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The Journal of Neuroscience, July 2, 2003, 23(13):5407-5415
Previous Article | Next Article
The Amyloid Precursor Protein and Its Regulatory Protein, FE65, in Growth Cones and Synapses In Vitro and In Vivo
Shasta L. Sabo,1 Annat F. Ikin,1,2 Joseph D. Buxbaum,2 andPaul Greengard1 1Laboratory of Molecular and Cellular Neuroscience and the Zachary and Elizabeth M. Fisher Center, The Rockefeller University, New York, New York 10021, and 2Laboratory of Molecular Neuropsychiatry, Departments of Psychiatry and Neurobiology, Mount Sinai School of Medicine, New York, New York 10029
Abstract
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Abstract
Introduction
Although the Alzheimer amyloid protein precursor (APP) has been studied intensely for more than a decade, its function in neurons is unresolved. Much less is known about its binding partner FE65. We have shown recently that APP and FE65 synergistically regulate the movement of transfected cells. It remained to be shown whether endogenous APP and FE65 could play a similar role in vivo. Here, we show that FE65, like APP, is expressed at high levels in neurons. Using a combination of immunofluorescence, live imaging, and subcellular fractionation, we find that FE65 and APP localize in vitro and in vivo to the most motile regions of neurons, the growth cones. Within growth cones, APP and FE65 concentrate in actin-rich lamellipodia. Finally, APP and FE65 interact in nerve terminals, where they associate with Rab5-containing synaptic organelles but not with synaptic vesicles. Our data are consistent with a role for the APP/FE65 complex in regulation of actin-based membrane motility in neurons, which could be important for highly dynamic processes such as neurite growth and synapse modification.
Key words: APP; FE65; Mena; growth cone; synapse; Alzheimer's disease
Introduction
Although the function of the Alzheimer amyloid protein precursor (APP) in neurons remains unclear, genetic manipulations of APP expression have suggested that APP has roles in synaptogenesis and synaptic plasticity. For example, overexpression of APP in Drosophila results in altered synaptic structure (Torroja et al., 1999). In addition, deletion of the APP gene from mice leads to deficits in learning and memory, impaired long-term potentiation (LTP), and decreased expression of synaptic markers (Dawson et al., 1999
We have shown recently that APP, in a complex with FE65, can regulate cell motility in transfected cells (Sabo et al., 2001
If APP regulates growth cone motility and synaptic plasticity through its interaction with FE65, then it should interact with FE65 in growth cones and synapses. We show here that APP and FE65 colocalize in growth cones both in vitro and in vivo. We show further that APP and FE65 are found in actin-rich mobile structures within the growth cone, where they are poised to interact with the cytoskeleton indirectly through Mena. Finally, we provide evidence for an important interaction between APP and FE65 in synapses in vitro and in vivo as well. Our data are consistent with the hypothesis that APP and FE65 regulate membrane dynamics in growth cones and nerve terminals much as they do in lamellipodia of migrating cells.
