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Previous Article | Next Article
The Journal of Neuroscience, November 15, 1999, 19(22):9890-9899
The Extracellular Matrix Modulates Olfactory Neurite Outgrowth on Ensheathing Cells
Katarina T. Tisay1 and Brian Key2 1 Department of Anatomy and Cell Biology, University of Melbourne, Victoria 3052, Australia, and 2 Neurodevelopment Laboratory, Department of Anatomical Sciences, University of Queensland, Brisbane 4072, Australia
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Primary olfactory axons grow along a stereotypical pathway from the nasal cavity to the olfactory bulb through an extracellular matrix rich in laminin and heparan sulfate proteoglycans (HSPGs) and bounded by the expression of chondroitin sulfate proteoglycans (CSPGs). This pathway is pioneered by olfactory ensheathing cells, which provide a substrate conducive for axon growth during early development. In the present study, we examined the effect of several extracellular matrix constituents on the spreading and migration, as well as the neurite outgrowth-promoting properties, of olfactory ensheathing cells. Laminin and Matrigel enhanced the spreading and migration of olfactory ensheathing cells and increased their neurite outgrowth-promoting activity. In contrast, HSPG and CSPG had little effect on the spreading and migration of olfactory ensheathing cells and hence did not promote olfactory neurite outgrowth. In vitro olfactory axons grew preferentially on the surface of olfactory ensheathing cells rather than the underlying extracellular matrix. We propose that olfactory ensheathing cells secrete laminin and HSPGs, which together with other cofactors, stimulate these cells to migrate and adopt a neurite outgrowth-promoting phenotype. Expression of CSPGs in the surrounding mesenchyme confines the growth of ensheathing cells, as well as the axons, which grow on the surface of these cells, to a specific pathway. Thus, the ECM indirectly modulates the growth and guidance of olfactory axons during development.
Key words: neurite outgrowth; laminin; proteoglycan; ensheathing cells; chondroitin sulfate; primary olfactory neuron
INTRODUCTION
Olfactory ensheathing cells (OECs) are specialized glia that ensheathe bundles of primary olfactory axons. These cells are born in the olfactory neuroepithelium (OE) and migrate together with growing axons, populating both the olfactory nerve and nerve fiber layer of the olfactory bulb (Tennent and Chuah, 1996
). OECs are a highly conducive substrate for primary olfactory axon outgrowth in vitro (Goodman et al., 1993
OECs are not lineally related to Schwann cells in other peripheral nerves; they are instead derived from progenitor cells within the olfactory placode (Chuah and Au, 1991
The spatiotemporal expression pattern of various components of the extracellular matrix in the developing olfactory nerve pathway suggests that these molecules may play an important role in the growth and guidance of primary olfactory axons. For instance, laminin, heparan sulfate proteoglycan (HSPG), and collagen IV are expressed along the olfactory nerve pathway (Doucette, 1996
Although the ECM may directly affect the growth of primary olfactory axons, we have suggested previously that it modulates the outgrowth-promoting properties of OECs (Key et al., 1996
MATERIALS AND METHODS
Explant cultures of olfactory neuroepithelium. Timed pregnant Sprague Dawley rats were anesthetized with Nembutal (80 µl/100 gm body weight) at embryonic day 19.5 (E19.5). The morning of positive sperm dam was designated E0.5. Embryos were removed aseptically and decapitated, and the posterior third of the nasal septum with attached olfactory neuroepithelium was removed. The olfactory neuroepithelium was peeled from the nasal septum and cut into explants ~1 mm2 in size. Explants were plated onto 12 mm Millicell-M culture inserts (Millipore, Bedford, MA), which were coated previously with various substrates. Membranes were prepared by diluting each substrate in sterile PBS, pH 7.4, and incubating 100 µl of each solution overnight at room temperature. Membranes were then washed three times with PBS and twice with warmed medium, before explant plating. The substrates used were as follows: poly-L-lysine (PLL) (100 µg/ml; Sigma, St Louis, MO), Matrigel basement membrane matrix secreted by Englebreth-Holm-Swarm (EHS) mouse sarcoma cells (1540 µg/ml; Collaborative Research, Bedford, MA), EHS-laminin (100 µg/ml; Collaborative Research), EHS-HSPG (10 µg/ml; Sigma), and CSPG A from bovine trachea (10 µg/ml; Sigma). Cultures were maintained in DMEM (Sigma) containing 10% fetal bovine serum (v/v), Monomed serum-free hybridoma supplement (Commonwealth Serum Laboratories, Melbourne, Australia), and gentamicin (50 µg/ml). In some experiments, cytosine arabinoside (10 µM; Sigma) and 5-fluoro-2'-deoxyuridine (10 µM; Sigma) were included in the culture medium. Explants were cultured for 5 d at 37°C in 5% carbon dioxide, then fixed in methanol at
20°C or in 4% paraformaldehyde for 30 min, and washed in PBS before removing the membranes from the plastic inserts.
