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The Journal of Neuroscience, January 26, 2005, 25(4):971-976; doi:10.1523/JNEUROSCI.3489-04.2005
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BRIEF COMMUNICATION
Evidence That Disinhibition Is Associated with a Decrease in Number of Vesicles Available for Release at Inhibitory Synapses
Veronica A. Ledoux andCatherine S. Woolley Department of Neurobiology and Physiology and Northwestern University Institute for Neuroscience, Northwestern University, Evanston, Illinois 60208
Abstract
Top
Abstract
Introduction
We used three-dimensional reconstruction from serial electron micrographs to investigate two structural changes that could underlie estrogen-induced disinhibition of hippocampal CA1 pyramidal cells: a decrease in the number of inhibitory inputs per neuron and/or a change in inhibitory boutons that could limit GABA release. We analyzed 373 boutons forming 510 inhibitory synapses in estrogentreated and control animals. Our results show that estrogen specifically decreases the number of synaptic vesicles adjacent to the presynaptic membrane of inhibitory synapses without affecting the overall number of vesicles. We detected no difference in the density of inhibitory inputs. These findings provide a novel mechanism for the functional effects of estrogen on synaptic inhibition and represent the first in vivo evidence that the number of presynaptic vesicles available for release is a regulated property of synapses that affects synaptic physiology.
Key words: estrogen; hippocampus; GABA; IPSC; paired-pulse depression; serial reconstruction
Introduction
Synaptic transmission depends on neurotransmitter release from vesicles that are docked at the presynaptic membrane and primed for membrane fusion and exocytosis (Sudhof, 1995). Presynaptic action potentials evoke transmitter release with a probability less than 1. Although many factors can influence probability of release, studies of excitatory synapses in the hippocampus indicate that release probability is positively related to the size of a readily releasable pool of vesicles (Dobrunz and Stevens, 1997
Despite these correlations, at least two studies challenge the view that the number of docked vesicles parallels release probability. Ultrastructural comparisons of synapse types with very different release probabilities, parallel fiber versus climbing fiber inputs to cerebellar Purkinje cells (Xu-Friedman et al., 2001
As an alternative approach to address the relationship between presynaptic vesicles and synaptic function, we compared one type of synapse in two hormonal states with known physiological differences. Previously, we showed that 24 h of estrogen treatment disinhibits hippocampal CA1 pyramidal cells by suppressing GABAergic synaptic transmission. Estrogen decreases the amplitude of evoked IPSCs, decreases the frequency of miniature IPSCs (mIPSCs) (Rudick and Woolley, 2001
To investigate these possibilities, we analyzed axosomatic inhibitory synapses on CA1 pyramidal cells in estrogen-treated and control rats using serial reconstruction electron microscopy. Our results show that estrogen-induced disinhibition is paralleled by a profound and specific decrease in the number of synaptic vesicles adjacent to the presynaptic membrane (i.e., those in position to be released). We found no decrease in the density of inhibitory inputs. These findings provide the first in vivo evidence that the number of vesicles available for release is a regulated property of synapses that influences synaptic physiology and support the idea that release probability is related to the size of a releasable vesicle pool at hippocampal inhibitory synapses.
Materials and Methods
Hormone treatment and tissue processing. The Northwestern University Animal Care and Use Committee approved all of the animal procedures. Eight adult female Sprague Dawley rats (180-220 g) were ovariectomized (OVX) under ketamine (85 mg/kg, i.p.) and xylazine (13 mg/kg, i.p.) anesthesia. Three days later, four rats received a 10 µg subcutaneous injection of 17-estradiol benzoate (OVX+E) in sesame oil vehicle, and the other four received oil alone (OVX+O). Twenty-four hours later, the animals were anesthetized with Nembutal (80 mg/kg, i.p.) and perfused with heparinized saline, followed by 2.5% paraformaldehyde/0.5% glutaraldehyde in 0.1 M phosphate buffer, pH 7.4. After perfusion, brains were postfixed overnight at 4°C. Dorsal hippocampal blocks were cut at 100 µm, stained for 1 h with 1% osmium tetroxide, dehydrated in graded ethanols, flat embedded in epoxy resin, and trimmed to contain CA1. Between 60 and 130 serial thin (
80 nm) sections per block were collected on Formvar-coated slot grids.
