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The Journal of Neuroscience, July 1, 2000, 20(13):4912-4921
Active Zones on Motor Nerve Terminals Contain
3
1 Integrin
Monroe W. Cohen1, Benjamin G. Hoffstrom2, and Douglas W. DeSimone2 1 Department of Physiology, McGill University, Montreal, Quebec Canada H3G 1Y6, and 2 Department of Cell Biology, University of Virginia, Charlottesville, Virginia 22908
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Active zones are the sites along nerve terminals where synaptic vesicles dock and undergo calcium-dependent exocytosis during synaptic transmission. Here we show, by immunofluorescent staining with antibodies generated against Xenopus laevis integrins, that
3
1 integrin is concentrated at the active zones of Xenopus motor nerve terminals. Because integrins can link extracellular matrix molecules to cytoskeletal elements and participate in the formation of signaling complexes, the localization of integrin at active zones suggests that it may play a role in the adhesion of the nerve terminals to the synaptic basal lamina, in the formation and maintenance of active zones, and in some of the events associated with calcium-dependent exocytosis of neurotransmitter. Our findings also indicate that the integrin composition of the terminal Schwann cells differs from that of the motor nerve terminals, and this may account at least in part for differences in their adhesiveness to the synaptic basal lamina.
Key words: active zones;
INTRODUCTION
Integrins are a large family of transmembrane heterodimers. They can interact with and establish a link between extracellular matrix and cytoskeletal molecules and can also participate in the generation of signaling cascades. The expression of the individual
; Clarke and Brugge, 1995
Integrins are differentially expressed in different regions of the nervous system (Pinkstaff et al., 1999
Besides having a postsynaptic localization, integrins can also be present presynaptically. The
In the present study we have used antibodies generated against Xenopus laevis integrins to examine, by immunofluorescent staining, the localization of integrins at Xenopus neuromuscular junctions. These synapses are particularly advantageous for assessing precise localization because the junctional folds and apposed active zones have a characteristic pattern of distribution, and the presynaptic and postsynaptic elements can be separated from each other. Our results reveal that the
MATERIALS AND METHODS
Animals and surgical procedures. Xenopus laevis frogs, weighing <2 gm, were anesthetized in 0.5 mg/ml tricaine methanesulphonate. The sartorius muscles were removed and stored at low temperature (4-6°C) in a solution consisting of 67% (v/v) L-15 and 1% (v/v) goat serum (Life Technologies, Burlington, ON, Canada). To denervate sartorius muscles, animals were anesthetized, and their left spinal nerve was resected shortly after its exit from the spinal cord. Care was taken not to injure any blood vessels. Muscles were removed 3 or 6 d later.
Fluorescent staining and imaging. Sartorius muscles were stained alive at low temperature (4-6°C). The standard bathing solution consisted of 67% (v/v) L-15 and 1% (v/v) goat serum. Muscles were exposed to the primary and secondary antibodies for at least 2 hr and were rinsed several times over a period of at least 20 min after each antibody. Fluorescent toxins were usually included with the secondary antibody but were sometimes used earlier in the staining protocol. After being stained the muscles were rinsed with 67% L-15 and fixed with 2% formaldehyde for at least 1 hr. For some experiments, the muscles were treated with l mg/ml collagenase (Life Technologies) in 67% L-15 for 1 hr at room temperature (22-25°C) before fixation. The collagenase solution also contained 1.5 µM tetrodotoxin (Sigma, St. Louis, MO). Some fixed muscles were subsequently rinsed with 67% L-15, permeabilized with 1% Triton X-100 (30 min at 4-6°C), and stained for the synaptic vesicle protein SV2. The staining protocol after fixation and permeabilization was the same as described for the initial staining of living muscles. After staining and rinsing, the muscles were stored in the fixative.
Individual muscle fibers were isolated from the fixed muscles. Typically, each of the isolated fibers contained two to three neuromuscular junctions, but no attempt was made to include the myotendinous junction. At least 20 muscle fibers from each muscle were mounted on glass slides. The mounting medium consisted of 10 mg/ml p-phenylenediamine, 10 mM sodium carbonate, and 90% (v/v) glycerol. The slides were examined on a Zeiss IM35 microscope equipped with appropriate oil-immersion objectives and filters for viewing fluorescein, rhodamine and Cy3, and aminomethylcoumarin (AMCA) fluorescence as well as phase contrast. High (100× objective) and low (25× objective) magnification photographs were taken with T-MAX 3200 Kodak (Eastman Kodak, Rochester, NY) film. The negatives were digitized on an MCID-M4 imaging system (Imaging Research, St. Catharine's, Ontario, Canada), and figures were prepared using Adobe PhotoShop.