Isolation of olfactory ensheathing cells. Neonatal Sprague Dawley rats [postnatal day 7 (P7)-P8] were killed by decapitation, and the posterior half of the nasal septum with attached olfactory neuroepithelium was collected. The olfactory neuroepithelium was dissected from the nasal septum, and fine forceps were used to tease away large olfactory nerve fascicles from the lamina propria. These nerve fascicles were incubated in a mixture of trypsin-versene (Commonwealth Serum Laboratories), collagenase-dispase (1 mg/ml; Sigma), and RQ1 DNase (10 U; Promega, Madison, WI) at 37°C for 15 min. Enzymatic digestion was stopped by the addition of 500 µl of medium containing 10% (v/v) fetal bovine serum (dialyzed to remove molecules below 1000 Da; Sigma), and the tissue was centrifuged at 1000 rpm for 5 min. The pellet of tissue was washed with warmed medium, recentrifuged for another 5 min, and then resuspended in 1 ml of culture medium. The olfactory nerve fascicles were mechanically dissociated by trituration until semidissociated and plated into two to three wells of a 24-well plate (Nunc, Naperville, IL). The culture medium consisted of minimal essential D-valine medium (Sigma), 10% (v/v) dialyzed fetal bovine serum, and gentamicin (50 µg/ml). OECs were maintained at 37°C in 5% CO2 for 6 d. OECs were then subcultured as a dissociated culture into four-well chamber slides as follows (Nunc). OECs were rinsed with PBS and then incubated in trypsin-versene for 5 min. To inactivate the trypsin, 500 µl of warmed medium was added to each well, and cells were dislodged by trituration. The cell suspension was pelleted (1000 rpm) for 5 min, washed with warmed medium, and recentrifuged. Cells were plated at 10,000 cells per well and cultured for another 6 d. Cultures were fixed in methanol for 20 min at
Olfactory ensheathing cells on ECM-coated coverslips. Round glass coverslips (12 mm) were cleaned overnight in concentrated nitric acid, washed thoroughly with distilled water, and air dried. Coverslips were then immersed in 70% ethanol (v/v) and flame sterilized. Coverslips were coated with poly-L-lysine (1 µg/ml) for 2 hr, washed with PBS, and then coated with various ECM molecules for another 2 hr. The different substrata used were as follows: chondroitin sulfate proteoglycan (0.1, 1, and 10 µg/ml), heparan sulfate proteoglycan (0.1, 1, and 10 µg/ml), EHS-Matrigel (15.4, 154, and 1540 µg/ml), and EHS-laminin (1, 10, and 100 µg/ml). OECs were subcultured as described above and plated on to the coated glass coverslips at a density of 3000 cells per coverslip. Twenty-four hours after plating, coverslips were washed with fresh medium and fixed in methanol for 20 min at
Neural cell adhesion molecule immunostaining of explant cultures. Explant cultures that had been fixed in methanol were washed with Tris-buffered saline (TBS), pH 7.4, blocked with 2% bovine serum albumin (BSA) (Sigma) in TBS, and incubated overnight at 4°C with a rabbit polyclonal neural cell adhesion molecule (N-CAM) antiserum (1:500) (Akeson et al., 1988
Double-label immunostaining of explant cultures. Explants previously fixed in 4% paraformaldehyde were washed with TBS and 0.3% Triton X-100, pH 7.4, and blocked with 2% BSA in TBS and 0.3% Triton X-100. Explants were incubated overnight at 4°C with mouse ascites against
-tubulin III (1:200; Sigma), washed with TBS and 0.3% Triton X-100, and then incubated overnight at 4°C with rabbit anti-human p75 immunoglobulins (1:200; Promega). Explants were then washed with TBS and 0.3% Triton X-100, incubated for 1 hr with horse anti-mouse immunoglobulins (1:200; Vector Laboratories, Burlingame, CA), and rewashed. Next, the tissue was incubated with tetramethyl rhodamine isothiocyanate-labeled extra avidin (1:50; Sigma) and FITC-labeled goat anti-rabbit immunoglobulins for 1 hr, washed thoroughly with TBS and 0.3% Triton X-100, mounted on glass slides, coverslipped with an aqueous mounting medium, and then visualized by confocal microscopy.
