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Address correspondence to Shuh Narumiya, Dept. of Pharmacology, Kyoto University Faculty of Medicine, Yoshida, Sakyo-ku, Kyoto 606-8315, Japan. Tel.: 81-75-753-4392. Fax: 81-75-753-4693. E-mail: snaru{at}mfour.med.kyoto-u.ac.jp
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Abstract |
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Key Words: mDia; Rho; axon elongation; cerebellar granule neuron; SDF-1
* Abbreviations used in this paper: CRIB, Cdc42/Rac interactive binding; CNS, central nervous system; DA, dominant-active; DN, dominant-negative; EGFP, enhanced GFP; EGL, external granule cell layer; IGL, internal granule cell layer; mDia, mammalian homologue of the Drosophila gene Diaphanous; P, postnatal day; PAK, p21-associated kinase; RBD, Rho-binding domain; RNAi, RNA interference; siRNA, short interfering double stranded RNA oligomer; SDF, stromal cellderived factor.
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Introduction |
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A dynamic morphological alteration is initiated during the acquisition of neuronal polarity and must continue until the completion of synaptogenesis. Recent findings indicate a critical role for the antagonism between Rac and RhoGTPases in these events (Narumiya et al., 1997; Hall, 1998; Luo, 2000; Dickson, 2001). A large body of work has now established that several soluble or transmembranous guidance molecule systems can exhibit either chemorepulsion or chemoattraction toward axonal growth cones, at least in part, via coupling to either Rho or Rac, respectively. Such systems include EphrinA (Shamah et al., 2001), EphB reverse signaling (Lu et al., 2001), Sema4D/PlexinB (Driessens et al., 2001; Swiercz et al., 2002), Sema3A/PlexinA-Neuropilin (Jin and Strittmatter, 1997; Liu and Strittmatter, 2001; Jurney et al., 2002), Netrin/DCC (Li et al., 2002), Slit/Robo (Wong et al., 2001), and neurotrophins/p75/trk (Yamashita et al., 1999; Huang and Reichardt, 2001; Ozdinler and Erzurumlu, 2001; Nusser et al., 2002). Thus, antagonistic interactions and hierarchical cascades between distinct small GTPases had been considered as most likely ways by which distinct gradient cues could be decoded into reliable maps of afferents projecting into one specific area of the central nervous system (CNS).*
However, to date, a clear understanding regarding what specific effectors of the small GTPases contribute to each of these opposing signaling events is still missing. Furthermore, whether Rho always antagonized with Rac remains controversial (Sebok et al., 1999; Bashaw et al., 2001).
The rodent cerebellar granule cells represent a highly advantageous resource to study in detail the molecular sequence of events controlling axonogenesis, neuronal migration, dendritogenesis, and synaptogenesis. Indeed, each of these steps that is critical for neuronal maturation and circuit formation occurs in an organized and sequential fashion in the cerebellum during the postnatal 3 wk after birth (Altman and Bayer, 1996; Hatten, 1999). Many of these steps involve dramatic changes in neuronal morphology, yet previous studies indicated that many of their features could be recapitulated, at least in part, in primary culture (Powell et al., 1997; Bito et al., 2000; Yamasaki et al., 2001; Yacubova and Komuro, 2002).
Previous investigation of molecular determinants involved in axon formation in cerebellar granule cells, from our laboratory and others, have begun to uncover the critical importance of piagranule cell interaction (Bhatt et al., 2000) on one hand and control of actin dynamics on the other (Bito et al., 2000; Yamasaki et al., 2001). Thus, we considered the possibility that a factor supplied by the pia mater may be involved in the signaling pathway controlling axon initiation and elongation. One candidate factor we tested was stromal cellderived factor (SDF)-1, a chemokine heavily expressed in the pia mater and chemoattractant for migration of cerebellar granule cells (Lu et al., 2001; Klein et al., 2001; Tham et al., 2001; Zhu et al., 2002). Our interest was prompted by the striking phenotype of the knockout mice lacking either SDF-1
(Ma et al., 1998) or its cognate receptor CXCR4 (Ma et al., 1998; Zou et al., 1998). In both lines of mice, the formation of the cerebellar granule cell layers was abolished. This suggested that early events in cerebellar granule cell morphogenesis, such as axon initiation, axon elongation, or migration of the cell body, might be severely perturbed in the absence of SDF-1
signaling.