Separate sets of sections were collected on nickel grids for postembedding immunogold labeling for GABA. Periodic acid/sodium periodate-etched sections were incubated in 1:500 rabbit anti-GABA IgG (Sigma, St. Louis, MO) for 2 h, followed by 1:20 goat anti-rabbit IgG-20 nm colloidal gold (Ted Pella, Redding, CA) for 1 h. All of the sections were counterstained with 3% uranyl acetate, followed by 2.66% Reynold's lead citrate, and then examined with a JEOL (Peabody, MA) 100CXII electron microscope. Tissue was coded so that investigators were blind to hormone treatment conditions until all of the reconstructions and analyses were complete.
Image acquisition and analysis. For each brain, one 600x image in the middle of a series was used to randomly select four CA1 pyramidal cells for analysis. For each section, two to three micrographs at 10,000x were taken per cell; negatives were scanned (1600 dots per inch) and montaged to form a 16-20 µm perimeter of the cell membrane. This was repeated through 60-80 serial sections, and then images were aligned using SEM Align (K. M. Harris, Medical College of Georgia, Augusta, GA and J. C. Fiala, Boston University, Boston, MA; www.synapses.mcg.edu). For each section, the somatic membrane, apposed glial profiles, boutons forming symmetric synapses and/or containing pleiomorphic vesicles, presynaptic densities, and presynaptic vesicles were traced and quantified in IGL Trace (www.synapses.mcg.edu). Synapses were identified as apposed electron-dense regions on bouton and soma membrane having at least three vesicles in the bouton within 50 nm of the presynaptic membrane. Each measured variable was averaged to obtain a single mean value per animal (n = 4 for all of the comparisons). We used unpaired, two-tailed Student's t tests to compare means, Pearson's test for correlations, and the Kolmogarov-Smirnov test to compare distributions. All of the data are presented as mean ± SEM. Illustrative images were made using 3D Studio Max 4 (Autodesk, San Raphael, CA).
Results
We used serial-section electron microscopy to investigate two mechanisms for estrogen-induced disinhibition of hippocampal CA1 pyramidal cells: a decrease in the number of inhibitory boutons in synaptic contact with pyramidal cells and/or a decrease in GABA release at individual synapses. We focused on axosomatic inhibitory synapses because inhibitory innervation of CA1 pyramidal cells is most concentrated at the soma (Megias et al., 2001Before analyzing synaptic inputs in serial sections, we first confirmed that we could reliably identify GABAergic boutons based on two morphological criteria: pleiomorphic vesicles and symmetric presynaptic and postsynaptic densities. In sections labeled for GABA using postembedding immunogold (Fig. 1A), we found that 247 of 259 (95%) axosomatic boutons (184 of 192 OVX+O and 63 of 67 OVX+E) that fulfilled both criteria were also GABA positive. Given that we could identify the vast majority of GABAergic boutons morphologically, we proceeded with serial reconstruction using nonimmunolabeled tissue because procedures for immunolabeling compromise ultrastructure quality.
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Figure 1. Estrogen does not affect glial ensheathment or density of inhibitory inputs. A, Immunogold labeling for GABA shows GABAergic boutons apposed to a CA1 pyramidal cell soma. Boutons are highlighted in blue; glia are highlighted in green; red arrows indicate synaptic densities. Note that gold particles (black dots) selectively label boutons. B1, B2, Reconstructed patches of CA1 pyramidal cell soma (gray), apposed boutons (blue), and glia (green) from an OVX+O (B1) and OVX+E(B2) cell. Scale bars: A, 500 nm; B, 2 µm. C, D, Neither percentage of somatic surface apposed by glia (C) nor synaptically connected bouton density (D) is significantly affected by estrogen (mean ± SEM; n = 4). O, OVX+O; E, OVX+E. Error bars represent SEM.
