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The Journal of Neuroscience, August 30, 2006, 26(35):8881-8891; doi:10.1523/JNEUROSCI.1302-06.2006
Previous Article | Next Article
Development/Plasticity/Repair
Cooperative Astrocyte and Dendritic Spine Dynamics at Hippocampal Excitatory Synapses
Michael Haber, Lei Zhou, andKeith K. Murai Centre for Research in Neuroscience, Department of Neurology and Neurosurgery, The Research Institute of the McGill University Health Centre, Montreal General Hospital, Montreal, Quebec, H3G 1A4, Canada
Abstract
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Abstract
Introduction
Accumulating evidence is redefining the importance of neuron–glial interactions at synapses in the CNS. Astrocytes form "tripartite" complexes with presynaptic and postsynaptic structures and regulate synaptic transmission and plasticity. Despite our understanding of the importance of neuron–glial relationships in physiological contexts, little is known about the structural interplay between astrocytes and synapses. In the past, this has been difficult to explore because studies have been hampered by the lack of a system that preserves complex neuron–glial relationships observed in the brain. Here we present a system that can be used to characterize the intricate relationship between astrocytic processes and synaptic structures in situ using organotypic hippocampal slices, a preparation that retains the three-dimensional architecture of astrocyte–synapse interactions. Using time-lapse confocal imaging, we demonstrate that astrocytes can rapidly extend and retract fine processes to engage and disengage from motile postsynaptic dendritic spines. Surprisingly, astrocytic motility is, on average, higher than its dendritic spine counterparts and likely relies on actin-based cytoskeletal reorganization. Changes in astrocytic processes are typically coordinated with changes in spines, and astrocyte–spine interactions are stabilized at larger spines. Our results suggest that dynamic structural changes in astrocytes help control the degree of neuron–glial communication at hippocampal synapses.
Key words: plasticity; glia; motility; cross talk; neuron–glia; organotypic slices
Introduction
Structural modifications to cellular components are critical for establishing and remodeling connections within the nervous system. Recent studies have offered unprecedented views of structural changes at neuromuscular (Walsh and Lichtman, 2003; Bishop et al., 2004
Surprising roles for glial cells in synapse development and physiology have recently emerged (Castonguay et al., 2001
Intriguingly, astrocytes display morphological rearrangements in acute brainstem and organotypic hippocampal slices (Hirrlinger et al., 2004
Materials and Methods
Semliki Forest virus plasmid construction and virus preparation. For expressing fluorescent proteins in hippocampal slices, Semliki Forest virus (SFV) constructs were created (Ehrengruber et al., 1999Tissue preparation and hippocampal slice culture. For diolistic labeling of neurons and astrocytes in the hippocampus, 300 µm hippocampal slices were created using a McIllwain tissue chopper (Stoelting, Kiel, WI) and immediately fixed in 4% paraformaldehyde/0.1 M PO42– buffer for 30 min. Tungsten particles (1.3 µm) (Bio-Rad, Hercules, CA) carrying the lipophilic dyes DiI or DiO (Invitrogen, Carlsbad, CA), were prepared as described previously (Gan et al., 2000
Organotypic hippocampal slices were prepared as described previously (Stoppini et al., 1991
7.2). Media were replaced every 2 d, and slices were cultured for 1–3 weeks before viral gene delivery. At 16–20 h after infection, slices were either fixed for static confocal imaging or used for time-lapse imaging experiments.