However, whether SDF-1 could stimulate axon formation via direct control of actin cytoskeletal signaling mechanisms in cerebellar granule cells has not been demonstrated. Here we show that SDF-1
activates Rho but not Rac small GTPase in cerebellar granule cells. A low concentration (100 ng/ml) of SDF-1
induced significant amount of axon outgrowth in a C3 exoenzymesensitive fashion. In contrast, at a higher concentration SDF-1
rather repressed axon formation in a Rho-dependent manner. However, Y-27632 treatment was sufficient to uncover an axon elongating activity even under high dose of SDF-1
. Thus, SDF-1
stimulated two distinct opposing Rho effectors: a novel Rho effector, which promoted axon elongation, and ROCK to inhibit axonogenesis. The facilitatory effect of SDF-1
in the presence of Y-27632 could be mimicked by overexpressing a dominant-active (DA) form of the mammalian homologue of the Drosophila gene Diaphanous (mDia)1, a Rho effector involved in control of actin polymerization during cell polarization and directed cell growth. This dominant activation of mDia was dependent on intact Rac activity. Furthermore, the axon outgrowth induced by SDF-1
could be antagonized either by overexpression of a dominant interfering mutant or by RNAi knockdown of mDia1. Thus, we identify a novel function for mDia1 as a critical Rho effectormediating SDF-1
dependent axon elongation in concert with Rac.
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Results |
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Rho/mDia pathway mediates SDF-1stimulated axon elongation in cerebellar granule neurons in part via a coordination with a Rac-dependent pathway
We next examined the contribution of endogenous mDia1 on SDF-1stimulated axon elongation by use of a dominant-negative (DN) form of mDia1, mDia1-
N3(HindIII) (Fig. 4 A; Tsuji et al., 2002). This mutant was able to abolish the effect of DA-mDia1 on axon length (Fig. 7 A). DN-mDia1 also inhibited axon numbers back to baseline levels (Fig. 7 A); however, since DA-mDia1 had little effect per se (Fig. 6 D), we currently favor the simplest view that rather than acting on the axonogenesis itself, mDia's axon elongating activity may be required in order to visualize even the smallest process. Consistently, when this DN mutant was transfected in neurons stimulated with SDF-1
in the presence of Y-27632, both axon number and axon length were significantly diminished (Fig. 7, B and C). Together, these results support the notion that axon elongation induced by SDF-1
may be regulated in an mDia-dependent manner.
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Together, our data establish a critical role for the Rho/mDia1 pathway in mediating axon elongation in SDF-1stimulated cerebellar granule neurons, presumably in concert with Rac activity (Fig. 10).
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Discussion |
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In this study, we have formally demonstrated that Rho may in fact mediate both stimulation and inhibition of axon outgrowth downstream of the same ligand SDF-1 in the context of early postnatal cerebellar granule cells. Although a classically recognized Rho/ROCK pathway repressed axon formation, a Rho/mDia pathway was identified which rather potently facilitated axon elongation. How ROCK can dominantly antagonize the expression of the axon elongation machinery, while another Rho effector mDia is facilitating this event, is currently being investigated. One possibility that is consistent with our finding is that ROCK and mDia1 may locally respond to different levels of GTP-bound Rho. Our finding of a multiplicity in Rho-mediated sites of action is reminiscent of the recent findings suggesting that Rac also acts on multiple steps of axon outgrowth during Drosophila development (Ng et al., 2002).
How then does mDia, an adaptor protein containing multiple formin homology domains, exert its effect on axon elongation? A clear picture is still missing, since only a few binding partners of mDia such as profilin (Watanabe et al., 1997), IRSp53 (Fujiwara et al., 2000), or mDia-interacting protein (Satoh and Tominaga, 2002) have been reported. Interestingly, in Saccharomyces cerevisiae the Diaphanous homologue Bni1p was shown to be critically involved in controlling assembly of actin cables required for establishment of cell polarity and directed growth (Ozaki-Kuroda et al., 2001; Pruyne et al., 2002; Sagot et al., 2002). Furthermore, recently a DA mutant of mDia1 was also shown to affect orientation of microtubules in HeLa cells, thus implying that mDia may perhaps spatially coordinate actin polymerization and the stability/rate of assembly of microtubule polymers (Ishizaki et al., 2001; Palazzo et al., 2001).
