Correspondence to Toshio Hirano: hirano{at}molonc.med.osaka-u.ac.jp
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Abbreviations used in this paper: BMMC, bone marrowderived mast cell; Fc
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Introduction |
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FcRI stimulation initiates a signaling cascade that includes activation of tyrosine kinases, such as Syk, Lyn, Fyn, and BTK, and phosphorylation of numerous adaptor proteins (Eiseman and Bolen, 1992; Hata et al., 1998; Nadler et al., 2000; Rivera, 2002; Siraganian et al., 2002). These adapters include the linker for the activation of T cells (LAT), SH2 domaincontaining leukocyte protein of 76 kD (SLP-76), Grb2-associated binder 2 (Gab2), MIST/Clnk, 3BP2, and adhesion- and degranulation-promoting adaptor protein (ADAP) (Hamawy et al., 1997; Cao et al., 1999; Goitsuka et al., 2000; Geng et al., 2001; Gu et al., 2001; Kimura et al., 2001; Sada et al., 2002; Xie et al., 2002).
Gab2 is a member of the Gab family of adaptor proteins and displays sequence similarity with Drosophila DOS, a substrate for Corkscrew, a homologue of SHP2, a mammalian protein tyrosine phosphatase (Hibi and Hirano, 2000; Liu and Rohrschneider, 2002; Gu and Neel, 2003; Nishida and Hirano, 2003). The Gab family adaptor proteins are involved in signal transduction through a variety of cytokine and growth factor receptors including c-kit (Nishida et al., 1999, 2002). These FcRI-associated adaptor proteins regulate the generation of downstream second messengers, such as phosphatidylinositol-3,4,5-trisphosphate and the induction of calcium influx. The deletion of adaptor proteins LAT, SLP-76, or Gab2 results in decreased Fc
RI-mediated mast cell activation (Pivniouk et al., 1999; Saitoh et al., 2000, 2003; Gu et al., 2001; Gonzalez-Espinosa et al., 2003; Kettner et al., 2003). Collectively, these reports indicate that adaptor proteins play important roles in mast cell degranulation.
Recent studies suggest that FcRI-mediated signaling occurs through two distinct adaptor complexes (Nadler and Kinet, 2002; Parravicini et al., 2002; Blank and Rivera, 2004). LAT forms a molecular complex that includes the adapters SLP-76, Grb2, phospholipase C
1, and the guanine nucleotide exchange factor, Vav1. Assembly of the LAT complex requires calcium signaling through PLC
1 and PLC
2. In addition, the calcium response is partially impaired in Lyn-deficient mast cells (Nishizumi and Yamamoto, 1997). On the other hand, the adaptor molecule Gab2 has been shown to be critical for mast cell signaling due to its ability to recruit PI-3 kinase (Gu et al., 2001). Fyn is required for the Fc
RI-induced phosphorylation of Gab2 and mast cell degranulation, but not for calcium signaling (Parravicini et al., 2002). These reports suggest the presence of a calcium-independent pathway in mast cell degranulation, in addition to the well-known calcium-dependent pathway.
The FcRI-mediated signal pathway controls cytoskeletal rearrangements that influence and accompany mast cell degranulation. Two observations underscore the importance of the microtubules in mast cell degranulation. First, tubulin polymerization-inhibiting agents can suppress Fc
RI-induced degranulation (Nielsen and Johansen, 1986; Tasaka et al., 1991; Martin-Verdeaux et al., 2003). Second, Fc
RI-mediated movement of granules is dependent on microtubules in the mast cell line, RBL (Smith et al., 2003). These reports suggested that microtubules play an important role for mast cell degranulation. However, the precise roles and molecular mechanisms of cytoskeletal rearrangements in the degranulation process were not well known.
In this study, we demonstrated that the formation of microtubules is important for FcRI-induced granule translocation to the plasma membrane. Furthermore, we showed that this process is dependent on the Fyn/Gab2/RhoA signaling pathway, but independent of calcium, Lyn, and SLP-76.