Immunostaining cultures of olfactory ensheathing cells. Primary cultures of olfactory ensheathing cells were washed with TBS and 0.3% Triton X-100, followed by blocking in 2% BSA in TBS and 0.3% Triton X-100. After 1 hr, cells were incubated overnight at 4°C with polyclonal antibodies against GFAP (1:200; Dako, Carpinteria, CA), S-100 (1:1000; Dako Corporation), p75 (1:500), or with a monoclonal anti-p75 antibody (1:20; Boehringer Mannheim, Indianapolis, IN). Cells were washed with TBS and 0.3% Triton X-100 and incubated for 1 hr with an appropriate biotinylated secondary antibody (1:200). The secondary antibodies used were horse anti-mouse immunoglobulins (Vector Laboratories) or goat anti-rabbit immunoglobulins (Vector Laboratories). The cultures were washed again and incubated for 1 hr with the avidin-biotin horseradish peroxidase complex (Vectastain Elite ABC kit; Vector Laboratories). Next, the cultures were washed with TBS and 0.3% Triton X-100, rinsed in TBS, and then reacted with 3,3-diaminobenzidine (0.5 mg/ml) in the presence of 0.02% H2O2. No nonspecific staining of olfactory ensheathing cells was observed in control incubations using either nonimmune sera or no primary antisera.
Characterization of olfactory ensheathing cells. The purity of dissociated olfactory ensheathing cell cultures was analyzed by determining the percentage of flat cells and spindle-like cells that expressed each glial marker. Cells were counted in three randomly selected fields from at least three different cell cultures. The number of cells that spread (cells with no birefringence under bright-field microscopy) on the ECM-coated coverslips was determined by counting the percentage of cells with spindle-like morphology (with processes) and flat ovoid morphology (without processes) in one field from each coverslip (n = 9). Counts were expressed as percentages and presented as the mean percentage of cells that spread or did not spread. Data were statistically analyzed by the Kruskal-Wallis and Mann-Whitney tests for nonparametric statistics. The total length of OEC processes was measured using the Image-Pro Plus image analysis computer package (Media Cybernetics, Silver Spring, MD). Digital images of 20 randomly selected OECs were recorded from three coverslips, and the length of every process was measured. Because OECs typically had one long process and one to two short processes, data were expressed as total length of processes per cell. Data were then averaged and statistically analyzed by one-way ANOVA and Tukey's multiple comparisons.
Neurite outgrowth from explant cultures. Neurite outgrowth from explants of olfactory neuroepithelium was quantified using the Image-Pro Plus computer package. Digital images of each explant (n = 82) were binarized, and the total surface area of neurites was measured. Axon area was measured from the edge of each explant and did not include any axons that had grown over the top of explants. Data were analyzed by one-way ANOVA and Tukey's multiple comparisons.