Intriguingly, in our study Rac activity was shown to be required to support an mDia-based change in neuronal morphology. Indeed, a high amount of basal Rac activity is found in the early postnatal cerebellum (unpublished data). In vivo and in vitro studies examining the consequence of defects in Rac/Pak/Cdk5/p35 signaling have provided numerous lines of evidence in support for a role for Rac-mediated control of cytoskeletal dynamics during axon outgrowth (Luo et al., 1994, 1996; Nikolic et al., 1996, 1998; Kaufmann et al., 1998; Hing et al., 1999; Newsome et al., 2000; Zukerberg et al., 2000; Ng et al., 2002). Since we detected an increase in Rho but not Rac activity upon SDF-1 stimulation, we presume that Rac may play a rather permissive role in mediating the Rho/mDia-dependent events, although we cannot exclude the possibility that mDia may also directly regulate Rac or one of its upstream regulators (Fig. 9; Tsuji et al., 2002).
A critical role for a pial chemokine SDF-1 as a guidance molecule regulating axon outgrowth
Recently, SDF-1 (Tashiro et al., 1993; Nagasawa et al., 1994) has attracted a lot of attention as a prototypical chemokine that acts as a mitogen and participates in positional control of a large variety of highly differentiated cell types. Gene targeting of either the ligand molecule SDF-1
or its receptor CXCR4 resulted in a strikingly similar phenotype in the respective knockout mice, thereby demonstrating a crucial role for SDF-1
/CXCR4 signaling in the development of appropriate cell layer formation in the cerebellum, the hippocampal dentate gyrus, the thymus, the spleen, vascular endothelium, and the intestinal epithelium (Nagasawa et al., 1996; Ma et al., 1998; Tachibana et al., 1998; Zou et al., 1998; Lu et al., 2002). In the cerebellum, absence of SDF-1
/CXCR4 signaling resulted in premature invasion of many proliferating granule cells into the cerebellar anlage, and aberrant onset of migration from the external granule cell layer (EGL) to the internal granule cell layer (IGL) (Ma et al., 1998; Zou et al., 1998). Complementary experiments demonstrated that SDF-1
acted as a chemoattractant for migration of both EGL- and IGL-derived cerebellar granule cells in culture (Klein et al., 2001; Lu et al., 2001; Zhu et al., 2002). Together, these lines of evidence are consistent with the idea that neuronal migration and patterning may heavily involve chemokine and G proteincoupled receptor signaling.
However, it was not known which exact step of neuronal morphogenesis was directly targeted by SDF-1, nor was it clear what intracellular signaling it activated in order to fulfill its role as a neural guidance molecule. Here we found that a large part of the initial morphogenetic and cytoskeletal action of SDF-1
might be specifically mediated by the Rho signaling pathway, independent of its potency as a mitogen, in a pertussis toxin-insensitive manner (unpublished data). Previously, it was suspected that SDF-1
might exhibit its growth promoting or chemotactic effect on neurons via pertussis-sensitive Gi/o heterotrimeric G proteins (Klein et al., 2001) and/or via PLC-mediated activation of intracellular calcium stores (Klein et al., 2001; Lu et al., 2002). The possible contribution of these signaling pathways to the neurite elongation still needs to be properly addressed in our cultured cerebellar granule neurons.
Control of actin dynamics via multiple effectors of small GTPases: potential antagonism and coordination between distinct signaling pathways
Our study demonstrates that the Rho-dependent signaling cascade implicated in the developmental control of neural hardwiring may consist of two apparently opposing streams of signals: an inhibitory pathway mediated by ROCK (Bito et al., 2000) and a facilitatory pathway mediated by mDia1 (this study). Coordination of these two pathways may be suited to sequentially express the unique property of SDF-1 either as a repellant or as an attractant. These findings shed light on the new possibility that Rho- and Rac-dependent pathways may interact not just in an antagonistic but also in a cooperative way in the regulation of the timing and the extent of axon elongation in cultured cerebellar granule cells (Fig. 10). Our study raises the possibility that the stimulation of Rho/mDia-mediated pathway by SDF-1
might provide a modulatory link between the Rho- and Rac-based modes.
