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Previous Article | Next Article
The Journal of Neuroscience, December 1, 2001, 21(23):9325-9333
Modular Transport of Postsynaptic Density-95 Clusters and Association with Stable Spine Precursors during Early Development of Cortical Neurons
Oliver Prange1 and Timothy H. Murphy1, 2 Kinsmen Laboratory, Departments of 1 Psychiatry and 2 Physiology, University of British Columbia, Vancouver, British Columbia, Canada V6T 1Z3
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
The properties of filopodia and spines and their association with the postsynaptic density (PSD) protein PSD-95 were studied during early development of cultured cortical neurons using time-lapse confocal microscopy. Neurons were transfected with recombinant PSD-95 constructs fused to green fluorescent protein (GFP) for, on average, either 8 d in vitro (DIV) or 14 DIV. We find that, during 1 hr of imaging, filopodia and spines bearing PSD-95/GFP clusters are significantly more stable (i.e., do not turnover) than those lacking clusters. When present within a spine precursor, a PSD-95/GFP cluster appeared to nucleate a relatively stable structure around which filopodium-spine membranes can move. Although processes bearing clusters were generally stable, in 8 DIV neurons, we observed that a subset (~10%) of PSD-95/GFP clusters underwent rapid modular translocation between filopodia-spines and dendritic shafts. We conclude that, during early synaptic maturation, prefabricated PSD-95 clusters are trafficked in a developmentally regulated process that is associated with filopodial stabilization and synapse formation.
Key words: development; dendritic spine; filopodium; glutamate receptor; NMDA receptor; PSD-95
INTRODUCTION
The postsynaptic density (PSD) protein PSD-95 is a founding member of the growing superfamily of PDZ (PSD-95-Disks large-zona occludens1/2) domain-containing proteins (Craven and Bredt, 1998
; Fanning and Anderson, 1999
PSD-95 is an integral protein of the postsynaptic density at excitatory synapses. Binding partners of PSD-95 include the NMDA (via PDZ1 and PDZ2) and kainate (via SH3) receptors and the cell adhesion molecule neuroligin (via PDZ3). Furthermore, binding to the proteins CRIPT [(cysteine-rich interactor of PDZ three) via PDZ3] and GKAP [(guanylate kinase domain-associated protein) via GK] can tether PSD-95 and its binding partners to the intracellular tubulin and actin lattice, respectively (Scannevin and Huganir, 2000
Previous evidence for a role of filopodia in synaptic contact formation (Ziv and Smith, 1996
Here we use simultaneous time-lapse imaging of green fluorescent protein (GFP)-labeled PSD-95 and of filopodial motility to examine the disposition of PSD-95 clusters in dynamic filopodia. We report that PSD-95 clusters are transported as modular units and become associated with stable filopodia.
MATERIALS AND METHODS
Cell culture and particle-mediated gene transfer. Embryonic cortical neurons and glia were dissociated from 18-d-old Wistar rat fetuses and cultured on poly-D-lysine-coated 12 mm glass coverslips at a density of ~1.5 million cells per milliliter (Mackenzie et al., 1996
Imaging and electrophysiology. Coverslips were placed into a customized perfusion chamber (~500 µl vol) and fixed by platinum weights to prevent movement. The cultures were continuously perfused (~1.5 ml/min) with an HBSS containing (in mM): 137 NaCl, 2.5 CaCl2, 1.0 MgSO4, 5.0 KCl, 0.34 Na2HPO4(7H2O), 10.0 Na+-HEPES, 1.0 NaHCO3, and 22.0 glucose at pH 7.4 (~305 mOsm). The solution was heated to 32°C using a flow-through heater (Warner Instruments, Hamden, CT). Whole-cell patch clamp on GFP fluorescence-positive cells was conducted using an Axon Instruments (Foster City, CA) Axopatch 200B amplifier and 7-10 M
electrodes pulled from 1.5 mm glass capillaries. The patch pipette solution contained 122 mM K+-gluconate, 20 mM NaCl, 5 mM Mg2+-ATP, 0.3 mM GTP, 10 mM HEPES, 100 µM EGTA, and 500 µM sulforhodamine 101 (Molecular Probes, Eugene, OR), pH 7.2. The solution was allowed to perfuse into cells during whole-cell recording for 3-5 min, during which spontaneous postsynaptic currents were recorded. After that period, the electrode was carefully removed from the cell soma, allowing the membrane to reseal. The dye was allowed to equilibrate in the cell for at least 10 min before imaging experiments were performed.