Immunofluorescence on hippocampal slices. Immunofluorescence on hippocampal slices was performed as described previously (Murai et al., 2003
Static and time-lapse confocal imaging. Static confocal imaging was performed using an Ultraview spinning disk confocal system (PerkinElmer, Wellesley, MA) connected to an Eclipse TE2000 (Nikon, Tokyo, Japan) equipped with a 60x oil immersion lens (1.25 numerical aperture with 1.5x optical zoom; Nikon). Z-stacks were collected using MetaMorph imaging software (Molecular Devices, Palo Alto, CA) and deconvoluted in three dimensions using Autodeblur software (AutoQuant, Media Cybernetics, Silver Spring, MD). A calculated point-spread function optimized for spinning disk confocal microscopy was used. For time-lapse imaging, an Ultraview spinning disk system was connected to a Leica (Nussloch, Germany) DMS upright microscope equipped with a 63x extra-long working distance lens (Leica). Hippocampal slices were secured in a heated electrophysiology chamber (Warner Instruments, Hamden, CT) and perfused with oxygenated artificial CSF (ACSF) (125 mM NaCl, 3 mM KCl, 1.25 mM NaH2PO4, 26 mM NaHCO3, 2.4 M CaCl2, and 10 mM glucose, 95% O2/5% CO2) that was heated to 32–34°C (Warner Instruments). Z-stacks were taken at 3 min intervals unless specified otherwise using MetaMorph software. In pharmacology experiments, baseline time-lapse images were collected before treatment of slices with ACSF containing cytochalasin-D (5 µM; Sigma) or bicuculline methochloride (20 µM; Sigma). Imaging was resumed 3 min after the start of the drug treatment.
Measurements and quantifications. For quantification of spine and astrocytic process motility, a motility index was computed for astrocytic processes adjacent to spines similar to Dunaevsky et al. (1999)
Three-dimensional reconstructions. For Figures 3, g and h, and 4 and supplemental Figure 2 (available at www.jneurosci.org as supplemental material), deconvoluted confocal Z-stacks were rendered in three dimensions using IMARIS 4.5.2 (Bitplane, Zurich, Switzerland). For Figure 4 and supplemental Figure 2 (available at www.jneurosci.org as supplemental material), synaptophysin and GLT-1/EAAT-2 proximity to dendrites were determined by masking the synaptophysin or GLT-1/EAAT-2 channel with a second three-dimensional rendering of the dendritic segment extending
Three-dimensional quantifications. For quantification of astrocytic process extension and retraction (see Fig. 5), individual astrocytic processes from deconvoluted Z-stacks were isolated using contour surfaces (IMARIS MeasurementPro; Bitplane) and rendered in three dimensions (IMARIS 4.5.2; Bitplane). Volume changes were plotted over time.
For quantifications in Figure 8, dendritic segments containing spines that were encompassed within an astrocyte domain were chosen for analysis (with the assumption that each astrocyte occupies its own territory) (see Fig. 2). For three-dimensional quantification of dendritic spine–astrocyte profiles, contour surfaces (IMARIS MeasurementPro; Bitplane) were first used to separate dendritic shafts from spines or spine heads. Three-dimensional surfaces of spines were generated and used to mask the surrounding astrocytic channel, leaving only the overlap between spines and astrocytic processes (IMARIS 4.5.2; Bitplane). Surfaces of the overlap, or astrocytic profile, of each spine were generated and used to track volume changes. To control for artifacts caused by minor fluctuations in signal intensity or sample photobleaching, multiple dendritic shaft segments along each quantified region were used to adjust surface thresholds for spine and astrocytic profile volume rendering at each time point (supplemental Fig. 1, available at www.jneurosci.org as supplemental material). We assumed that dendritic shaft segments were stable structures over the imaging period. In Figure 8b, percentage volume change was determined by comparing the minimum and maximum value of both spine and astrocytic profile volume over six time points at 3 min intervals (15 min total; n = 32 pairs of astrocytes and spines over three experiments taken at 3 weeks in vitro).
Results
Comanipulation of neurons and astrocytes in hippocampal slices
Recent studies have described dynamic morphological changes at synapses in the nervous system with particular emphasis on postsynaptic dendritic spines (Dailey and Smith, 1996
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Figure 1. Targeting complex neuron–glial interactions in the hippocampus using organotypic hippocampal slices and viral gene delivery. a, SFV constructs used in the study. EGFPf or RFPf were cloned after the genes encoding viral nonstructural proteins and a subgenomic promoter (arrow) on SFV plasmids. b, c, Confocal images showing examples of apical dendrites with prominent spines on CA1 pyramidal neurons infected with SFV PD EGFPf (b, green) or SFV PD RFPf (c, red). d–f, Low-magnification epifluorescence images showing the selectivity of SFV A7 for protoplasmic astrocytes in the stratum radiatum of area CA1. Infected astrocytes expressing EGFPf (d, green; arrowheads) are labeled for GFAP (e, red). g–i, Single-plane confocal images of an SFV A7-infected astrocyte showing EGFPf expression (g, green) and GFAP immunoreactivity (h, red). Note how the GFAP immunolabeling only labels the main processes of the infected protoplasmic astrocyte, whereas EGFPf reveals the fine processes (i). Scale bars: b, c, 5 µm; d–i, 10 µm.