Together, these findings underscore the significance of ROCK/mDia antagonism during early CNS development. An appropriate balance and coordination between these two signaling systems may be key to controlling the initial timing and extent of axon outgrowth as a function of the strength of stimuli exhibited by the gradient of external guidance cues such as the pial chemokine SDF-1.
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Materials and methods |
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Materials and reagents
Y-27632, a ROCK inhibitor, was supplied by Dr. Masayoshi Uehata (Mitsubishi Pharma Co., Osaka, Japan). Botulinum C3 exoenzyme was purified as described (Morii and Narumiya, 1995). SDF-1 was purchased from PeproTech EC. GST-Rhotekin RBD and GST-PAK CRIB proteins were prepared as described (Ren et al., 1999; Tsuji et al., 2002). pEGFP-C1 was from CLONTECH Laboratories, Inc. pEGFP-mDia1
N3, pFL-mDia1
N3, pEGFP-mDia1
N3 (HindIII), and pEGFP-N17Rac were as described (Watanabe et al., 1999; Tsuji et al., 2002). All other reagents were of analytical grade unless noted otherwise.
Transient transfection of plasmid cDNA constructs and pharmacological assays
Transfection was performed in the following way as modified from Bito et al. (2000). At the end of cerebellar granule cell preparation, a cell pellet was recovered from a 1,000 rpm, 10-min centrifugation at 4°C and resuspended with 20% FCS/HANKS(-) at densities of 5 x 105 cells. The cell mixture (80 µl) was plated onto 12-mm round Matrigel-coated (Becton Dickinson) coverslips (Assistent) placed in a 24-well plate. Each coverslip had been coated with 80 µl Matrigel, 4 h before use. Cells were allowed to settle down for 30 min at RT and were incubated for 30 min at 37°C in a CO2 incubator after each coverslip was fed with 0.5 ml of Medium A (Earle's MEM supplemented with 10% FCS [Hyclone], 1x B-27 supplement [Invitrogen], insulin [25 mg/L; Sigma-Aldrich], glucose [5 g/L], transferrin [100 mg/L; Calbiochem], and 2 mM glutamine). Then, for each coverslip subjected to transfection 100 µl OptiMEM (Invitrogen) containing a total amount of 1 µg of plasmids (0.5 µg of each plasmid for cotransfection) and 1 µl of Lipofectamine 2000 (Invitrogen) was added drop by drop. The plate was incubated in a CO2 incubator for 3 h and replaced with 0.5 ml of Medium A (same as above) per well. When necessary, either Rho or ROCK activity was inhibited in transfected cells by adding Y-27632 (final concentration 50 µM) or C3 (final concentration 50 µg/ml), respectively. Cells were put back into a CO2 incubator and cultured for another 12 h.
To examine the effect of various pharmacological reagents on various aspects of axon outgrowth, cerebellar granule cells were plated onto 12-mm round Matrigel-coated coverslips placed in a 24-well plate as described above. Cells were allowed to settle down for 30 min at RT. After each coverslip was fed with 0.5 ml of Medium A, they were incubated for another 3.5 h at 37°C in a CO2 incubator and then replaced with Medium A supplemented with either the vehicle or SDF-1 (500 ng/ml), Y-27632 (50 µM), SDF-1
(10, 100, 250, 500, and 1,000 ng/ml) plus Y-27632 (50 µM), SDF-1
(500 ng/ml) plus C3 (50 µg/ml), and indicated concentrations of C3 exoenzyme. The cells were put back into a CO2 incubator and cultured for another 12 h.
Pharmacological assays were performed in transfected cells in a similar way except that the cells were incubated in a CO2 incubator for 3 h after the end of transfection procedure and then replaced with 0.5 ml of Medium A containing similar amounts of drugs as described above.
For transfection, Swiss 3T3 cells were plated on a cover glass at a density of 2 x 104 cells per 22-mm dish and cultured in DME containing 10% FCS for 24 h. The cells were washed with PBS(-) once and incubated with the indicated amounts of pEGFP-C1 or pEGFP-mDia1-N3 mixed with 1 µl of Lipofectamine 2000 for 3 h in 1 ml of OPTI-MEM. The medium was replaced with DME containing 10% FCS, and the cells were cultured for 18 h. The cells were then cultured in serum-free DME for 24 h and treated with 30 µM Y-27632 for the last 30 min. The cells were fixed and stained as described below.