Estrogen does not affect glial ensheathment or density of inhibitory inputs
Initially, we favored the hypothesis that estrogen-induced disinhibition is attributable to a decrease in inhibitory synapse number because of a precedent in the arcuate nucleus of the hypothalamus. Perez et al. (1993To evaluate glial hypertrophy and axosomatic bouton displacement in the hippocampus, we reconstructed patches of CA1 pyramidal cell body membrane, as well as glial processes and inhibitory boutons apposed to each patch (Fig. 1B). Patches from four cells in each of four OVX+O and four OVX+E animals were reconstructed from 60-80 serial electron micrographs per cell. Each patch was
Estrogen decreases the number of vesicles adjacent to the presynaptic membrane
Subsequently, we considered the possibility that estrogen produces a change in presynaptic boutons that could limit GABA release. A total of 373 axosomatic boutons forming 510 inhibitory synapses (OVX+O, 166 boutons forming 219 synapses; OVX+E, 207 boutons forming 291 synapses) that were completely contained within our series were used to quantify bouton volume, presynaptic density area, and vesicle number, density, and location. Boutons contained only partially within a series were excluded. The number of synapses is greater than the number of boutons because some boutons form multiple synapses. With the exception of vesicle location (see below), none of the measured parameters was significantly affected by estrogen (Table 1). As observed for excitatory synapses in the hippocampus (Harris and Sultan, 1995
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Table 1. Ultrastructural characteristics of axosomatic boutons and symmetric synapses
In contrast to other parameters examined, analysis of vesicle location revealed that estrogen produced a profound decrease in the number of vesicles adjacent to the presynaptic density. For each synapse, we quantified the number of vesicles located 0-30, 31-50, or51 nm from the presynaptic membrane. We chose 30 nm as the limit of the closest range because this is the shortest distance from a synapse that we could measure reliably. Because our experimental design involved the evaluation of all of the synapses within a particular volume of tissue, some synapses or parts of synapses were sectioned obliquely; in these cases, it was not possible to confirm all of the vesicles that were physically associated with the presynaptic membrane. However, this distance range is within that reported by others to reflect docked vesicles [e.g., 0-70 nm (Schikorski and Stevens, 2001
Reconstructed synapses from OVX+O (Fig. 2A,C) and OVX+E (Fig. 2B,D) animals were used to quantify the number of vesicles within 30 nm of the presynaptic membrane (Fig. 2E-H). As has been shown for excitatory synapses, the number of vesicles near the presynaptic membrane at inhibitory synapses was highly variable, ranging from 0 to 61. Interestingly, estrogentreated animals had more than twice as many synapses with no vesicles within 30 nm, although this was a small proportion of synapses overall. OVX+E animals had 13.8 ± 1.7% synapses with zero vesicles within 30 nm compared with 5.6 ± 1.8% in OVX+O animals (p < 0.01) (Fig. 2E,F). Among synapses that did contain vesicles within 0-30 nm, the distribution was significantly shifted toward fewer vesicles in OVX+E animals (p < 0.01) (Fig. 2G). This shift led to, on average, one-half as many vesicles adjacent to the presynaptic membrane in estrogen-treated animals compared with controls. OVX+E animals had 6.2 ± 1.3 vesicles within 30 nm of the presynaptic membrane, whereas OVX+O animals had 12.1 ± 1.2 vesicles within this range (p = 0.01) (Fig. 2H). This decrease in number of vesicles near the synapse was paralleled by a decrease in vesicle density. The density of vesicles from 0 to 30 nm was 440 ± 74 vesicles/µm3 in OVX+E compared with 828 ± 95 vesicles/µm3 in OVX+O (p = 0.02). Slightly farther from the synapse, 31-50 nm, the average number of vesicles was lower in OVX+E animals (15.6 ± 3.4) compared with OVX+O animals (24.1 ± 4.5), but this difference was not statistically significant (p = 0.19). Similarly, the number of vesicles
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Figure 2. Estrogen decreases the number of vesicles adjacent to the presynaptic membrane. A, B, Individual boutons and three serial sections from representative OVX+O (A1-A4) and OVX+E (B1-B4) synapses. Scale bar, 150 nm. C, D, Reconstructed presynaptic densities (red) and vesicles within 0-30 nm (yellow) and 31-50 nm (dark gold) of the same OVX+O (C) and OVX+E (D) synapses. E, F, Histograms of percentage of synaptic densities on OVX+O (E) and OVX+E (F) cells containing variable numbers of vesicles with in 30 nm of the presynaptic membrane; data are from all of the cells analyzed. Note the shift toward fewer vesicles in OVX+E. G, Cumulative histograms of data in E and F (p < 0.01). H, Number of vesicles 0-30 nm from the presynaptic membrane is reduced at OVX+E compared with OVX+O synapses (mean ± SEM; n = 4; *p = 0.014). O, OVX+O; E, OVX+E. Error bars represent SEM.