To deliver genes to astrocytes, we modified a nonvirulent strain of SFV that is known to infect glial cells (SFV A7) (Ehrengruber et al., 2003Preservation of complex three-dimensional glial–glial and neuron–glial interactions in organotypic hippocampal slices
We observed that EGFPf- or RFPf-expressing astrocytes in hippocampal slice cultures retained their complex three-dimensional morphologies, similar to what has been described with Golgi labeling or single-cell injections of fluorescently labeled probes into fixed brain tissue (Bushong et al., 2002
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Figure 2. Astrocytic elaboration and domain spacing in area CA1 of the adult mouse hippocampus and in organotypic slice culture. a–c, Diolistic labeling of protoplasmic astrocytes in fixed hippocampal tissue. Maximum projections of confocal images of neighboring astrocytes labeled with DiI (a, red) and DiO (b, green) reveals their distinct domain spacing. d–f, Astrocytes in organotypic hippocampal slice culture also occupy distinct territories. Maximum projections of confocal images of adjacent astrocytes expressing RFPf (d, red) and EGFPf (e, green) after 1 week in vitro. The dashed lines in c and f indicate the boundary between neighboring astrocytes. Scale bars, 10 µm.
We next turned our analysis to complex neuron–astrocyte interactions in the stratum radiatum of area CA1. Intricate three-dimensional interactions between astrocytes and neurons have been described using serial electron microscopy (Ventura and Harris, 1999
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Figure 3. Complex neuron–glial interactions in the hippocampal CA1 neuropil. a–c, Confocal maximum projections of a DiI-labeled apical dendrite from a CA1 pyramidal cell (a, red) extending through a DiO-labeled astrocyte domain (b, green) in a fixed slice of the adult hippocampus. Areas of overlap show the complexity of neuron–glial interactions. d–f, Confocal maximum projections of a dendrite from an SFV PD RFPf-infected CA1 pyramidal neuron (d, red) projecting through an SFV A7 EGFPf-infected astrocyte domain (e, green) after 1 week in vitro. g, h, Three-dimensional reconstructions of the boxed areas in f, demonstrating the complex interplay between astrocytic processes and dendritic spines. Inset in h shows the neuron–glial association rotated 90°. Arrowheads show examples of astrocytic processes extending toward spines. Scale bars, 5 µm.
We confirmed that the majority of dendritic spines in our slice culture system were associated with presynaptic terminals (Fig. 4). After 1 and 3 weeks in culture, we subjected slices to immunolabeling with anti-synaptophysin antibodies. As depicted in Figure 4, the majority of spines showed synaptophysin labeling adjacent to RFPf-labeled dendritic spines, indicating that most of the spines have presynaptic innervation. Altogether, these results indicate that many of the properties of astrocyte–astrocyte, neuron–astrocyte, and neuron–neuron interactions are maintained and easily visible in three dimensions in organotypic slice culture.
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Figure 4. Dendritic spines are innervated in hippocampal slice culture. a, b, SFV PD RFPf-infected slices at 1 and 3 weeks in vitro and immunolabeled for synaptophysin (white) to label presynaptic terminals. At both time points, the majority of CA1 pyramidal cell dendritic spine heads (red) are innervated by presynaptic terminals (arrowheads), whereas only a small proportion are not (arrows). Spines that show association of synaptophysin punctae on the neck are not labeled. Shown are images of the synaptophysin labeling before and after performing a three-dimensional "masking" procedure to preserve only the synaptophysin punctae that are associated with the dendrite (see Materials and Methods). Scale bars, 1 µm.