Materials and Methods
Neuronal cell culture and transfection. Primary neuronal cultures were prepared from cortices of embryonic day (E) 17 or postnatal day (P) 1 rats. E17 brains were dissociated by trypsinization and trituration in DMEM with 10% fetal bovine serum. Dissociated neurons were cultured on poly-lysine or poly-lysine and laminin (Biocoat, Bedford MA) and maintained in neurobasal medium, B27 supplement (Invitrogen, Carlsbad CA), and antibiotics (Invitrogen). P1 brains were dissociated with papain and plated directly on glia in MEM, 10 mM HEPES, N2 supplement, glucose, and 10% horse serum.Neurons were transfected 3 or 6 d after plating using Lipofectamine 2000 (Invitrogen) essentially according to the manufacturer's instructions. FE65–enhanced green fluorescent protein (EGFP) cDNA was made by subcloning FE65 into pEGFP-C1 (Clontech, Palo Alto CA). Synaptobrevin–dsRed was generated by subcloning synaptobrevin into pdsRed-N1 (Clontech). The localization of synaptobrevin–dsRed was identical to that of synaptobrevin–EGFP, which is correctly targeted to synaptic vesicles (Miesenbock et al., 1998
Axons and dendrites were distinguished on the basis of accepted morphological criteria (Banker and Goslin, 1998
Antibodies. FE65 and APP (369) polyclonal antibodies were affinity purified as described (Sabo et al., 1999
Immunoblotting. Nitrocellulose membranes were blocked with Tris-buffered saline containing 5% (w/v) nonfat dry milk and 0.05% Tween 20 (TBS-T) and then probed with primary antibodies and HRP-conjugated secondary antibody (Calbiochem, La Jolla CA) in TBS-T. Immunoreactivity was visualized by ECL (DuPont NEN, Boston, MA) and exposure to x-ray film (DuPont NEN).
Immunofluorescence. Cells were fixed in 4% paraformaldehyde in PBS with 0.12 M sucrose, permeabilized with 0.1% Triton X-100 in PBS, blocked with 10% normal goat serum (NGS) in PBS, and then immunolabeled in 5% NGS in PBS. Coverslips were mounted with 1,4-diazbicyclo (2.2.2) octane in Tris-buffered polyvinyl alcohol and glycerol. Secondary antibodies were goat anti-mouse Oregon Green, goat anti-rabbit Texas Red (Molecular Probes, Eugene OR), goat anti-mouse Cy5, and goat anti-rabbit Rhodamine red X (Jackson ImmunoResearch, West Grove PA). Actin was detected with Oregon Green phalloidin (Molecular Probes). All immunofluorescence was eliminated by omission of primary antibody. In multiple label experiments, labeling patterns were identical to those seen with single labeling, and channels were imaged sequentially to avoid bleed-through. Immunofluorescence was examined by confocal laser scanning microscopy (Zeiss LSM510 or Leica TCS-SP) using 63x and 40x lenses, Ar488, KrNe543, and KrNe633 nm lasers, and BP560–615, BP505–550, and LP650 filters. For colocalization, optical sections were no thicker than 1.5 µm.
Live imaging. Neurons were transferred to imaging solution containing (in mM): 120 NaCl, 3 KCl, 2 CaCl2, 2 MgCl2, 30 dextrose, 20 HEPES, pH 7.3 (McAllister and Stevens, 2000
Image quantification. The mean pixel intensity for each image was determined in Photoshop 5.0. Each image was thresholded at the mean intensity plus 2 SDs above the mean. The thresholded images were then multiplied. At any pixel where intensity = 0 (i.e., no fluorescence) for either image, the product = 0; therefore, non-zero pixel intensities correspond to colocalization.
Growth cone fractionation. Growth cone particles (GCPs) were prepared as described previously (Pfenninger et al., 1983
Synaptosome fractionation. Synaptosomes and synaptic vesicles were prepared by standard methods (Huttner et al., 1983
Coprecipitation. Crude synaptosomes were suspended in 1% Triton X-100, 50 mM NaPO4, 5 mM EDTA, protease inhibitors, and 20 mM HEPES, pH 7.4. After centrifugation at 40,000 x g, the supernatant was incubated with glutathione–Sepharose beads saturated with glutathione S-transferase (GST)–fusion protein. After extensive washing, bound proteins were analyzed by SDS-PAGE and immunoblotting.