The following anti-Xenopus integrin mouse monoclonal antibodies (mAbs) were prepared and characterized (see below): P2A5 and P7A12 directed against
-conotoxin (R
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Table 1. Integrin immunofluorescence along muscle cellsa Characterization of anti-integrin monoclonal antibodies. Xenopus S3-1 cells represent a clonal cell line that was isolated from trypsinized dorsal explants of stage 18 neurulae cultured in 61% L-15 media containing 10% FBS. These cells were selected for use as immunogen on the basis of their adhesion to a variety of extracellular matrix substrates, including fibronectin, and for the presence of multiple integrins on their cell surface. Mice were immunized with live S3-1 cells, and anti-Xenopus mAbs were generated using the methods for hybridoma fusion and screening described by Wayner and Carter (1987)
Four mAbs (P2A5, P7A12, P2A7, P3C12) from this screen were used in the current study and characterized by immunoprecipitation and Western blot analyses. Unlabeled S3-1 cells and S3-1 cells surface-labeled with sulfosuccinimidyl-6-(biotinamido) hexanoate (NHS-LC- Biotin; Pierce, Rockford, IL) were washed in PBS and extracted in IP buffer (1% NP-40, 10 mM Tris, pH 7.75, 150 mM NaCl, 1 mM PMSF, 2 µg/ml aprotinin, 2 µg/ml leupeptin, and 1 µg/ml pepstatin A). Integrins were immunoprecipitated from biotin-labeled and unlabeled cell extracts (1.0 × 105 cell equivalents) using mAbs (2 µg/ml) and goat anti-mouse coupled agarose (Sigma) as described in Hens and DeSimone (1995)
RESULTS
Characterization of anti-Xenopus integrin monoclonal antibodies
The specificities of the Xenopus-specific anti-integrin mAbs were established by immunoprecipitation and Western blot analyses of Xenopus S3-1 cell extracts. S3-1 represents a clonal line of cells obtained from dorsal explants of neurula stage embryos. As shown in Figure 1, immunoprecipitation of biotin-labeled S3-1 cells with an anti-
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Figure 1. Specificity of mAbs directed against Xenopus integrins. For lanes 1-5, Xenopus S3-1 cells were labeled by cell-surface biotinylation, extracted in IP buffer, and immunoprecipitated using the following mAbs: 8C8 (anti-
A similar approach was used to confirm the specificities of the anti-
Staining patterns with mAb P2A5 (anti-
Figure 2 shows face views of portions of two different neuromuscular junctions stained for AChRs,
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Figure 2. Face views of two neuromuscular junctions (A, B) stained for AChRs (top panels),
Although there was extensive congruity between the AChR bands and the integrin bands, subtle differences were also observed. Examples of such differences are indicated by the numbered lines in Figure 2. Line 1 points to a short AChR band with no corresponding integrin stain. Some AChR bands were longer than the corresponding integrin bands (lines 2), and sometimes an integrin band was segmented, whereas the corresponding AChR band was not (line 3). Occasionally short integrin bands had no corresponding AChR fluorescence (lines 4), and some integrin bands were longer than the corresponding AChR band (line 5).
In side views of neuromuscular junctions (Fig. 3), the AChR stain consisted of a thin line with short, periodic, perpendicular extensions. The latter are the sites where the postsynaptic membrane invaginates to form the junctional folds, whereas the thin continuous horizontal line of AChR fluorescence is attributable to the presence of AChRs in the noninvaginated portion of the postsynaptic membrane between the junctional folds (Anderson and Cohen, 1974
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Figure 3. Side views of two neuromuscular junctions (A, B) stained for AChRs (top panels),
In addition to its presence at neuromuscular junctions, integrin immunofluorescence was observed elsewhere along the muscle cells. This consisted of faint immunofluorescence along the entire surface of the muscle cells and brighter immunofluorescence localized at costameres and satellite cells (see Fig. 7A). The intensity of the integrin immunofluorescence at these sites, like that at the terminal Schwann cells, was variable. When the integrin stain at terminal Schwann cells was faint or undetectable, so too was the integrin stain at neighboring costameres and satellite cells, even though the synaptic integrin bands were relatively bright, and the SV2 immunofluorescence was also bright (Fig. 2B). Presumably such cases involved teased muscle cells whose neuromuscular junctions were originally positioned more deeply within the whole muscle so that during the staining protocol they were exposed to a lower concentration of antibody than the more superficial ones. In support of this notion, when the staining protocol was performed with a tenfold lower concentration of mAb P2A5 there was often no detectable immunofluorescence at terminal Schwann cells, costameres, and satellite cells even though integrin bands, in spatial register with the AChR bands, were still observed at neuromuscular junctions (Table 1). This preferential staining of the synaptic membrane may reflect a higher affinity of the antibody for the synaptic integrin and/or a greater concentration of integrin at the synaptic sites than at Schwann cells, costameres, and satellite cells.