Confocal time-lapse microscopy was performed on a Bio-Rad MRC 600 system attached to a Olympus Optical (Tokyo, Japan) BX50WI upright microscope using an Olympus Optical 0.9 numerical aperture 60× water immersion objective. The confocal pinhole was set to 3-4 (Bio-Rad units), and two-channel imaging was performed in slow scan mode (without averaging). For data acquisition, every 5-9 min (average, 7 ± 2 min), a (vertical) Z-series was taken over an area of 96 × 128 µm (384 × 512 pixels) containing the full extent of the dendrite of interest. The spacing of successive Z-images was 1 µm and provided sufficient overlap between sections as the Z-resolution of the imaging system at the settings used was 2.5 µm (measured as the width of the point spread function at half-maximum fluorescence intensity). The number of Z-images acquired ranged from three to seven but was always constant within an experiment. To correct for potential vertical movement of the specimen between time points, all Z-series in one experiment were started from a marker point chosen within the first optical plane.
Immunohistochemistry. For quantifying colocalization of PSD-95 clusters with presynaptic markers, cell cultures expressing WT PSD-95/GFP were fixed in paraformaldehyde at either 8 or 14 DIV. Cell cultures were immunolabeled using a mouse (IgG) monoclonal antibody (Ab) against synaptophysin (Boehringer Mannheim, Mannheim, Germany) at 28 µg/ml (1:50) and an IgG polyclonal donkey-derived Texas Red-conjugated secondary Ab (Jackson ImmunoResearch, West Grove, PA) at 200 ng/ml (1:50). Coverslips with immunostained cells were embedded in anti-fade (Molecular Probes) agent, and confocal dual-channel imaging was performed using a 100× Zeiss (Oberkochen, Germany) Fluar oil-immersion lens.
Analysis. For analysis of PSD-95 localization and filopodial stability, only cells were used that did not show any morphological signs of cellular degeneration or impending death (i.e., cell swelling and/or collective loss of filopodia) before, during, or after imaging. For each time point, fluorescence data collected in a Z-series was projected into one layer using the maximum intensity method. Two-channel confocal images were separated off-line into their respective channels (sulforhodamine and GFP signal) and coded. This procedure allowed analysis of filopodial-spine stability to be performed on the sulforhodamine signal (red channel) without knowledge of which construct (WT PSD-95 or MUT PSD-95) the cells were transfected with. To be included for analysis, a filopodium-spine had to fulfill the following criteria: (1) being >1 and <10 µm in length, (2) not contacting another process, (3) not being extensively branched (<3 branches), and (4) being sufficiently filled with dye so that it is clearly visible throughout the entire period of imaging (~1 hr). Processes that fit these criteria were not further subcategorized into either filopodia or spines, because unambiguous distinction by solely morphological criteria cannot be always made. The stability of each filopodium was judged by evaluating its status over 1 hr of imaging. A filopodium-spine was defined as stable if it was present (visible) during the whole course of image acquisition. An unstable filopodium-spine either appeared new and/or disappeared during the time course of imaging. After this analysis, for each cell, the Z-projection of the corresponding GFP signal (green channel) was superimposed on the sulforhodamine (red channel) signal.
For WT PSD-95/GFP-expressing cells, PSD-95 clustering was based on the data collected on the green channel. In spines and dendritic shafts, the characteristics of each cluster were assessed throughout the period of imaging. In cases in which clustering could not be unambiguously attributed to a specific accumulation of PSD-95/GFP rather than a volumetric effect of the dendritic process, the fluorescence intensity of a potential PSD-95/GFP cluster was divided by the fluorescence signal of an area adjacent to the cluster. This ratio was then compared with the fluorescence ratio between the same areas (obtained using the same coordinates) on the sulforhodamine (red) channel, which represents a volumetric marker. If the ratio obtained on the green channel was more than two times the ratio on the red channel, then the PSD/95-GFP clustering was concluded to be specific.