RESULTS
Qualitative observations of explant cultures of olfactory neuroepithelium
The expression pattern of various components of the ECM in the developing olfactory nerve pathway suggests that these molecules may modulate the growth and guidance of primary olfactory axons en route to the olfactory bulb. To investigate the interplay between the ECM and migrating glia and olfactory neurites, explants of OE from E19.5 Sprague Dawley rats were plated onto Millicell-CM inserts coated with various substrates. When OE explants were cultured on a substrate of Matrigel for 5 d, there was considerable cellular migration away from the explant (Fig. 1A). These cells formed a dense sheet between adjacent explants and were identified as OECs because they weakly expressed N-CAM (Fig. 1A) and strongly expressed p75 (Fig. 1B). Growing over the surface of the sheet of ensheathing cells were numerous small fascicles of neurites, as well as N-CAM reactive olfactory neurons (Fig. 1A,C, arrows). The large amount of cell migration on Matrigel made it difficult to analyze and quantify the level of neurite outgrowth because the neurites were often in small bundles, which branched and defasciculated, interweaving between adjacent ensheathing cells (Fig. 1A, arrowhead). To decrease OEC proliferation, cytosine arabinoside and fluorodeoxyuridine were added to the culture medium. In the presence of these two mitotic inhibitors, the extent of OEC migration was considerably reduced and neurites grew in large bundles, rarely extending further than the edge of the OEC sheet (Fig. 1C).
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Figure 1. Explant cultures of E19.5 olfactory neuroepithelium grown on Matrigel (154 µg/ml). Explant in A was grown in culture medium that did not contain any mitotic inhibitors. In B and C, explants were grown in medium that contained cytosine arabinoside and fluorodeoxyuridine. A, N-CAM immunostaining revealed bundles of olfactory neurites growing over the surface of OECs. OECs have formed a dense sheet of cells that weakly expressed N-CAM (arrow). Bundles of neurites defasciculate and grow between adjacent OECs (arrowhead). B, p75 is expressed by OECs (arrow), which have migrated from the explant. C, N-CAM immunostaining demonstrates large bundles of neurites growing over the surface of ensheathing cells. In these cultures, the extent of cell migration is markedly reduced (arrow). Scale bars, 200 µm.
Neurite outgrowth is promoted when explants are plated on laminin and Matrigel
We have proposed previously that expression of laminin and heparan sulfate proteoglycans in the olfactory nerve pathway provide a conducive substrate for axon growth, whereas expression of chondroitin sulfate proteoglycans surrounding the pathway act to restrict axon growth (Treloar et al., 1996
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Figure 2. Explant cultures of E19.5 olfactory neuroepithelium plated on different substrates. Cultures were grown in the presence of cytosine arabinoside and fluorodeoxyuridine and were immunostained for N-CAM. When explants were plated on PLL (A) (0.1 µg/ml), CSPG (B) (1 µg/ml), and HSPG (C) (1 µg/ml), there was a low level of neurite outgrowth. Neurite outgrowth was confined to the upper surface and the edges of the explants. Large numbers of N-CAM-positive olfactory neurons (Calof and Chickaraishi, 1989
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Figure 3. Double-label immunofluorescence of neurites extending from an explant plated on Matrigel (154 µg/ml). A, Immunostaining for
The extent of neurite outgrowth from the explants (n = 82) was determined by measuring the surface area of N-CAM-labeled processes in digital images. There was no significant difference between the mean area of neurite growth from explants cultured on either Matrigel or laminin (Fig. 4). However, the extent of neurite growth on Matrigel and laminin was significantly greater than on PLL, HSPG, or CSPG (p < 0.001). There were no significant differences in neurite outgrowth from explants cultured on PLL, HSPG, or CSPG (Fig. 4).
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Figure 4. Quantification of the extent of neurite outgrowth from explant cultures on different ECM substrates. The surface area of neurites was measured from the edge of each explant (n = 82). Data were analyzed by one-way ANOVA and Tukey's multiple comparisons. The extent of neurite outgrowth on laminin and Matrigel was significantly greater than on PLL (0.1 µg/ml), CSPG (1 µg/ml), or HSPG (1 µg/ml) (p < 0.001). There were no significant differences between the mean surface area of neurites on PLL, CSPG, or HSPG. The mean area of neurite outgrowth on Matrigel (154 µg/ml) and laminin (10 µg/ml) was also not significantly different. Error bars indicate the SEM. n = 82 is the total number of explants analyzed with between 9 and 17 explants for each experiment.