Immunoisolation. Immunoisolation was performed as described (Ikin et al., 1996
Results
FE65 is enriched in human and rat brains
It was important to establish first whether FE65 is expressed in neurons in vivo. Immunoblotting with FE65 antibodies showed that expression of FE65 (100 kDa) was highest in the brains of rats and humans (Fig. 1a,b). Low levels of expression in some peripheral tissues might be caused by innervation. Expression was high throughout the brain and particularly high in cortex, hippocampus, and cerebellum (Fig. 1a). APP is also expressed in all brain areas, with cortex, hippocampus, and cerebellum among the areas expressing especially high levels of APP (Shivers et al., 1988
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Figure 1. FE65 is highly enriched in brain. a, Tissues from adult rat were immunoblotted with FE65 antibody. Preincubation of FE65 antibody with excess antigen (+excess antigen) eliminated the FE65-immunoreactive bands. b, Immunoblotting of human tissues for FE65. c, Immunoblotting of expressed FE65 in neural (SKN-SH-SY5Y, H4) and non-neural cell lines with (CHO+FE65) and without (CHO) FE65 transfection.
FE65 antibodies also recognized a second band in brain, at
FE65 and APP colocalize in neuronal growth cones in vitro and in vivo
When primary neuronal cultures were examined by immunofluorescence, FE65 and APP colocalized in growth cones (Fig. 2a–d). Both proteins were found in growth cones with various morphologies and at the tips of both long and short neurites. In addition, labeling of neurons grown on laminin was indistinguishable from that of neurons grown on poly-lysine (data not shown). These results agree with reports citing the presence of APP in growth cones (Ferreira et al., 1993
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Figure 2. FE65 and APP localize to growth cones in vitro and in vivo. a–c, Confocal images of several embryonic neuronal growth cones double-labeled with APP (a) and FE65 (b) antibodies. Yellow in the overlay (c) represents colocalization of APP and FE65. Blue arrows point to the intense labeling of three growth cones by APP and FE65 antibodies. a'–c', Thresholded versions of the images in a–c illustrate that the most intense labeling for both APP and FE65 (represented by white in the images) is found within growth cones (indicated by blue arrows). d, Line intensity profile of the intensity of APP (green) and FE65 (red) labeling in the growth cone and axon indicated by the blue star in a–c. The line was drawn through the center of the growth cone and down the axon, parallel to the axonal axis. The region that corresponds to the growth cone is indicated by a gray box in the intensity profile. Although intensity values reached saturation within the growth cone, intensity values were lower and highly variable within the axon. The close covariance of the red and green signals illustrates the high degree of colocalization of APP and FE65. The two sharp peaks at the beginning of the profile correspond to puncta of APP and FE65 within the growth cone filopodia. e, Growth cone of a neuron transfected with FE65–EGFP. The fluorescence image is showed as an overlay on the DIC image. A blue arrow indicates the position of the growth cone on the labeled axon. Notice the labeled filopodium on the bottom, right (shown with a yellow arrow). f, Immunoblotting of purified growth cones with APP, FE65, and GAP-43 antibodies. GAP-43 was used to monitor the purification procedure. H, Embryonic rat brain homogenate; GCP, growth cone particles; GCM, growth cone membranes. g, Dendritic filopodia (indicated by blue arrows) of a neuron transfected with FE65–EGFP. The fluorescence image is shown as an overlay on the DIC image. Dendrites were identified by conventional morphological criteria (see Materials and Methods) (Banker and Goslin, 1998
To ensure that FE65 immunoreactivity in growth cones could not be attributed solely to FE65LP, we transfected cultured primary neurons with cDNA encoding FE65 fused to EGFP (FE65–EGFP). Live imaging of FE65–EGFP confirmed the localization of FE65 in growth cones (Fig. 2e). In addition, FE65 and APP colocalized in the growth cones of differentiated SH-SY5Y cells, which do not express FE65LP (data not shown).