Staining patterns with other anti-integrin mAbs
The staining patterns obtained with mAb P7A12, which like mAb P2A5 is directed against
mAb P2A7, which is directed against
Staining the sartorius muscle for
The staining pattern obtained with mAb 8C8, which is directed against the
Staining patterns in denervated muscle
After denervation, motor nerve terminals degenerate and are phagocytosed by the terminal Schwann cells that remain at the neuromuscular junctions even after all motor nerve terminal remnants have been eliminated (Birks et al., 1960b
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Figure 4. Disappearance of synaptic bands of
Presynaptic location of synaptic integrin bands
The absence of synaptic integrin bands at denervated neuromuscular junctions suggests that, at innervated neuromuscular junctions, they are associated with active zones on the motor nerve terminals. An additional possibility is that they are associated with the postsynaptic membrane at the tops of the junctional folds, but their survival there requires the presence of intact motor nerve terminals. To assess whether the synaptic integrin bands are associated with motor nerve terminals, muscles were treated with collagenase to displace the nerve terminals from their neuromuscular junctions. Such enzymatic treatment, by digesting the synaptic basal lamina, weakens the adhesion of the motor nerve terminals to their muscle cells and makes them susceptible to displacement (McMahan et al., 1972
Figure 5 shows a low-magnification view of a neuromuscular junction after enzymatic treatment. The AChR fluorescence (top panel) reveals the location of the postsynaptic membrane, and the SV2 immunofluorescence (third panel) reveals that the motor nerve terminal was partially displaced from the postsynaptic membrane. A short length of displaced nerve terminal is seen on the left side of the figure, and a longer length is seen on the right. Portions of the displaced motor nerve terminal are also apparent in the phase-contrast image (bottom panel). Significantly, the integrin immunofluorescence (obtained with mAb P2A5; second panel) was associated with the displaced nerve terminal, whereas the portion of postsynaptic membrane that lacked motor nerve terminal (bracket in top panel) also lacked integrin stain. This absence of integrin immunofluorescence along nerve terminal-free portions of postsynaptic membrane was also observed in cases in which the surrounding costameres and neighboring satellite cells had relatively bright integrin immunofluorescence (see Fig. 7).
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Figure 5. Low-magnification view of a neuromuscular junction treated with collagenase. Comparison of the AChR fluorescence (top panel) and the SV2 immunofluorescence (third panel) reveals that the motor nerve terminal was displaced from a portion of the postsynaptic membrane (top panel, bracket). Displaced nerve terminal branches are also apparent in the phase-contrast image (bottom panel, arrowheads). The
Figure 6 shows higher magnification views of the framed areas in Figure 5. At the portion of neuromuscular junction that remained intact the synaptic integrin bands had become disorganized. Many of the individual integrin bands were no longer spatially aligned with the transversely oriented AChR bands, and some even had a horizontal orientation. In addition, the integrin bands were less numerous than the AChR bands. Such changes are similar to those that have been described for active zones examined by electron microscopy after enzymatic treatment (Nystrom and Ko, 1988
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Figure 6. Higher magnification view of framed portions of Figure 5. Top panels, AChR stain; middle panels,
Integrin bands having a variety of orientations were also observed on the displaced motor nerve terminals. As seen in the examples of Figures 6 and 7, the integrin bands on the displaced motor nerve terminals had an appearance that was essentially similar to the appearance of the integrin bands at intact portions of enzyme-treated neuromuscular junctions. Similar results were obtained when mAb P7A12 was used instead of mAb P2A5. Taken together, these observations indicate that the
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Figure 7. Synaptic and nonsynaptic staining patterns after treatment with collagenase. A, Low magnification view of AChR stain (top panel),
Further confirmation of this conclusion was obtained by comparing the distribution of presynaptic N-type calcium channels, known to be located at the active zones of frog motor nerve terminals (Robitaille et al., 1990
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Figure 8. Active zones altered by collagenase treatment contain
DISCUSSION
This study has indicated that
That
That
Specific
Another potential role for the integrin at active zones is participation in one or more of the steps involved in calcium-dependent exocytosis of neurotransmitter. Current models suggest that nerve terminal membrane proteins such as syntaxin, SNAP-25, and RIM interact with proteins on the surface of the synaptic vesicles, directly or indirectly, to permit targeting of synaptic vesicles to the active zone, docking of the synaptic vesicle at that site, and the subsequent fusion of the synaptic vesicle membrane with that of the nerve terminal (Calakos and Scheller, 1996
The presence of integrins on terminal Schwann cells may also be consequential for synaptic structure and function. Schwann cells respond to nerve and muscle damage, act as a guide for nerve sprouts and regenerating nerve terminals, and can influence the stability of the developing neuromuscular junction (Birks et al., 1960b
FOOTNOTES Received Feb. 25, 2000; revised April 6, 2000; accepted April 10, 2000.
This work was supported by a grant to M.W.C. from the Medical Research Council of Canada and by grants to D.W.D. from the United States Public Health Service (HD26402 and HD01104). D. McDonald and T. Inoue provided expert technical assistance. We thank S. Carbonetto for monoclonal antibody 8C8, S. S. Carlson for the anti-SV2 antibody, and O. T. Jones for R
Correspondence should be addressed to M. W. Cohen, Department of Physiology, McGill University, 3655 Drummond Street, Montreal, Quebec, Canada H3G 1Y6. E-mail: monroe{at}med.mcgill.ca.
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