Astrocytes display a wide range of dynamic motility
Most reports have described the structural properties of glial cells in dissociated cultures in which astrocytes typically exhibit a simplified two-dimensional cellular morphology. Thus, dissociated astrocytes do not fully mimic the features of astrocytes in vivo. This is in contrast to astrocytes in hippocampal slice cultures, in which the cells show complex three-dimensional morphology (Benediktsson et al., 2005
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Figure 5. Astrocytes undergo rapid structural modifications. a, An example showing astrocytic process retraction and extension over a 10 min imaging period (confocal maximum projections of the first 4 time points are shown). b, Three-dimensional reconstructions of the area outlined in a over the 10 min period. c, Volume measurements of retracting (red circles) and extending (blue squares) processes plotted over time. Scale bars: a, 10 µm; b, 4 µm.
Cooperative astrocyte–dendritic spine motility
We next were interested in determining the dynamic relationship between astrocytes and dendritic spines. We focused our attention on postsynaptic spines because they have been shown to have a wide range of motile behaviors (Dailey and Smith, 1996
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Figure 6. Astrocyte–spine interactions show dynamic structural interplay. a, Example of an astrocytic process (green) extending toward a dendritic spine (red). b, Example of an interaction that is lost between a dendritic spine (red) and a retracting astrocytic process (green). Insets show 90° (a) or top-down (b) views of the astrocyte–spine interactions. Scale bars, 1 µm.
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Figure 7. Properties of astrocyte–spine interactions. a, Astrocytic processes have significantly higher motility indices (MI) than spines (n = 71 spine–astrocyte pairs from 7 experiments; p < 0.007, paired Student's t test; error bars represent SEM). b, Plot of astrocyte versus spine motility reveals three populations of interactions: astrocytes with similar (51%, astrocyte MI/spine MI is >0.5 but <1.5; circles, line represents best fit), greater (32%, astrocyte MI/spine MI is >1.5; squares), or less (17%, astrocyte MI/spine MI is <0.5; triangles) motility than dendritic spines. c, Approximately 50% of astrocytic process–spine pairs show coordinated changes in size over time, 27% are not coordinated, and 23% show opposite changes (10% cutoff for increases or decreases in size; see Materials and Methods; error bars represent SEM). d, Plot of spine motility index versus average spine area. Spines with greater area show less motility. Curve represents a power trend. e, Cytochalasin-D treatment (5 µM) reduces both spine and astrocyte motility. Motility indexes calculated before (circles) and after (squares) the start of cytochalasin-D (Cyto-D) treatment for individual spines and astrocytic processes (spines, p < 0.003, paired Student's t test, n = 20 spines; astrocytic processes, p < 0.006, paired Student's t test, n = 25 astrocytic processes). f, Perfusion of bicuculline (20 µM) significantly reduces the motility of dendritic spines but not astrocytic processes. Motility indexes calculated before (circles) and after (squares) the start of bicuculline application for spines and astrocytic process (spines, p = 0.002, paired Student's t test, n = 31 spines; astrocytic processes, p > 0.05, paired Student's t test, n = 49 astrocytic processes).