To determine whether APP and FE65 localize to growth cones in vivo, growth cones isolated from embryonic rat brain were probed for APP and FE65 by immunoblotting (Fig. 2f). These GCPs contain all proteins tested that are known to be in growth cones in vivo (Pfenninger et al., 1983
Interestingly, FE65–EGFP also localized to dendritic shaft filopodia (Fig. 2g), highly mobile structures known to depend on actin dynamics for their motility. At this stage of development, dendrites can be identified on the basis of their length (i.e., the axon is much longer than the dendrites) and by their decreasing caliper with increasing length (Banker and Goslin, 1998
FE65 and APP concentrate in growth cone peripheral domains
Growth cones can be divided into two functional domains: the central (C) domain and the peripheral (P) domain. The C domain is enriched in microtubules and organelles. The P domain is actin-rich, containing lamellipodia and filopodia, the most motile structures of the growth cone. If the APP/FE65 complex is involved in regulation of actin-dependent growth cone motility, then it should localize to the P domain.Immunofluorescent labeling for APP and FE65 showed that both proteins often concentrated in distal regions of the growth cone, likely corresponding to P domain lamellipodia, and frequently extended into the base of the filopodia (Fig. 3a,b). Occasionally, staining was seen down the length of filopodia. FE65 and APP antibodies also recognized small puncta in the C domain that might correspond to transport vesicles being delivered to the growth cone because APP travels via fast axonal transport (Koo et al., 1990
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Figure 3. FE65 and APP localize to growth cone P domains. Primary neuronal cultures from E17 rat brain were labeled with the indicated antibodies and stains and examined by confocal microscopy. a, b, Growth cone labeled with APP (a) and FE65 (b) antibodies. Images were pseudocolored with an intensity scale indicated by the guide. Blue represents the lowest intensity, and red represents the highest intensity. The most intense staining was often in the more distal region of the growth cone. c–f, Growth cone labeled with tubulin antibody to label microtubules (c) and with APP antibody (d) and phalloidin to label F-actin (e). APP colocalizes more strongly with actin in the P domain than with tubulin in the C domain. g–j, Growth cone labeled with tubulin antibody (g), FE65 antibodies (h), and phalloidin (i). FE65 also colocalizes more strongly with actin in the P domain than with tubulin in the C domain. Scale bars, 5 µm.
Because APP and Mena colocalize in lamellipodia of motile cells (Sabo et al., 2001
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Figure 4. APP and Mena colocalize in growth cones. Primary neuronal cultures from E17 rat brain were double-labeled with APP (a) and Mena (b) antibody and examined by confocal microscopy. Arrows point at the growth cone in the image. Colocalization is indicated by yellow in the overlay (c).
APP and FE65 interact in nerve terminals
In mature neurons, APP is enriched in nerve terminals (Koo et al., 1990
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Figure 5. APP and FE65 colocalize with synaptophysin at synapses. a–c, Confocal images of the axonal arbors of 7–8 DIV neurons double-labeled with APP (a) and synaptophysin (b) antibodies. Yellow in the overlay (c) represents colocalization of APP and synaptophysin. Arrows point at a few of the synaptic puncta that contain synaptophysin and APP. d, Thresholding and multiplication of the images in a and b yield only the overlapping signal. By comparison with the thresholded synaptophysin signal, this image was used to determine the fraction of synaptophysin-containing sites that also contain APP. e–g, Confocal images of the axonal arbors of neurons double-labeled with FE65 (e) and synaptophysin (f) antibodies. Yellow in the overlay (g) represents colocalization of FE65 and synaptophysin. Arrows point at a few of the synaptic puncta that contain synaptophysin and FE65. h, Thresholding and multiplication of the images in e and f yield only the overlapping signal. By comparison with the thresholded synaptophysin signal, this image was used to determine the fraction of synaptophysin-containing sites that also contain FE65.