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Results |
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Microtubule dynamics are involved in mast cell degranulation
We next demonstrated the need for both microtubule formation and F-actin ring disassembly in FcRI-mediated degranulation using various cytoskeletal inhibitors. First, we tested drugs affecting F-actin, latrunculin B (which disrupts F-actin), and jasplakinolide (which stabilizes F-actin). Latrunculin B treatment induced the disassembly of the F-actin rings (Fig. 3, B and G) and significantly enhanced ß-hexosaminidase release (Fig. 3 K). In contrast, jasplakinolide suppressed F-actin ring disassembly (Fig. 3, C and H) and slightly reduced ß-hexosaminidase release (Fig. 3 L). These results are consistent with the idea that the disassembly of the F-actin ring is required, at least in part, for mast cell degranulation in a calcium-dependent manner.
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FcRI-mediated granule translocation depends on microtubule dynamics, but not calcium
To visualize the granules, we introduced a CD63-GFP fusion protein into BMMCs. Before FcRI stimulation, we observed that CD63-containing granule structures were retained in cytoplasm (Fig. 4 A, left) as reported by Nishikata et al. (1992). After Fc
RI stimulation, the CD63-containing granules were translocated to the plasma membrane (Fig. 4 A, middle; Fig. S1 A, available at http://www.jcb.org/cgi/content/full/jcb.200501111/DC1). Consistent with this, FACS analysis showed the increase of CD63 cell surface expression, indicating that granuleplasma membrane fusion occurred (Fig. 4 B, middle).
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The Fyn/Gab2/RhoA- but not Lyn/SLP-76mediated pathway is required for the FcRI-mediated formation of microtubules and translocation of granules to the plasma membrane
Fyn-deficient BMMCs are defective in degranulation, but they have an intact calcium influx. The degranulation process is known to be associated with phosphorylation of Gab2 in a Fyn-dependent manner (Parravicini et al., 2002). Therefore, we examined the possibility that Fyn/Gab2 signaling is involved in the translocation of granules to the plasma membrane.
Gab2- or Fyn-deficient BMMCs showed a decreased ß-hexosaminidase release (Fig. 5 A). We further confirmed that the FcRI-induced phosphorylation of Gab2 was decreased in Fyn-deficient BMMCs (Fig. 5 B). More importantly, the Fc
RI-induced formation of polymeric tubulin was decreased in Fyn- and Gab2-deficient BMMCs, as shown in Fig. 5 C. Consistent with this, the microtubule formation was impaired in Fyn- or Gab2-deficient BMMCs, but was intact in Lyn- and SLP-76deficient BMMCs (Fig. 5, DM).
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Finally, we showed that there was a decrease in granule translocation in Fyn- and Gab2-deficient BMMCs, whereas granule translocation still occurred in Lyn- and SLP-76deficient BMMCs (Fig. 4 D). Together, all these data indicate that the Fyn/Gab2/RhoA signaling pathway is required for the microtubule-dependent FcRI-induced translocation of granules to the plasma membrane.
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Discussion |
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The presence of a calcium-independent pathway was suggested previously by a study showing that Fyn-deficient BMMCs have an impaired FcRI-induced mast cell degranulation, but an intact calcium influx (Parravicini et al., 2002). Taking this and our findings together, we propose that the mast cell degranulation process can be dissected into two steps: the calcium-independent and microtubule-dependent process and the calcium-dependent one. The former step is involved in the translocation of granules to the plasma membrane, the latter involved in the fusion of granule with the plasma membrane and exocytosis (Fig. 7).
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We found that FcRI stimulation triggers F-actin ring disassembly in a calcium-dependent manner in mast cells, and that disruption of the F-actin cytoskeleton by latrunculin B enhances the Fc
RI-mediated mast cell degranulation. Others have described a similar effect in RBL cells and neuroblastoma cell lines (Frigeri and Apgar, 1999; Holowka et al., 2000; Ohnishi et al., 2001). Together, these data suggest that F-actin disassembly is involved in a mast cell exocytotic step. One explanation is that the removal of cortical F-actin permits granules greater access to the plasma membrane. Alternatively, as shown in chromaffin cells, cortical F-actin may act as a barrier between the reserve and the release-ready secretory vesicle pools (Cheek and Burgoyne, 1986; Vitale et al., 1995). F-actin disassembly may act to disrupt this actin barrier. At present, we do not have conclusive data indicating the precise role of F-actin disassembly in mast cell degranulation.
