rat subjected to KA-induced SE 3 d before, translamellar inhibition (B1) and dorsal hilar (B2) neurons were preserved, whereas CA3 pyramidal cells had degenerated (B3). C1, C2, Fluoro-Jade B-stained dorsal (C1) and ventral (C2) sections from a KA-treated animal. Note that brightly fluorescent cell bodies and processes reflect acute degeneration. Despite extensive injury to dorsal hippocampal CA1–CA3 pyramidal cells (C1), ventral dentate hilar neurons (h), and CA1 pyramidal cells and temporal cortical nuclei including the lateral entorhinal cortex (LEnt; C2), translamellar inhibition was preserved, and the only apparently undamaged hippocampal region in this animal was the dorsal dentate gyrus (C1, asterisk). Calibration: A1–B2, 5 mV and 10 msec. Scale bar: A2, B2, 100 µm; A3, B3, 356 µm; C1, C2, 237 µm. Magnification: A2, B2, 46x; A3, B3, 14x; C1, C2, 19x.
Figure 7 illustrates the correlation between hilar neuron loss at the BMI electrode site and the loss of translamellar inhibition. The clustering together of all 10 disinhibited animals (six PP-stimulated rats and four KA type 2 rats) at the origin of the x- to y-axes, and the more scattered distribution of all controls and KA type 1 animals, suggests that translamellar disinhibition was uniquely associated with extensive hilar cell loss, whereas partial hilar cell loss produced no obvious granule cell disinhibition (Fig. 7), as demonstrated previously by Milgram et al. (1991
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Figure 7. Correlation between hilar neuron loss and loss of translamellar inhibition. The average number of Nissl-stained hilar neurons per section from each of 31 rats tested is plotted against the percentage of suppression of the second of two granule cell population spikes evoked by PP stimulation at 0.3 Hz in control, KA-treated, and 24 hr PP-stimulated rats. There was a correlation between the number of hilar neurons and the degree of second spike suppression (r2 = 0.68). Although the data display a somewhat linear relationship, there was a distinct clustering of data points. All rats that exhibited a failure of translamellar inhibition (4 KA type 1 and all 6 PP-stimulated rats) were subsequently found to have extensive hilar neuron loss and were clustered close to the origin of the x- to y-axes. Conversely, all control and KA type 1 rats exhibited intact second spike suppression and relative hilar neuron preservation.
Longitudinal associational projections of hippocampal inhibitory interneurons
Despite our hypothesis that longitudinally projecting hilar mossy cells evoke translamellar inhibition by exciting inhibitory neurons (Sloviter, 1991FG injection produced a large FG-labeled region that involved all dentate gyrus laminas and the CA1 region above the injection target site, as illustrated previously (Zappone and Sloviter, 2001
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Figure 8. Retrograde transport of FG from the saline electrode site to the BMI electrode site. The retrograde tracer FG was used to identify the hippocampal neuron subtypes with axonal projections spanning the longitudinal distance over which translamellar inhibition was evoked. A, At the approximate outer edge of the FG injection zone, all neuronal subpopulations in the dentate gyrus were FG immunopositive, including granule cells, hilar neurons (h), and presumed interneurons of the granule cell layer [arrows in stratum granulosum (sg)]. B, C, GAD67- and FG-immunostained sections, respectively, at the
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Figure 9. Limited longitudinal transport of the retrograde tracer FG by hippocampal interneurons. A1, Immunocytochemical localization of the neuronal marker NeuN shows the normal location and number of hippocampal principal cells and interneurons in the dorsal hippocampus. A2, In a section
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Figure 10. Longitudinal transport of FG by dentate hilar neurons. A, Colocalization of FG (green) and GluR2 (red) immunoreactivities
In the hippocampus proper, the steep longitudinal decline in FG labeling of interneurons included the large populations of hippocampal interneuron somata in strata oriens, radiatum, and lacunosum-moleculare (Fig. 9A, A2). One consistent exception was a small number of intensely FG-immunolabeled interneurons at the stratum radiatum/lacunosum-moleculare border and in the stratum oriens (Fig. 9A2). Thus, our ability to detect intense FG immunoreactivity in a small number of interneurons relatively far (>2 mm) from the FG injection site indicates the effectiveness of the methods we used to detect FG in interneurons and demonstrates that the vast majority of interneurons, including all basket cell somata of all hippocampal principal cell layers, did not transport even a minimally detectable concentration of FG 2–4 mm from the injection site. Results of the FG control injections indicated that the FG labeling of dentate gyrus neurons was the result of site-specific transport of FG from the dentate gyrus injection site. Neither FG injection into area CA1 above the dentate gyrus, nor into the neocortex above the dentate gyrus, labeled any dentate gyrus neurons.As described previously after injection of retrograde tracer into the anterior hippocampus (Qiu and Han, 1995