Discussion
The results presented here show that estrogen-induced disinhibition of hippocampal CA1 pyramidal cells is associated with a decrease in the number of vesicles adjacent to the presynaptic membrane of inhibitory synapses (i.e., those vesicles most likely to be readily releasable). A reduction in the number of releasable vesicles provides a novel mechanism for the functional effects of estrogen on GABAergic inhibition. Each of the previously established electrophysiological effects of estrogen is consistent with a reduction in GABA release: decreased amplitude of evoked IPSCs, decreased frequency, but not amplitude, of mIPSCs (Rudick and Woolley, 2001To our knowledge, this is the first demonstration in vivo that the number of neurotransmitter vesicles available for release is a regulated property of synapses that affects synaptic physiology. Studies in the 1970s and 1980s showed that sensory or electrical stimulation in vivo can acutely alter the distribution of presynaptic vesicles (Feher et al., 1972
Release probability, paired-pulse depression, and the docked vesicle pool
Release probability is a critical variable in synaptic function. One way to assess release probability is with paired-pulse experiments, in which two synaptic stimuli are given in close succession and the postsynaptic response evoked by the second pulse is compared with that evoked by the first. At GABAergic synapses on CA1 pyramidal cells, the second response tends to be depressed compared with the first (Davies et al., 1990On one hand, this relationship between paired-pulse depression and release probability might be explained by depletion of release sites. For example, if, after releasing a single vesicle, a release site becomes refractory until some repriming event occurs, then the pool of potential release sites would be depleted temporarily. Thus, when the probability is high that any site will release a vesicle, a greater fraction of sites releases on the first stimulus, leaving relatively fewer sites capable of release on the second stimulus, leading to depression. Conversely, when release probability is low, less depression is observed because a relatively greater fraction of release sites remains capable of release on the second stimulus. Given the positive relationship between the number of docked vesicles and release probability shown for hippocampal excitatory synapses (Dobrunz and Stevens, 1997
On the other hand, the situation is not necessarily so simple. Two previous serial electron microscopic studies that compared docked vesicle number at different types of synapses with high versus low release probability and correspondingly different behavior in paired-pulse experiments showed either no difference (Xu-Friedman et al., 2001
Our findings add a new piece to this complex puzzle and support the idea that release probability, paired-pulse depression, and the docked vesicle pool are directly related. The approach was to evaluate the same type of synapse in two hormonal states with known differences in physiology. Previous studies established that the same estrogen treatment used here decreases the amplitude of IPSCs evoked by single stimuli and reduces paired-pulse depression. Together, these data suggest a scenario in which an estrogen-induced decrease in the number of vesicles available for release at inhibitory synapses reduces release probability, resulting in GABA release from fewer release sites and, consequently, smaller evoked IPSCs and less depression of the second IPSC in paired-pulse experiments. Estrogen may also affect nonstructural parameters that influence release probability and/or synaptic depression. However, whether or not such additional effects exist, our data suggest a model in which release probability at inhibitory synapses in CA1 is related to the size of the releasable pool of vesicles, and depletion of release sites could contribute to synaptic depression.
Estrogen action in the hippocampus
In addition to its effects on inhibitory synapses, estrogen also regulates excitatory synapses in CA1. Seventy-two hours of estrogen treatment increases the density of dendritic spines and excitatory synapses on CA1 pyramidal cells, increases the sensitivity of CA1 pyramidal cells to excitatory synaptic input, enhances long-term potentiation (for review, see Woolley, 1998The classical mechanism of estrogen action is via nuclear transcription factor receptors. A curious aspect of the effects of estrogen in the dorsal hippocampus is the paucity of cells that express nuclear estrogen receptors (ERs). The few cells in dorsal CA1 that do express nuclear ERs are GABAergic neurons, but this is only a small subset of all of the GABAergic neurons in the region (Hart et al., 2001
Footnotes
Received Aug 24, 2004; revised December 8, 2004; accepted December 13, 2004.This work was supported by National Institutes of Health Grants NS 37324 and MH 067564, the W. M. Keck Foundation, and the Northwestern University Biological Imaging Facility. We thank Dr. Indira Raman for helpful comments on this manuscript.
Correspondence should be addressed to Catherine S. Woolley, Department of Neurobiology and Physiology, 2205 Tech Drive, Northwestern University, Evanston, IL 60208. E-mail: cwoolley{at}northwestern.edu.
Copyright © 2005 Society for Neuroscience 0270-6474/05/250971-06$15.00/0
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