Immunofluorescence microscopy and measurements of axon parameters
Immunocytochemistry and GFP-imaging was performed essentially as described (Bito et al., 1996, 2000) using a LSM 510 system (Carl Zeiss MicroImaging, Inc.). Primary and secondary antibodies were as follows: rabbit polyclonal anti-p140mDia1 antibody (AP50) (Watanabe et al., 1997), anti-FLAG mAb (M2; Eastman Kodak Co.), rat antitubulin mAb (Chemicon), antiß-tubulin mAb (TUB.2.1) (Sigma-Aldrich); anti-GFP monoclonal and polyclonal (Molecular Probes); and Alexa Fluor 488, 594, and 633conjugated goat antirabbit, antirat, and antimouse secondary (Molecular Probes). Alexa Fluor 594, and 633phalloidin (1:1,000; Molecular Probes) were used to stain the F-actin. In all image analyses, no background subtraction was performed, and all pseudocolor representations were assembled using Adobe Photoshop® version 6.0 for illustrative purpose only.
Quantitation of axon length and number was performed on cerebellar granule neurons cultured in the presence of 10% FCS using parameters similar to those described previously (Bito et al., 2000). Axons were distinguished from the filopodia by the presence of microtubules as verified by ß-tubulin staining. As established previously (Bito et al., 2000), ß-tubulin immunoreactivity was missing in virtually all processes with less than 3 µm in length. Because the average axon number was below two (i.e., exact number was usually one or zero) during the experimental time window in most of our assays in this study, we restricted our measurement of axon length to the longer first process. Since an axon was equal or larger than 3 µm in length, its contour could be unambiguously traced from the cell soma up to the very tip of the processes; all turning points within the longest process was defined and the sum of the cumulated distances between these points was considered as axon length. The calculation was performed off-line using the software plug-in of the LSM 510 system. Measurements in transfected neurons were performed identically except that transfected neurons were first identified using an antitag immunostaining (with an anti-GFP or an anti-FLAG antibody) to maximize the probability of detection; when directly compared, FLAG- and GFP-tagged constructs yielded similar results and phenotypes. Statistical analyses were performed using Prism 3.02 (Graphpad Software). All data are indicated as means ± SEM. Unpaired t test with Welch's correction was employed to determine statistical significance and p values below 0.05 was considered as significant.
Videomicroscopy
Cerebellar granule cells labeled with PKH-26 (Sigma-Aldrich) were seeded at a density of 105 per dish in a 35-mm glass-bottom dish (Matsunami Glass) and cultured for 3 h. The dish was transferred to a temperature-controlled CO2 incubator (Carl Zeiss MicroImaging, Inc.) attached to the microscope stage. SDF-1 (100 ng/ml, a final concentration) was then added, and the cell movement was monitored at 37°C in 5% CO2 for 60 min using a confocal laser scanning unit (LSM 510-V2.5; Carl Zeiss MicroImaging, Inc.). One optical section was acquired every 3 min, and the video image were constructed from these sequential images.
Immunohistochemistry
P1 or adult brain was taken out and immediately frozen in TissueTek O.C.T. Compound (Sakura) on dry ice. Cryostat sections of 20-µm width were obtained and subjected to indirect immunofluorescence staining using an anti-p140mDia1 primary (AP50; Watanabe et al., 1997) and Alexa Fluor 488conjugated goat antirabbit secondary antibodies. TO-PRO-3 iodide (Molecular Probes) was used for nuclear staining. Specimens were examined on Axioplan or LSM 510 confocal imaging system (Carl Zeiss MicroImaging, Inc.). Stacked optical sections were merged using Maximum Projection Software (Carl Zeiss MicroImaging, Inc.).
Western blot analysis
Total brain or cerebellar tissues were collected from ICR mice of indicated ages. Thin slices were cut in parasagittal directions in ice-cold HANKS and lysed in the lysis buffer containing 50 mM Tris-HCl, pH 7.5, 150 mM NaCl, 1% NP-40, 0.5% sodium deoxycholate, and 1x Complete (Protease Inhibitor Cocktail Tablets) (Roche Diagnostics). The samples were centrifuged at 100,000 g for 30 min, and the supernatant was collected as the cell lysates. Protein concentration of the lysates was determined by the Lowry method. For Western blot analysis using the total cell lysates, one fifth volume of the 5x Laemmli sample buffer was added to the lysates. The mixtures were boiled for 5 min and subjected to SDS-PAGE and Western blot analysis using anti-p140mDia1 antibody (AP50).