For analysis of colocalization between the Texas Red-conjugated Ab-labeled presynaptic marker synaptophysin (red channel) and PSD-95/GFP clusters (green channel), Z-series from both channels were superimposed. Synaptophysin and PSD-95/GFP clusters were considered colocalized and indicative of a putative synapse if they were present within the same focal plane and were overlapping by at least 0.25 µm (1 pixel row).
For statistical analysis, the nonparametric two-tailed Mann-Whitney and Kruskal-Wallis ANOVA tests were used, unless otherwise noted. Data are expressed as the mean ± SEM.
RESULTS
We used transfection of GFP-tagged PSD-95 constructs to examine the dynamics of filopodia and spines during development of primary cortical neurons. Biolistic particle-mediated transfer of DNA constructs was performed at 3-6 (average, 3.5 ± 0.2; n = 41 cells) d after plating cell cultures. At this time, the total amount of endogenous PSD-95 and the degree of synaptic PSD-95 clustering is low (Rao et al., 1998
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Figure 1. Two-channel confocal imaging to independently analyze PSD-95/GFP distribution and dendritic morphology. Cultured cortical neurons were transfected with GFP-tagged WT (top row) or cys3,5ser MUT (bottom row) forms of PSD-95. Before imaging, cells were colabeled with sulforhodamine. Dual-channel confocal imaging was performed, allowing the separation of the GFP (left panels) and sulforhodamine (right panels) signal. The middle panels show pseudocolored composite images of the left and right panels in their respective row; areas of GFP (green) and sulforhodamine (red) colocalization appear yellow. Localization of PSD-95/GFP in dendritic shafts and spines is clustered in cells expressing WT PSD-95/GFP (top row) and dispersed in cells expressing the MUT PSD-95/GFP form (bottom row). Cells were cultured for 13 d (top row) and 8 d (bottom row). Scale bar, 5 µm.
To assess the potential role of PSD-95 clustering in synapse development, maturation, and motility, we also transfected a mutant (palmitoylation deficient) nonclustering form of PSD-95 into sister cultures of cortical neurons. As shown previously (Craven et al., 1999
To simultaneously assess the localization of PSD-95 and the stability of filopodial processes, we used patch-clamp techniques to inject a second fluorescent marker (sulforhodamine) with different spectral properties into neurons expressing PSD-95/GFP. This allowed us to reliably resolve filopodia and spines, including ones that do not express the PSD-95/GFP protein (Fig. 1, top row). At this early developmental stage, it was often not possible to further subcategorize processes into either filopodia or spines based solely on morphological features. Hence, we used the term filopodia-spines to describe all dendritic protrusions of length >1 and <10 µm (see also Materials and Methods). Using two-channel confocal microscopy, double-labeled cells were imaged on average every 7 min over a time period of 60-65 min (Fig. 2). Filopodia-spines with PSD-95/GFP clusters were stable (did not appear or retract) over the entire period of imaging. Time-lapse imaging indicated that, although the PSD-95/GFP clusters themselves were stable, the unlabeled membranes around the cluster were in constant motion (Fig. 2). Furthermore, nearby unlabeled (by PSD-95/GFP) processes were found to transiently extend and retract (Fig. 2) (see animation for Fig. 2 at www.interchg.ubc.ca/neurosci/faculty/murphy.html#j_ns2).
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Figure 2. Confocal time-lapse analysis of filopodia-spine stability and PSD-95 clustering. Time-lapse series of a neuron (10 d in vitro) that expressed WT PSD-95/GFP (green) and was filled with sulforhodamine (red). Spots of PSD-95/GFP clustering appear yellow. The bottom panel shows an overview of the dendrite. Scale bar, 5 µm. Three areas are magnified (see dashed outlines labeled a-c). Time series in the top rows advances in columns from left to right for the three areas of interest; the second row shows time stamps in minutes. For simplicity, not every time point is shown. Newly forming (white arrowheads) and disappearing (black arrowheads) filopodia-spines are marked. Note that PSD-95/GFP-containing structures are stable over time (i.e., they do not turnover) but can exhibit structural changes. Scale bars: magnified areas, 1 µm; bottom panel overview, 5 µm.