We demonstrated that FcRI stimulation triggers the formation of microtubules in a calcium-independent manner in mast cells. We observed a rapid increase in the polymeric form of tubulin soon after Fc
RI stimulation and an enhanced rate of polymer formation over the next 15 min. Fc
RI-induced microtubule formation returned to the basal level at 20 min after stimulation. We found that nocodazole, which induces the depolymerization of the microtubule, significantly inhibited the Fc
RI-mediated mast cell degranulation. We obtained similar results with Taxol, a stabilizer of microtubules. These data indicated that a dynamic microtubule network is required for mast cell degranulation.
We observed that granules containing CD63-GFP translocated to the plasma membrane within 10 min after FcRI stimulation. The translocation of CD63-containing granule to the plasma membrane could be induced as a result of granulegranule fusion. However, this is unlikely because (1) the translocation of granule to the plasma membrane is calcium independent; (2) it is considered that the membrane fusion is calcium dependent in general (Lin and Scheller, 2000); and (3) it is reported that granulegranule fusion is calcium dependent, like the fusion of granule with the plasma membrane (Guo et al., 1998). Actually, we observed the translocation of CD63-containing granules to the plasma membrane in the absence of calcium, under the condition that we did not observe Fc
RI-induced increase of cell surface expression of CD63 by FACS analysis. Furthermore, the observed translocation of granules to the plasma membrane was totally dependent on a dynamic microtubule network. These results support the idea that Fc
RI stimulation induces the translocation of granules to the plasma membrane in a manner dependent on microtubule and independent of calcium, although the involvement of granulegranule fusion in a part of the translocation process is not excluded. Anyway, this is consistent with recent studies showing that granules are translocated to the plasma membrane in RBL cells after stimulation (Amano et al., 2001; Smith et al., 2003).
The Fyn/Gab2/RhoA-mediated pathway controls the FcRI-induced polymerization of tubulin and translocation of granules to the plasma membrane
Mast cell degranulation depends on the FcRI-induced formation of a complex consisting of several adaptor molecules and catalytic enzymes, including src family kinases. However, little is known about the molecular mechanism that relays the early Fc
RI-activated signals to cytoskeletal changes that occur subsequently. Our study provides the first direct evidence for a critical role of adaptor proteins such as Gab2 in Fc
RI-dependent microtubule organization. Using Gab2- and Fyn-deficient BMMCs, we showed that the Fyn/Gab2-mediated pathway controlled microtubule formation. We then found that Fc
RI stimulation induced the activation of RhoA and Rac, and that the activation of RhoA was decreased in Gab2-deficient BMMCs. We also found that dominant-negative RhoA, when introduced into mast cells, inhibited Fc
RI-induced microtubule formation and degranulation. Consistent with our findings, another group reported that Rho regulates mast cell secretion (Price et al., 1995; Mariot et al., 1996). These data indicated that the Rho GTPase activity is critical for microtubule organization and degranulation in mast cells. There are two potential effects of Rho on microtubule. One is that Rho activation leads to microtubule stabilization. The other is that Rho activation inactivates a microtubule-destabilizing protein. Some reports have showed that Rho promotes the stabilization of microtubule through its target mDia (Ishizaki et al., 2001; Palazzo et al., 2001). Further biochemical analyses will clarify the mechanisms by which RhoA controls microtubule organization.
In summary, our results in this paper showed that the FcRI-mediated degranulation process can be dissected into two steps: the calcium-independent microtubule-dependent translocation of granules to the membrane, and the calcium-dependent degranulation accompanied with granuleplasma membrane fusion. We further showed that the Fyn/Gab2/RhoA signaling pathway, but not the Lyn/SLP-76-mediated one, plays a critical role in the calcium-independent microtubule-dependent pathway (Fig. 7). These novel results inspire new appreciation for the role of the microtubule cytoskeleton in supporting secretory cell functions such as Fc
RI-mediated degranulation in mast cells, and most likely in cells of other lineages cells as well.