To quantify the occurrence of FE65 and APP in synapses, the percentage of synaptophysin-positive synapses that also contained either FE65 or APP was determined. The fluorescence signals for APP (Fig. 5a) or FE65 (Fig. 5e) were thresholded and multiplied by the thresholded fluorescence signals for synaptophysin from the same neurons (Fig. 5b,f). The product of the two signals represents all sites in the image where either APP and synaptophysin (Fig. 5d) or FE65 and synaptophysin (Fig. 5h) colocalize. Of 191 synaptophysin-positive synapses counted along 9 randomly chosen axon segments, 67.6 ± 4.0% (mean ± SE) of the synapses contained APP, and 84.4 ± 5.0% (mean ± SE) of synaptophysin-positive synapses contained FE65 (n = 157 synapses from 11 axon segments). Because most neurons in the cultures were labeled by the antibodies, it was difficult to determine with this method whether the APP and FE65 were localized with synaptophysin in the presynaptic terminal or opposite synaptophysin in the postsynaptic terminal. Furthermore, it remained possible that diffuse cytoplasmic staining for FE65 could appear stronger at sites where neurites cross simply because the diffuse signals for the crossing neurites sum at their intersections.
To resolve these issues, 7–8 DIV neurons were cotransfected with FE65–EGFP and synaptobrevin–dsRed cDNAs. The localization of synaptobrevin–dsRed was identical to that of synaptobrevin–EGFP (data not shown), which is correctly targeted to synaptic vesicles (Miesenbock et al., 1998
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Figure 6. FE65–EGFP colocalizes with synaptobrevin–DsRed in living presynaptic terminals. a, b, e, f, Two examples of axon segments of neurons (7–8 DIV) that were double-transfected with FE65–EGFP (a, e) and synaptobrevin–DsRed (b, f) and then examined by live confocal imaging. c, g, Overlay of the FE65–EGFP and synaptobrevin–DsRed with the DIC image. Colocalization of the FE65–EGFP and synaptobrevin–DsRed is indicated by yellow in the overlays. Both proteins accumulate along the axon at sites of cell–cell contact, most likely corresponding to synapses. Contact can be seen in the DIC image where the labeled axon is crossed by or touched by an unlabeled neurite or soma. d, h, Overlap of FE65–EGFP and synaptobrevin–DsRed was extracted by thresholding and multiplying the two signals. The product reveals the sites that contain both proteins. Arrows point to cell–cell contacts that contain both proteins. Scale bars, 10 µm.
We did not perform a similar analysis of APP–EGFP because it is expected that cytoplasmic domain fusions with GFP would interfere with the interaction of FE65 and APP. However, because the colocalization of APP and FE65 is so strong by immunofluorescence, it seems that we can be confident that the localization of APP and FE65 at presynaptic contacts is likely to be similar. Furthermore, it has been demonstrated previously that APP is localized to presynaptic terminals (Caporaso et al., 1994
In randomly chosen segments of doubly transfected axons (n = 14), 380 sites of synaptobrevin accumulation were observed; 308 of these synaptobrevin-containing sites also appeared to contain FE65. Within individual axons, 81.0 ± 2.9% (mean ± SE for 14 axons) of presynaptic terminals also contained FE65. This is not significantly different from the values obtained by immunofluorescence colocalization with synaptophysin (p > 0.05 by ANOVA), supporting the idea that most of the colocalization seen by immunofluorescence was within the presynaptic terminal.
Of the 126 synaptobrevin and FE65-containing sites in images in which phase-contrast images were also captured, 124 appeared to occur at sites of contact with another neuron and therefore were probable synapses. Focal accumulation of FE65–EGFP was not seen at sites that did not appear to correspond to cell–cell contacts. Moreover, FE65–EGFP fluorescence appeared stronger at sites with a larger contact area. Some diffuse cytoplasmic staining of FE65 was seen throughout many of the neuronal processes, which is not surprising because FE65 is a soluble cytosolic protein. This staining was strongest in proximal regions of the neuronal processes, consistent with the synthesis of FE65 in the cytosol and its diffusion into regions closest to the cell body.