To remove potential experimenter bias, two-color (PSD-95/GFP and sulforhodamine) fluorescence images were separated into their respective channels and coded. Analysis of filopodia-spine turnover was performed using only the sulforhodamine (red) channel. This procedure ensured that analysis of filopodia-spine movement was done without previous knowledge of PSD-95 disposition for particular spines or the type of construct transfected. To examine the dynamics of PSD-95 clustering and its potential role during early synaptic development, we compared PSD-95 translocation and filopodium
spine motility at two different in vitro ages. Cells from the first group (labeled 8 DIV) were studied at an average age of 7.9 ± 0.3 DIV (range, 6-10 DIV; n = 26 cells), a period that is expected to correspond to the early onset phase of synaptogenesis (Lee and Sheng, 2000
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Figure 3. Quantitation of filopodia-spine development and the association with PSD-95/GFP clusters. A, Increase in number and stability of filopodia-spines during early neuronal development. Cells were cultured for, on average, either 8 or 14 d, and filopodia-spine dynamics were imaged using confocal time-lapse microscopy over 1 hr. The total number of filopodia-spines increases (by 37%; *p < 0.05) between the two age groups. A disproportionately large increase in the number of stable filopodia-spines (by 135%; ***p < 0.001) was observed. A concomitant decrease (by 65%; **p < 0.01) in the number of unstable filopodia-spines was observed. All numbers are normalized to dendritic length. B, Increase in the number of filopodia-spines with PSD-95 clusters but not of PSD-95 shaft clusters during early neuronal development. Comparison of cells in the younger (n = 13 cells) with the older (n = 10 cells) age group indicated a significant increase in the density of filopodia-spines with PSD-95/GFP clusters (by 350%; ***p < 0.001). No significant (ns) change in the number of PSD-95 shaft clusters (21% decrease; p > 0.4). C, Filopodia-spines with PSD-95/GFP clusters are more stable than filopodia-spines without clusters. The stability of filopodia-spines was compared between filopodia-spines with PSD-95/GFP clusters and filopodia-spines devoid of clusters. Filopodia-spines without PSD-95/GFP clusters are significantly more unstable at 8 DIV (***p < 0.001) and 14 DIV (**p < 0.005) compared with filopodia-spines with PSD-95/GFP clusters (8 DIV: n = 13 neurons, 303 filopodia-spines; 14 DIV: n = 10 neurons, 440 filopodia-spines).
To reduce potential bias associated with the selection of particular segments of dendrite for imaging, we normalized the number of stable and unstable filopodia-spines to the total number of filopodia-spines per cell. Using this procedure, we find no difference in the proportions of stable and unstable filopodia-spines between MUT and WT PSD-95/GFP-expressing cells in either age group (8 DIV, p > 0.2; 14 DIV, p > 0.5). Additionally, there was no difference in the proportion of stable and unstable filopodia-spines between PSD-95/GFP-expressing cells and control cells (n = 9) expressing only GFP in either age group (8 DIV, p > 0.5; 14 DIV, p > 0.7; Kruskall-Wallis test).