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Materials and methods |
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Antibodies and reagents
Anti-Gab2 antibodies were generated as described previously (Nishida et al., 1999). Anti-Flag (M2) and anti-phosphotyrosine (4G10) antibodies were purchased from Sigma-Aldrich and Upstate Biotechnology, respectively. Latrunculin B, nocodazole, paclitaxel (Taxol), and xestospongin C were purchased from Sigma-Aldrich. Jasplakinolide was purchased from Molecular Probes, Inc.
Primary mast cell cultures and cell lines
BMMCs were selectively grown in RPMI 1640 medium supplemented with IL-3 (supernatant of a mIL-3producing cell line, CHOmIL-3-3-12M; a gift from T. Sudo, Toray Industry, Inc.), 10% FBS, 10 mU/ml penicillin, and 0.1 mg/ml streptomycin for 48 wk. During culture the medium was changed every 34 d, and the cells were transferred to new dishes to separate them from adherent cells. After 5 wk, culture BMMCs were ready for in vitro experiments.
RBL-2H3 cells (a gift from T. Matsuda, University of Hokkaido, Hokkaido, Japan) were maintained in DME supplemented with 10% FBS. cDNAs encoding Flag-RhoA (N19) were provided by Y. Ohba and M. Matsuda (Research Institute for Microbial Diseases, Osaka, Japan). A total of 10 µg linearized Flag-RhoA (N19) cDNA in a pcDNA3 vector was transfected into RBL-2H3 cells by electroporation (950 µF, 250V). Clones were selected with 1 mg/ml of G418 (Nacalai Tesque).
Degranulation assay
The degree of degranulation was determined by measuring the release of ß-hexosaminidase. Cells (106/ml) were preloaded for 6 h with anti-DNP IgE (1 µg/ml, SPE-7) in medium (without IL-3). To measure ß-hexosaminidase release, sensitized cells were stimulated with 100 ng/ml DNP-HSA for 30 min in Tyrode's buffer. Samples were placed on ice and then centrifuged at 1,500 rpm for 5 min. The enzymatic activity of ß-hexosaminidase in supernatants and cell pellets solubilized with 1% Triton X-100 in Tyrode's buffer was measured with p-nitrophenyl N-acetyl-ß-D-glucosaminide (Sigma-Aldrich) in 0.1 M sodium citrate (pH 4.5) for 60 min at 37°C. The reaction was stopped by the addition of 0.2 M glycine (pH 10.7). The release of the product, 4-p-nitrophenol, was detected by absorbance at 405 nm. The extent of degranulation was calculated by dividing the 4-p-nitrophenol absorbance in the supernatant by the sum of the absorbance in the supernatant and detergent-solubilized cell pellet.
Confocal microscopy
Separate aliquots of 5 x 105 cells were each sensitized with 1 µg/ml SPE-7 for 6 h. Cells were pretreated with different reagents: 1 µM latrunculin for 15 min, 10 µg/ml nocodazole for 30 min, 5 µM jasplakinolide for 3 h, and 10 µM paclitaxel for 30 min. Cells were stimulated with 100 ng/ml DNP-HSA for 5 min at 37°C and fixed with 4% PFA for 30 min at 37°C. Cells were centrifuged at 1,500 rpm for 5 min and permeabilized in Perm Buffer (BD Biosciences) containing 1% BSA for 15 min at RT. Cells were washed with 1 ml of PBS () twice and resuspended in 100 µl of PBS () and attached to glass slides using cytospin (Thramo Shandon) at 600 rpm for 6 min. Primary and secondary stainings were performed on the glass slides: anti--tubulin (B5-1-2; Sigma-Aldrich) at a dilution of 1:50, FITC-conjugated antimouse IgG (Molecular Probes, Inc.) at 1:50, Alexa 594conjugated antimouse IgG at a dilution of 1:150, and phalloidin-rhodamine (Molecular Probes, Inc.) at 1:150. Staining was performed for 30 min in the dark; the slides were then washed with PBS () and coverslips were mounted with DAKO mounting solution (DakoCytomation). Confocal microscopy was performed using an LSM510 system in conjunction with an Axiovert200 (Carl Zeiss MicroImaging, Inc.).