Quantitative analysis of sections progressively distant from the FG injection site revealed that the proportion of hilar FG-positive neurons that were also GluR2 positive increased as the distance from the tracer injection site increased, whereas the proportion of FG-labeled neurons that were SS or PV positive decreased progressively and precipitously (Fig. 10). Within the region
Retrograde labeling of SS-positive hilar neurons after septal or hippocampal FG injection
Given the consistently infrequent and weak FG labeling of SS-positive hilar interneurons after intrahippocampal FG injection, we next determined whether these interneurons lack the ability to transport FG in concentrations that result in intense labeling. This experiment addressed the possibility that SS-positive hilar interneurons might have extensive associational projections, as suggested by Buckmaster and Schwartzkroin (1995
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Figure 11. Retrograde transport of FG by dentate hilar neurons after FG injection into the rostral hippocampus or the medial septum. A1, A2, After FG injection into the rostral hippocampus, hilar neurons were labeled
Discussion
The main findings of this study are, first, that the net translamellar influence of focal granule cell discharges on distant granule cells was inhibition, not excitation. Second, translamellar inhibition was abolished by SE whenever extensive hilar neuron loss resulted and by prolonged PP stimulation, which consistently produced extensive hilar neuron loss but minimal extra-hippocampal damage. Third, retrograde tracing indicated that: (1) mossy cells form extensive longitudinal axon projections spanning the distance over which translamellar inhibition was evoked; (2) basket cells and chandelier cells appear to have extremely limited longitudinal axonal projections; and (3) with rare exceptions, SS-positive interneurons form sparse and longitudinally limited axonal projections, despite sending extensive projections to the more distant septum.Translamellar inhibition rather than excitation
Although mossy cells have been hypothesized to constitute a recurrent excitatory system that links distant granule cells together (Amaral and Witter, 1989These results are consistent with previous conclusions that inhibitory interneurons are the primary targets of the excitatory associational–commissural pathway, which also produced commissural granule cell inhibition rather than excitation (Buzsáki and Eidelberg, 1982
Translamellar disinhibition as a possible consequence of hilar neuron loss
That the translamellar disinhibition we observed in lesioned animals was attributable to hilar neuron loss, rather than other effects of prolonged SE, is supported by the observation that all KA-treated rats exhibited SE lasting >3 hr, and all exhibited hippocampal and extrahippocampal damage. The main difference we detected between KA-treated rats with intact or impaired translamellar inhibition was the extent of hilar cell loss. More conclusively, identical translamellar disinhibition was reproduced by prolonged PP stimulation, which reliably produced extensive hilar neuron loss but little other damage. However, other undetected effects of prolonged granule cell discharges that might uniquely parallel hilar neuron injury, such as downregulation of GABAA receptors in granule cells (Brooks-Kayal et al., 1998Our finding that only extensive hilar cell loss was reliably associated with translamellar disinhibition explains why a previous study failed to observe translamellar disinhibition in KA-treated rats (Buckmaster and Dudek, 1997
Longitudinal projections of dentate inhibitory interneurons
The identity of neurons capable of mediating translamellar inhibition was addressed by our retrograde transport studies, which confirmed that mossy cells are the only dentate neuron population with significant longitudinal projections spanningPossible functional implications
Lamellar function may be established by inhibitory interneurons acting locally to focus strong excitation to local targets (intralamellar lateral inhibition) and by mossy cells establishing lateral inhibition in surrounding lamellae to increase the "signal-to-noise" ratio. Our finding that few inhibitory interneurons were FG labeled by relatively close FG injections suggests that inhibitory interneurons in one segment are unlikely to contribute significantly to lateral inhibition in distant segments. However, given the observation that individual inhibitory interneurons can have widely divergent influences on large numbers of principal cells (Cobb et al., 1995Regardless of which cell types and synaptic mechanisms mediate translamellar inhibition in the dentate gyrus, the present data support the concept of functional separation in the granule cell layer as a consequence of inhibitory translamellar impulses (Andersen et al., 1966
Finally, an extensive loss of hilar inhibitory interneurons (deLanerolle et al., 1989
Footnotes
Received July 18, 2003; revised November 25, 2003; accepted November 25, 2003.This work was supported by National Institutes of Health Grant NS18201. We thank Dr. Hemant Kudrimoti for constructive criticism of this manuscript.
Correspondence should be addressed to Dr. R. S. Sloviter, Department of Pharmacology, University of Arizona College of Medicine, 1501 North Campbell Avenue, Tucson, AZ 85724-5050. E-mail: sloviter{at}u.arizona.edu.
DOI: 10.1523/JNEUROSCI.1619-03.2004
Copyright © 2004 Society for Neuroscience 0270-6474/04/240853-12$15.00/0
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