To evaluate the relationship between PSD-95 clustering and filopodia-spine dynamics in neurons overexpressing the WT PSD-95/GFP construct, we separately analyzed data from the PSD-95/GFP (green) channel. First, we found a significant increase in the overall density of PSD-95 clusters in dendrites (from 86 ± 9 to 117 ± 19 per millimeter of dendrite; p < 0.05) when comparing between stages of earlier (8 DIV) and later (14 DIV) in vitro development. This difference was primarily attributable to a significant increase of filopodia-spines possessing PSD-95/GFP clusters (from 17 ± 4 to 60 ± 12 per millimeter of dendrite; p < 0.001) (Fig. 3B). However, the density of PSD-95/GFP clusters in dendritic shafts did not change significantly over the same period (from 69 ± 8 to 57 ± 9 per millimeter of dendrite; p > 0.4) (Fig. 3B). To determine whether the increasing number of PSD-95/GFP clusters was attributable to an increase in the cluster fluorescence intensity (and therefore in the likelihood of detection), we compared the PSD-95/GFP fluorescence signal between 8 DIV (n = 6 cells) and 14 DIV (n = 6 cells) using identical imaging settings. Our results indicate that this was not the case because we find that the intensity of PSD-95/GFP clusters actually decreases (by 52%; p < 0.001) between 8 and 14 DIV, confirming reports of declining levels of recombinant protein expression over this time (Craven et al., 1999
In young neurons, only a subset of filopodia-spines (14%) contain PSD-95/GFP clusters (Fig. 3), providing a scenario to test the relationship between the presence of clusters and stability. Accordingly, we analyzed the stability of filopodia-spines with PSD-95/GFP clusters in WT PSD-95/GFP-expressing cells (n = 23). We find that, of 190 filopodia-spines that possessed PSD-95/GFP clusters, only 3 (1.6%) were unstable during the ~1 hr period of imaging (Fig. 3C). This high level of stability differed significantly from that of filopodia-spines without PSD-95/GFP clusters in both age groups. At 8 DIV, 54 ± 6% of all filopodia-spines without PSD-95/GFP clusters were unstable, whereas only 9 ± 8% with PSD-95/GFP clusters were (p < 0.001) (Fig. 3C). At 14 DIV, only 1 ± 1% of all filopodia-spines with PSD-95/GFP were unstable versus 20 ± 6% without PSD-95/GFP clusters (p < 0.005) (Fig. 3C).
By restricting our acquisition of data to a 1 hr period, we minimized potential damage attributable to phototoxicity. However, it is possible that by selecting a single arbitrary time point we may have underestimated the number of unstable spines. To further examine the relative stability (i.e., turnover time) of filopodia-spines, additional experiments (n = 3) were performed in which the total imaging time was increased to 2.5 hr (sampling intervals extended to 15 min). As expected, we find that, by increasing the imaging time from 1 to 2.5 hr, a significantly higher proportion of filopodia-spines become unstable (83 ± 4 vs 48 ± 6% at 1 hr; p < 0.05; one-tailed Mann-Whitney test). However, we still find that all filopodia-spines (100%) associated with PSD-95/GFP clusters (n = 8; 11% of all filopodia-spines) are stable during the 2.5 hr imaging period. Together, these data suggest that the average half-life time for filopodia-spine structures without PSD-95 clusters approximates 1 hr and that most of these structures will eventually turnover during longer time periods. On the other hand, PSD-95/GFP-associated structures display structural stability over extended time periods.
Because our data indicate that filopodium-spine structures with associated PSD-95 clusters are highly stable, we next determined the stability of the PSD-95 clusters themselves. Of all PSD-95 clusters found in dendritic shafts (n = 317) and in filopodia-spines (n = 190), we did not find a single case demonstrating the breakdown (disappearance) and/or the appearance of the cluster within 1 hr of time-lapse imaging, indicating a slow turnover rate for PSD-95 clusters. However, unidirectional or bidirectional lateral movement of PSD-95 clusters within dendritic shafts and filopodia-spines could be observed (Fig. 4A,B). Of all shaft PSD-95 clusters, 14 ± 4% exhibited lateral movement at 8 DIV over a 1 hr period. This proportion decreased significantly to 2 ± 1% at 14 DIV (p < 0.05). The range of movement of PSD-95 shaft clusters was usually relatively small (1-3 µm) but could in single cases be up to 5 µm within 20 min of imaging. Additionally, small 1-2 µm movements of PSD-95/GFP clusters could be observed in 20 ± 9% (8 DIV) and 17 ± 7% (14 DIV) of all filopodia-spines with PSD-95 clusters. Moreover, in a few occasions (<5% of all clusters), we were able to observe "splitting" of a PSD-95 cluster (Fig. 4A,B) or "merging" of two or more PSD-95 clusters into one. For more information, see on-line animated version of Figure 4 (www.interchg.ubc.ca/neurosci/faculty/murphy.html#j_ns4).