Polymeric tubulin assay
After the stimulation the cells were suspended in extraction buffer, which contained the following: 0.1 M Pipes, pH 7.1, 1 mM MgSO4, 1 mM EGTA, 2 M glycerol, 0.1% Triton X-100, and protease inhibitors (10 µg/ml leupeptin, 10 µg/ml aprotinin, 5 µg/ml pepstatin A, and 0.5 mM phenylmethysulfonyl fluoride). After incubation on ice for 15 min, the cell lysates were centrifuged at 15,000 rpm for 15 min and the supernatant (containing 0.1% Triton-soluble tubulin) was placed into another 1.5-ml tube. The remaining pellet was resuspended in lysis buffer (25 mM Tris-HCl, pH 7.4, 0.4 M NaCl, and 0.5% SDS) and boiled for 10 min. The sample was centrifuged for 15,000 rpm for 5 min, and the polymeric tubulin-containing supernatant was collected and placed gently into another 1.5-ml tube. The 0.1% Triton-soluble and -insoluble solutions were subjected to SDS-PAGE and detected by immunoblotting with anti--tubulin antibodies.
Detection of GTP-bound RhoA and Rac1
GTP-bound RhoA and Rac1 were detected by pull-down assays. In brief, the cleared lysates were incubated with GST-Rhotekin RBD fusion protein (a gift from N. Mochizuki, National Cardiovascular Center Research Institute, Osaka, Japan) and 10 µl of glutathione-sepharose (Amersham Biosciences). The GST-Rhotekin RBD/Rho-GTP complex was collected by incubation with glutathione-sepharose beads and separated on an SDS polyacrylamide gel. The GTP-bound RhoA was visualized by immunoblotting with anti-RhoA antibodies (Santa Cruz Biotechnology, Inc.). To measure the Rac1 activity, cell lysates were incubated with GST-PAK CRIB agarose beads (Upstate Biotechnology). GTP-bound Rac precipitated with the beads was subjected to SDS-PAGE and detected by immunoblotting with anti-Rac1 antibody (Upstate Biotechnology).
Measurement of intracellular calcium
BMMCs were sensitized with 1 µg/ml SPE-7 for 12 h and incubated with the calcium-sensitive dye indo 1-AM (Molecular Probes, Inc.) in the presence of F127 and 0.2% FBS at 37°C for 30 min. Cells were washed twice and resuspended in 1 ml Tyrode's buffer containing 1 mM CaCl2. Cells were analyzed for calcium mobilization in BD-LSR (BD Biosciences). Values were plotted as ratio of fluorescence at FL4 (Ca2+-free indo-1) and FL5 (Ca2+-bound indo-1).
Retroviral transfection
Retroviral transfection was performed as previously described (Itoh et al., 2002). The CD63-GFP plasmid (a gift from M. Nakanishi, Nagoya City University, Nagoya, Japan) was inserted into the retroviral vector pMX (a gift from T. Kitamura, University of Tokyo, Tokyo, Japan). This was then used to transfect the 293T-based packaging cell line phoenix (a gift from G. Nolan, Stanford University, Stanford, CA) with Lipofectamine 2000 (Invitrogen) to generate recombinant retroviruses. Bone marrow cells were infected with the retroviruses in the presence of 10 µg/ml polybrene (Sigma-Aldrich) and IL-3.
Online supplemental material
Fig. S1 shows the GFP fluorescence time-lapse recording of antigen-stimulated BMMCs expressing CD63-GFP. Online supplemental material available at http://www.jcb.org/cgi/content/full/jcb.200501111/DC1.
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Acknowledgments |
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This work was supported by grants from the Ministry of Education, Culture, Sports, Science and Technology in Japan.
Submitted: 21 January 2005
Accepted: 1 June 2005
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References |
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