In young neurons, synaptobrevin can be found associated with mobile transport packets that are not synapses (Ahmari et al., 2000
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Figure 7. FE65 and synaptobrevin-containing synapses are stable over time. a–c, Time-lapse confocal microscopy of neurons transfected with FE65–EGFP and synaptobrevin–DsRed. a, FE65–EGFP in an axon segment at the start of imaging. b, Synaptobrevin–DsRed in the same axon segment at the start of imaging. c, Overlap of FE65–EGFP and synaptobrevin–DsRed signals at the start of imaging (t=0') and at 7, 13, and 20 min after the start of imaging (7', 13', 20', respectively). Arrows point to stationary presynaptic terminals. The blue arrowhead points to a synaptobrevin-containing site that leaves the field of view during imaging (compare 13' and 20'). The yellow arrowhead points to a synaptobrevin-containing site that enters the field of view during imaging (compare t=0' and 7') and then remains stable for the duration of imaging. Scale bars, 10 µm.
To confirm the presence of FE65 with APP in the presynaptic nerve terminal in vivo, synaptosomal fractions were purified from rat brain and immunoblotted with FE65 and APP antibodies. Both FE65 and APP were found in synaptosomes (Fig. 8a), supporting our imaging results. To verify that FE65 from nerve terminals binds to APP, the cytoplasmic domain of APP fused to GST (GST–C50) was immobilized on glutathione–Sepharose beads and then incubated with synaptic membranes (P2). Immunoblotting of bound proteins with FE65 antibodies revealed that synaptic FE65 coprecipitated with GST–C50 but not with GST alone or with an unrelated GST-fusion protein (Fig. 8b). Thus FE65 from nerve terminals binds to APP.
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Figure 8. FE65 interacts with APP in nerve terminals. a, Synaptosomes probed for FE65 and APP expression by immunoblotting. b, Coprecipitation of FE65 from synaptosomes (P2) with APP fused to GST (GST–C50). GST alone (GST) and GST fused to a portion of FE65 (GST–PID) were used as negative controls. c, Synaptic organelles immunoisolated with anti-synaptophysin (synaptophysin), anti-synaptobrevin (synaptobrevin), or anti-rab5 (rab-5) antibodies were immunoblotted for FE65, APP, and synaptophysin. d, Small synaptic vesicles (SG2) were separated from other small synaptic membranes (SG4) by sucrose gradient centrifugation and examined by immunoblotting with FE65 and APP antibodies. The effective higher spatial resolution afforded by the immunoisolation and fractionation approaches, as compared with fluorescence imaging shown in Figures 5 and 6, shows that APP and FE65 are found in a population of synaptic organelles that are distinct from the small synaptic vesicles that contain synaptophysin and synaptobrevin. PID, Protein interaction domain.
Like APP, FE65 associates with rab-5-containing organelles but not with synaptic vesicles
At nerve terminals, APP is localized to Rab5-containing organelles that are distinct from small synaptic vesicles (Ikin et al., 1996Preferential binding to small synaptic vesicles resulted in nearly equal association with synaptic vesicle protein and Rab5 immunoisolates, as illustrated by immunoblotting for synaptophysin. Conversely, preferential association with the Rab5-containing organelles yielded enrichment in the Rab5 fraction, as shown by immunoblotting for APP. Like APP, FE65 was highly enriched in Rab5 immunoisolates compared with synaptophysin or synaptobrevin fractions and therefore was preferentially associated with the Rab5-containing organelle.
To confirm these results, synaptic organelles were separated by sucrose gradient centrifugation and examined by immunoblotting. Fraction 2 of the sucrose gradient (SG2) is enriched in small synaptic vesicles, whereas fraction 4 (SG4) contains other synaptic organelles, such as the Rab5- and APP-containing organelle. Consistent with the immunoisolation results, FE65 and APP were enriched in SG4 compared with SG2 (Fig. 8d). Although FE65 is a cytosolic protein, it cofractionated with membranes that contained APP but not with those that did not, suggesting that FE65 specifically associates with APP-containing synaptic membranes through its interaction with APP.