Rho and Rac pull-down assays
Cerebellar granule cells were plated at a density of 5 x 105 cells per 10-cm dish. After treatment with Y-27632, C3 exoenzyme, and/or SDF-1, the cells were washed once with ice-cold HANKS and lysed in the pull-down lysis buffer containing 50 mM Tris-HCl, pH 7.5, 100 mM NaCl, 2 mM MgCl2, 10% glycerol, 1% NP-40, 1x Complete (Roche Diagnostics), 1 mM sodium fluoride, 1 mM EGTA, and 1 mM PMSF. The samples were centrifuged at 12,000 g for 30 min, and the supernatants were saved as the cell lysates. For cerebellar tissue lysates, cerebella were collected from P1 and adult ICR mice, and thin slices were cut in parasagittal directions in ice-cold HANKS and lysed in the pull-down lysis buffer. The tissue lysates were centrifuged at 100,000 g for 30 min, and the supernatant was collected as the cell lysates. 200 µg of cell lysates was incubated with 20 µg GST-Rhotekin RBD or GST-PAK CRIB immobilized on glutathioneSepharose 4B beads (Amersham Biosciences) for 1 h at 4°C. Beads were washed three times with the pull-down buffer, and GTP-bound RhoA and GTP-bound Rac1 were detected by Western blot with an anti-RhoA (Santa Cruz Biotechnology, Inc.) and an anti-Rac1 antibody (Upstate Biotechnology). Protein concentration was determined by the Lowry method.
Protein knockdown of mDia1 by RNAi using siRNA
siRNA corresponding to mDia1 mRNA sequences were designed as recommended with 5'-phosphate, 3'-hydroxyl, and two-base overhangs on each strand; it was chemically synthesized and annealed for duplex siRNA formation by Dharmacon Research, Inc. The following gene-specific sequences were used successfully: si-mDia1 (K2) sense 5'-GCUGGUCAGAGCCAUGGAU-3' and antisense 5'-CGACCAGUCUCGGUACCU-3'. Transfection of mDia1 siRNA for NIH-3T3 cells (104 cells/ml) was performed with Lipofectamine 2000 in 6-well plates. Per well, 2 µl lipofectamine 2000 diluted in 100 µl Opti-MEM was applied to a premix consisting of siRNA (20 µM, 4 µl)/Opti-MEM (100 µl) and incubated for 30 min. The whole mixture was added to the medium, which then was changed to DME 3 h after transfection. Cells were incubated for 2448 h before analysis of knock-down mDia1 by Western blot as described above.
Cotransfection of pEGFP-C1 and siRNA to cerebellar granule cells (5 x 105 cells/ml) were performed with Lipofectamine 2000. Briefly, for 106 cells 2 µl Lipofectamine 2000 diluted in 100 µl Opti-MEM was applied to a pEGFP-C1 (1 µg)/siRNA (20 µM, 8 µl)/Opti-MEM (200 µl) mixture and incubated for 30 min. The entire mixture was then added to the cell-containing medium, which was refed with the original culture medium 3 h after transfection. Cells were incubated for 12 h in solution and then finally plated onto 12-mm round Matrigel-coated coverslips placed in a 24-well plate. After another 12 h of culture on the coverslips, measurements of axon parameters were performed as described above.
Online supplemental material
Video 1, showing facilitation of axon elongation by a 100 ng/ml SDF-1 treatment in cultured cerebellar granule neurons, is available online at http://www.jcb.org/cgi/content/full/jcb.200210149/DC1).
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Acknowledgments |
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This work was supported in part by grants in aid from the Ministry of Education, Culture, Sports, Science and Technology of Japan (to S. Narumiya, K. Kimura, and H. Bito) and grants from PRESTO-Japan Science and Technology Corporation, the Tanabe Medical Frontier Conference, the Cell Science Research Foundation, and Human Frontier Science Program (to H. Bito). T. Furuyashiki is a postdoctoral fellow and Y. Arakawa and S. Takemoto-Kimura are predoctoral fellows from the Japan Society for Promotion of Science.
Submitted: 28 October 2002
Revised: 10 March 2003
Accepted: 10 March 2003
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