In most cases, the relative trajectories of spine and astrocyte movements were not associated. However, astrocytic processes rapidly reconfigured their location around spine heads (Fig. 6) (supplemental movies 2, 3, available at www.jneurosci.org as supplemental material). Despite the lack of coordinated directional movement, 50% of spines showed cooperative changes in size (in terms of growth, retraction, or stability) with astrocytic processes, whereas 27% of spines did not show cooperative changes, and 23% spines showed opposite changes in size relative to astrocytic processes. Thus, astrocytic processes mainly show cooperative growth processes with spines, indicating a positive relationship between astrocyte and spine growth/retraction.Dendritic spines are known to use actin-based cytoskeletal rearrangements for their motility (Fischer et al., 1998
To test whether general modifications to neural activity affect both spine and astrocytic motility, we calculated motility indices before and after application of the GABAA receptor antagonist bicuculline. We used bicuculline to globally increase neural activity in slices because a previous study has shown that it can stabilize rapid changes in dendritic spine shape (Korkotian and Segal, 2001
Continuous remodeling of astrocytic association with dendritic spines
An important function of astrocytes is to regulate the synaptic microenvironment by removing neurotransmitter from the extracellular space and releasing neuroactive substances (i.e., glutamate, ATP, and D-serine). This function is likely influenced by the location of fine astrocytic extensions near the synapse. We were interested in determining the degree to which astrocyte proximity could be reorganized around spines over time. We infected slices with viruses after 3 weeks in culture and subjected them to time-lapse confocal imaging. Sites of interaction between spines and astrocytic processes were reconstructed in three dimensions, and their relationship was examined (Fig. 8a). To reduce the possibility that spines were being contacted by multiple astrocytes, we chose spines that were localized within a single astrocyte domain. We observed that larger spines were more stable, showing lower spontaneous volume changes over time (Fig. 8b). This is consistent with our motility index analysis in which spine motility decreased with increased spine area and with in vivo data showing that larger spines are, in general, more stable (Grutzendler et al., 2002
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Figure 8. Stability of astrocyte–spine interactions. a, Example of an interaction between a stable spine and its associated astrocytic process during a 15 min imaging period. b, Plot of percentage spine volume change versus average spine volume showing that larger spines have smaller changes in volume over time and more stable contacts with astrocytic processes (n = 32 pairs from 3 experiments). Curves represent power trends. Scale bar, 0.5 µm.
Discussion
Structural plasticity of the CNS is widely believed to be important for brain function (Segal, 2005Spine movements likely change the association of synapses with components in the surrounding extracellular space, including glial cell processes (Dunaevsky et al., 2001
The proximity of astrocytes to dendritic spines in the hippocampus is known to be different from neuron–glial interactions in other systems, such as the cerebellum in which Bergmann glial extensions can fully encapsulate parallel fiber/Purkinje neuron synapses (Grosche et al., 2002
What is the physiological importance of dynamic neuron–glial interactions in the brain? Astrocyte motility may regulate the positioning of key molecules (i.e., glutamate transporters) that actively control the properties of the synaptic microenvironment (Huang and Bergles, 2004
Simultaneous modifications of neuronal and glial cell morphology are known to take place in the brain and have been linked to behavior. For instance, naturally occurring changes in dendrites and astrocytes occur during the estrus cycle. Dendritic spine density is increased on pyramidal cells (Woolley et al., 1990
Our results demonstrate that morphological changes in astrocytes can be rapid, occurring within minutes in hippocampal slice culture. This may be important for physiological changes that are induced over short time periods such as LTP. However, it should be mentioned that organotypic slice cultures cannot not fully mimic the properties of the intact brain. Although neuronal remodeling is remarkably similar in organotypic cultures and in vivo (Dunaevsky et al., 1999
Interestingly, accumulating evidence indicates that glutamate controls the structural features of both neurons and glial cells. For example, glutamate stabilizes spines when spontaneously released from presynaptic terminals (McKinney et al., 1999
Perhaps the level of synaptic activity determines the extent of astrocytic association with the synapse. Recent data indicate that increases and decreases in synaptic efficacy accompany spine enlargement and retraction, respectively. This correlates with our data suggesting that spine and astrocytic growth and retraction are coordinated in
Footnotes
Received March 27, 2006; revised June 21, 2006; accepted July 24, 2006.This work was supported by the Canadian Institutes of Health Research, Canada Research Chairs Program, Canadian Foundation for Innovation, and the EJLB Foundation (K.K.M.). M.H. was supported by a studentship from the Research Institute of the McGill University Health Centre and the McGill Department of Medicine. We are grateful to R. Dunn, Q. Deng, K. Lundstrom, and R. Bremner for providing SFV vectors and help with generating SFV particles. We thank R. Tsien (Howard Hughes Medical Institute) for providing monomeric red fluorescent protein DNA and S. Carbonetto and D. van Meyel for valuable comments regarding this manuscript.
Correspondence should be addressed to Dr. Keith K. Murai, Centre for Research in Neuroscience, Montreal General Hospital, 1650 Cedar Avenue, L7-212, Montreal, Quebec, H3G 1A4, Canada. Email: keith.murai{at}mcgill.ca
Copyright © 2006 Society for Neuroscience 0270-6474/06/268881-11$15.00/0
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