Discussion
Here we have shown that FE65 localizes with APP in the peripheral regions of neuronal growth cones, in nerve terminals, and in dendritic filopodia. Dynamic actin plays an important role in each of these subcellular domains, regulating both neuronal development and function. We have shown previously that an APP/FE65 complex localizes to actin-rich lamellipodia of non-neuronal cells and regulates cell motility (Sabo et al., 2001FE65 and APP localized to neuronal growth cones both in vitro and in vivo. The P domains of growth cones are known to be enriched in dynamic actin filaments. These actin filaments are essential for the formation and movement of the growth cone lamellipodia and filopodia. Lamellipodia and filopodia are important for the ability of growth cones to crawl toward their targets and for the growing neurite to sense and respond to its environment.
The localization of FE65 and APP in the growth cone P domain suggests a role for the APP/FE65 complex in regulation of growth cone motility. Effects on growth cone motility are expected to result in altered axon outgrowth. There is evidence in support of APP-dependent regulation of axon growth. For example, APP synthesis and axonal transport coincide with periods of axon elongation and synapse formation (Hung et al., 1992
In addition to its localization in growth cones, FE65–EGFP was seen in dendritic filopodia. Dendritic filopodia are thought to be precursors to dendritic spines, which contain the postsynaptic terminals of excitatory synapses. Actin dynamics are believed to provide the structural basis for spine formation and for the rearrangements that are necessary for plasticity of the postsynaptic terminals of mature excitatory synapses (Halpain, 2000
F-actin is essential for the development and maintenance of young synapses (Zhang and Benson, 2001
We showed here that both APP and FE65 localize to presynaptic terminals in vitro and in vivo by immunofluorescence and subcellular fractionation, respectively. Immunofluorescence demonstrated that APP and FE65 localize to synapses that contain synaptophysin. We also confirmed with time-lapse imaging of living neurons that FE65 localizes to synaptobrevin-containing presynaptic terminals. The higher resolution afforded by the fractionation approaches revealed that within synapses APP and FE65 localize to different organelles than synaptophysin. On the basis of the molecular weight of the APP in synaptosome fractions and on our ability to localize APP to nerve terminals by immunofluorescence with either N-terminal or C-terminal antibodies, it is likely that there is a substantial pool of full-length APP that is capable of interacting with FE65 in synapses. We confirmed that FE65 from synapses interacts with APP by performing coprecipitations. Overall, our data are consistent with a role for an APP/FE65 complex in synapses.
We have shown previously that the APP/FE65 complex regulates the motility of non-neuronal cells (Sabo et al., 2001
Morphological changes, such as those seen during motility, require coordination of cytoskeletal and membrane dynamics. Recent evidence links membrane dynamics important for motility to actin cytoskeletal dynamics through Rab5. Rab5 mediates phorbol ester-induced cell motility and actin cytoskeleton reorganization (Imamura et al., 1998
Footnotes
Received Feb. 12, 2003; revised Apr. 28, 2003; accepted Apr. 28, 2003.This work was supported by United States Public Health Service Grants AG09464 (P.G.) and AG14996 (J.D.B.), Alzheimer Association grants (J.D.B, A.F.I), National Institutes of Health Training Grant GM07524 (S.L.S.), and a Rockefeller University fellowship (S.L.S.). We also thank the Mount Sinai Hybridoma Shared Research Facility. We thank Drs. E. H. Koo and F. Gertler for antibodies and Dr. F. Benfenati for synaptic vesicles. We thank Drs. A. K. McAllister and N. Spitzer for advice on live imaging.
Correspondence should be addressed to Shasta L. Sabo, Center for Neuroscience, University of California, Davis, 1544 Newton Court, Davis, CA 95616. E-mail: slsabo{at}ucdavis.edu.
Copyright © 2003 Society for Neuroscience 0270-6474/03/235407-09$15.00/0
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