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Figure 4. Dynamic properties of PSD-95 clusters within developing neurons. Partial time-lapse series of dendrites of cells transfected with WT PSD-95/GFP (green) and filled with sulforhodamine (red) to assess structure. Areas of dye colocalization appear yellow. Images in respective columns were taken consecutively, with the exception of the last time point in A-C, which represents the last data point of the series. Time stamps are in minutes; all series start at 0 min. Scale bars, 1 µm. A, A 10 DIV neuron in which a PSD-95 cluster (white arrowhead) moves out of a filopodium-spine. Spine splitting at 27 min into a two-headed structure. B, A 6 DIV neuron in which a shaft cluster splits into two domains (0-5 min; top, black arrowheads). A cluster (bottom) leaves a filopodium-spine (between 11 and 16 min time points; white arrowhead) and transiently splits (22 min; black arrowhead). Filopodium-spine consecutively undergoes rapid outgrowth (22 min) and retraction (58 min). C, An 8 DIV neuron in which filopodium-spine outgrowth (0-9 min; black arrowhead) precedes localization of cluster into its tip (14-19 min; white arrowhead) and additional elongation of the structure with arrested cluster in its tip (26-50 min). D, An 8 DIV neuron in which a small PSD-95/GFP-labeled structure reversibly protrudes from a large shaft cluster (top). Another small filopodium reversible protrudes (bottom) from the dendritic shaft, carrying a PSD-95 cluster from the dendritic shaft with it.
Although PSD-95 clusters in filopodium-spine structures were mostly stable, we did occasionally observe filopodia-spines or small precursors to these structures into which PSD-95/GFP clusters became transiently located (Fig. 4A,B). Interestingly, we found nine cases in which PSD-95 clusters either exited (n = 7) and/or entered a filopodium-spine (n = 2), usually within <20 min (Fig. 4). Seven of these cases were found in neurons within the younger age group (8 DIV), representing 13% of all filopodia-spines with PSD-95 clusters. In the older age group (14 DIV), we observed this phenomenon in only two cases (1%) of filopodia-spines with PSD-95 clusters. Analysis of these images indicated that the PSD-95 clusters moved as modular units. Clusters were observed to move either independently along the length of a filopodium-spine (Fig. 4A,B) or to remain stationary and move as a consequence of a growing or retracting structure (Fig. 4C, D). In all cases in which PSD-95/GFP clusters were translocated, these processes appeared to occur rapidly (within minutes) and involved the coordinated relocation of an intact cluster rather than a gradual accumulation or breakdown of labeled material (see time courses in Fig. 4).
PSD-95/GFP movement within filopodia-spines was usually associated with significant structural changes of the structures (Fig. 4A,B). As illustrated in Figure 4A, retraction of a PSD-95 cluster from the tip of a filopodium-spine to the shaft occurred at a rate of ~4 µm in 30 min and was associated with a bifurcation of the filopodium-spine into a two-headed structure (27 min image). In other cases, we observed that the translocation of PSD-95/GFP clusters was associated with a sudden outgrowth of the structure (Fig. 4B). Alternatively, PSD-95 shaft clusters could be "picked up" by outgrowing filopodia-spines (Fig. 4C) or short-lived proto-filopodial structures (Fig. 4D), and subsequently located into their growing tips (Fig. 4C). These data indicate the existence of two distinct processes: one for preassembling PSD-95 into clusters and one for subsequently localizing PSD-95 complexes into emerging filopodia-spines, which is reversible (see also animated material).
To assess whether the developmental changes in filopodium-spine stability and PSD-95 localization were accompanied by presynaptic changes, we used an immunostaining approach. A primary antibody against the presynaptic marker synaptophysin and a secondary Texas Red-conjugated antibody were used in cultures transfected with WT PSD-95/GFP at 8 and 14 DIV (Fig. 5). Analysis of colocalization between PSD-95/GFP and synaptophysin shows a significant increase (p < 0.0001) between 8 DIV (37 ± 2% of all PSD-95 clusters colocalizing with synaptophysin; n = 9 cells) and 14 DIV (75 ± 5%; n = 9 cells) (Fig. 5). However, even at the younger age (8 DIV) when PSD-95/GFP was present in filopodia-spines (rather than dendrite shafts), colocalization with synaptophysin was significantly higher (71 ± 9%; p < 0.01) than the overall rate (Fig. 5). The same trend was apparent of older cultures (14 DIV) in which colocalization of PSD-95 and synaptophysin increased significantly to 93 ± 2% (p < 0.001) when only clusters in filopodia-spines were considered and shaft clusters were excluded (Fig. 5).