Effect of ECM on olfactory ensheathing cells
The above results suggested that neurite outgrowth was indirectly modulated by the ECM. It appeared that the ECM was modulating the neurite outgrowth-promoting properties of OECs. To examine the effect of ECM molecules on the spreading of these cells, we prepared dissociated cultures of OECs from the olfactory neuroepithelium. Previous studies have isolated OECs from the outer nerve fiber layer of the olfactory bulb (Chuah and Au, 1993
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Figure 5. Dissociated cultures of OECs isolated from olfactory nerve fascicles. OECs were cultured for 12 d and then stained for p75 (A), GFAP (B), and S-100 (C). A-C, Almost every cell expressed each of these markers. D, E, Phase contrast micrographs of p75 (D) and GFAP (E) demonstrate two cell morphologies. The majority of cells (96%) have spindle-like morphology, whereas the other 4% of cells are flat and triangular in shape (arrows). In addition, there are a small number of unstained flattened cells in the cultures (arrowhead). Scale bars: (in D) A-C, 200 µm; (in E) D, E, 75 µm.
Dissociated OECs were then replated onto coverslips coated with PLL (1 µg/ml), Matrigel (154 µg/ml), laminin (10 µg/ml), HSPG (1 µg/ml), or CSPG (1 µg/ml). After 24 hr, cultures were fixed and stained for p75. Many OECs that were plated on substrates of PLL, HSPG, or CSPG exhibited minimal spreading, and these cells were usually ovoid in shape (Fig. 6A-C, arrowheads). Only approximately half of the cells spread and obtained a spindle shape on these substrates (Figs. 6A-C, 7A, arrows). In contrast, ~95% of all OECs on Matrigel and laminin had spread out and differentiated into spindle-shaped cells (Figs. 6D,E, 7A, arrows). The percentage of spread OECs that adopted a spindle shape on Matrigel and laminin were significantly higher than those grown on PLL, CSPG, or HSPG (p < 0.0004) (Fig. 7A). In addition, there were significantly more spindle-shaped OECs on HSPG than on PLL (p < 0.04). No significant differences were found between the percentage of cells that spread over HSPG compared with CSPG, and PLL compared with CSPG. Furthermore there were no significant differences in the percentage of OECs that spread at any concentration of CSPG, HSPG, or Matrigel (Fig. 7A). In contrast, altering the concentration of laminin affected the spreading of OECs. Approximately 95% of cells spread as spindle-shaped cells when 10 and 100 µg/ml of laminin were used, whereas on laminin at 1 µg/ml, only 76.3% of cells exhibited this spindle shape (Fig. 7A). Although a different concentration of Matrigel substrates did not significantly affect the percentage of spread OECs, it did appear to change their morphology. OECs on high concentrations of Matrigel were more stellate, whereas on lower concentrations, the cells were more spindle-shaped.
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Figure 6. Dissociated cultures of OECs on different ECM substrates. Cells were cultured for 24 hr and immunostained for p75. When OECs were grown on PLL (A) (0.1 µg/ml), CSPG (B) (1 µg/ml), and HSPG (C) (1 µg/ml), there was minimal cell spreading. On these substrates, OECs were either ovoid-shaped (arrowhead) or small spindle-shaped (arrows) cells. When ensheathing cells were plated on to Matrigel (D) (154 µg/ml) and laminin (E) (10 µg/ml), there was extensive cell spreading. Most cells spread in large spindle-shaped cells with long tapering processes that curved across the substrate (arrows). Scale bar (in E): A-E, 100 µm.