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Figure 5. Developmental increase in the colocalization of PSD-95 and a presynaptic marker. Neurons were transfected with the WT PSD-95/GFP (top panels) construct and were immunostained for the presynaptic marker synaptophysin (SynPh; bottom panels) using a Texas Red-conjugated secondary antibody. The left and right columns depict representative confocal images from dendritic regions immunostained at 8 and 14 DIV, respectively. Middle panels, Composites of the PSD-95 (green) and synaptophysin (red) images. White arrows depict examples of PSD-95 and synaptophysin colocalization; black arrowheads indicate examples of PSD-95 clusters without corresponding synaptophysin clusters. Scale bar, 2 µm. Bar graph, Colocalization of PSD-95 and synaptophysin increases significantly between 8 DIV (37 ± 2% of all PSD-95 clusters are colocalized with synaptophysin; n = 9 cells) and 14 DIV (75 ± 5%; n = 9 cells) (left column). A significantly higher rate of colocalization was observed when PSD-95/GFP clusters were localized in filopodia-spines (compare the left and right columns for the same age group). **p < 0.01; ***p < 0.001
DISCUSSION
Dendritic filopodia are highly motile transient processes that move in an actin-dependent manner (Fischer et al., 1998
Accordingly, we performed time-lapse imaging experiments with GFP-tagged PSD-95 to simultaneously monitor filopodial-spine stability and PSD-95 localization during a time period of in vitro development believed to be critical for synaptogenesis and stabilization of dendritic processes. Although previous time-lapse studies of PSD-95 have been done (Okabe et al., 1999
Consistent with previous data (Ziv and Smith, 1996
The fact that PSD-95/GFP overexpression does not affect spine development in our cultures importantly indicates that we were not perturbing the system and altering the properties or number of filopodia-spines that were studied with time-lapse imaging. It was under these conditions that, within WT PSD-95/GFP-expressing neurons, we observed a profound increase in the stability of filopodia-spines with PSD-95 clusters compared with filopodia-spines that lack PSD-95 clusters at both developmental stages studied. These findings suggest that events associated with the presence of clusters lead to the development of stable filopodia-spines, which, over longer time periods, may transform into functional postsynaptic spines with their typical morphological features (Lee and Sheng, 2000
Consistent with the relative stability of the PSD (Allison et al., 1998
In a few examples, filopodia-spines exhibited significant structural changes after a PSD-95 cluster retracted, as if the cluster was part of a structural element that needed to be removed before the filopodium-spine could undergo this change (Fig. 4). In other cases, PSD-95 clusters were within a filopodium-spine in which the process would grow or morph around the cluster. That is, the cluster appeared to remain stable despite the surrounding process changing in shape (Fig. 2). This provides additional functional evidence that the PSD-95 cluster is a rather stable structural element.
By performing synaptophysin immunocytochemistry in combination with localization of PSD-95/GFP, we observed that, in young cultures (that have more dynamic dendritic processes), many of the clusters (>60%) were not associated with presynaptic terminals. Perhaps these nonsynaptic clusters are reserve materials for building new synapses from prefabricated structural elements. Consistent with this idea, we found a robust increase (by approximately two times) of PSD-95/synaptophysin colocalization when analysis was restricted to PSD-95 clusters that were located in filopodia-spines. Clearly, a better understanding of the molecular events associated with the formation and maintenance of PSD-95 cluster and its role in will be crucial to understanding its role in stabilizing dendritic filopodia and spines.
FOOTNOTES Received Aug. 8, 2001; revised Aug. 8, 2001; accepted Sept. 11, 2001.
T.H.M. is supported by an operating grant from the Canadian Institutes for Health Research (CIHR) and is a CIHR Scientist. O.P. is supported by a University Graduate Fellowship. We thank A. E. El-Husseini and D. S. Bredt for providing GFP-tagged PSD-95 constructs and antibodies.
Correspondence should be addressed to Dr. Tim Murphy, Kinsmen Laboratory, Department of Psychiatry, University of British Columbia, 2255 Wesbrook Mall, Detwiller Pavilion Room 4N1, Vancouver, British Columbia V6T 1Z3, Canada. E-mail: thmurphy{at}interchange.ubc.ca.
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