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Figure 7. A, Quantification of cell spreading on different substrates. OECs were grown on coverslips coated with PLL (0.1 µg/ml), CSPG (0.1, 1, and 10 µg/ml), HSPG (0.1, 1, and 10 µg/ml), Matrigel (15.4, 154, and 1540 µg/ml), and laminin (1, 10, and 100 µg/ml). After 24 hr, cells were fixed and stained for p75, and the mean percentage of ensheathing cells that spread, as spindle-shaped cells, was determined. Data were collected from nine independent samples and statistically analyzed by the Kruskal-Wallis and Mann-Whitney tests. The mean percentage of cells that spread on laminin and Matrigel was significantly different compared with PLL, CSPG, and HSPG (p < 0.0004). In addition, the mean percentage of cells that spread on HSPG was greater than on PLL (p < 0.04). There were no significant differences in the mean percentage of cells that spread on CSPG compared with HSPG, or PLL compared with CSPG. There were no significant differences in the percentage of ensheathing cells that spread on substrates of CSPG, HSPG, or Matrigel at any concentration used. However, the percentage of cells that spread on laminin at 1 µg/ml was significantly less than on laminin at concentrations of 10 µg/ml (p < 0.0008) and 100 µg/ml (p < 0.0011). Error bars indicate SEM. B, Quantification of the length of processes from olfactory ensheathing cells cultured on different substrates. OECs were grown on PLL (1 µg/ml), Matrigel (154 µg/ml), laminin (10 µg/ml), HSPG (1 µg/ml), or CSPG (1 µg/ml) for 24 hr. The length of processes from 20 random cells from each substrate was then measured and expressed as total length of process per cell. This experiment was performed in triplicate. Data were then averaged and analyzed by one-way ANOVA and Tukey's multiple comparisons. The total length of processes per cell was significantly greater on Matrigel and laminin compared with PLL, CSPG, or HSPG (p < 0.001). There were no significant differences between the total length of processes of cells cultured on PLL, CSPG, or HSPG. The total length of processes of cells on Matrigel was not significantly different from those on laminin. Error bars indicate SEM.
In addition to the low percentage of OECs that spread on PLL, HSPG, and CSPG, the length of spread processes were also considerably reduced. Spread cells on these substrates usually had one long process and one to two shorter processes that were straight and unbranched (Fig. 6A-C, arrows). In contrast, OECs on both Matrigel and laminin grew long thin processes, which were curved (Fig. 6D,E). The total length of processes per OEC was significantly longer on Matrigel and laminin compared with PLL, HSPG, or CSPG (p < 0.001) (Fig. 7B). There were no significant differences between the length of cell processes on PLL, CSPG, and HSPG or between Matrigel and laminin.
DISCUSSION
The growth cones of primary olfactory axons migrate toward the olfactory bulb over the surface of OECs, which are embedded in an ECM rich in laminin, HSPG, and collagen IV. These axons and cells are confined to a discrete pathway demarcated by the expression of CSPG and fibronectin in the surrounding mesenchyme (Treloar et al., 1996
ECM modulates the growth of olfactory ensheathing cells
We isolated ensheathing cells from fascicles of the olfactory nerve teased from the submucosa of the neuroepithelium lining the nasal septum. Almost every cell in these cultures expressed p75, GFAP, and S-100, which are phenotypic markers of OECs (Pixley, 1992
Schwann cells, like OECs, are also influenced by the nature of the ECM. Schwann cells transfected with Syndecan-1, a cell surface HSPG, adopt a flat cuboid cell shape rather than the typical spindle-shaped morphology (Carey et al., 1994
Cell spreading is an important prerequisite for cell migration and differentiation and is mediated by many cells via molecular interactions with the ECM, which lead to the formation of focal adhesions (Ridyard and Sanders, 1999
ECM molecules and neurite outgrowth from olfactory neuroepithelium
We demonstrated that substrates of Matrigel and laminin promoted the extension of neurites from explants of olfactory neuroepithelium when compared with PLL, CSPGs, and HSPGs. Laminin has been shown previously to directly promote the growth of olfactory neurites in vitro (Whitesides and LaMantia, 1996
Previous studies have demonstrated that OECs promote axon growth. OECs promote the extension of olfactory neurites in vitro (Goodman et al., 1993
Model of axon growth between the nasal cavity and olfactory bulb
We have shown previously that laminin and CSPGs have highly restricted patterns of expression in the frontonasal mesenchyme between the nasal cavity and olfactory bulb (Treloar et al., 1996
FOOTNOTES Received June 11, 1999; revised Aug. 20, 1999; accepted Aug. 27, 1999.
This work was supported by National Health and Medical Research Council grants. K.T.T. was supported by an Australian Postgraduate Award and a Queen's Trust Young Achiever Award.
Correspondence should be addressed to Brian Key, Neurodevelopment Laboratory, Department of Anatomical Sciences, University of Queensland, Brisbane 4072, Australia. E-mail: brian.key{at}mailbox.uq.edu.au.
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