Convergence of {{alpha}}v{beta}3 Integrin- and Macrophage Colony Stimulating Factor-mediated Signals on Phospholipase C{{gamma}} in Prefusion Osteoclasts

doi:10.1083/jcb.152.2.361

Published online 22 January 2001. doi:10.1083/jcb.152.2.361

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© The Rockefeller University Press, 0021-9525/2001/1/361/ $5.00
The Journal of Cell Biology, Volume 152, Number 2, January 22, 2001 361-374

Original Article

Convergence of ${alpha}$ _vß₃ Integrin– and Macrophage Colony Stimulating Factor–mediated Signals on Phospholipase C ${gamma}$ in Prefusion Osteoclasts

Ichiro Nakamura^a, Lorraine Lipfert^a, Gideon A. Rodan^a, and Le T. Duong^a
^a Department of Bone Biology and Osteoporosis Research, Merck Research Laboratories, West Point, Pennsylvania 19486

Correspondence to: Le T. Duong, Department of Bone Biology and Osteoporosis Research, Merck Research Laboratories, West Point, PA 19486. Tel:(215) 652-7574 Fax:(215) 652-4328 E-mail:le_duong{at}merck.com.

Abstract

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
Acknowledgements
References

The macrophage colony stimulating factor (M-CSF) and ${alpha}$ _vß₃integrins play critical roles in osteoclast function. This studyexamines M-CSF– and adhesion-induced signaling in prefusionosteoclasts (pOCs) derived from Src-deficient and wild-typemice. Src-deficient cells attach to but do not spread on vitronectin(Vn)-coated surfaces and, contrary to wild-type cells, theiradhesion does not lead to tyrosine phosphorylation of moleculesactivated by adhesion, including PYK2, p130^Cas, paxillin, andPLC- ${gamma}$ . However, in response to M-CSF, Src^-/- pOCs spread andmigrate on Vn in an ${alpha}$ _vß₃-dependent manner. Involvementof PLC- ${gamma}$ activation is suggested by using a PLC inhibitor, U73122,which blocks both adhesion- and M-CSF–mediated cell spreading.Furthermore, in Src^-/- pOCs M-CSF, together with filamentousactin, causes recruitment of ß₃ integrin and PLC- ${gamma}$ to adhesioncontacts and induces stable association of ß₃ integrinwith PLC- ${gamma}$ , phosphatidylinositol 3-kinase, and PYK2. Moreover,direct interaction of PYK2 and PLC- ${gamma}$ can be induced by eitheradhesion or M-CSF, suggesting that this interaction may enablethe formation of integrin-associated complexes. Furthermore,this study suggests that in pOCs PLC- ${gamma}$ is a common downstreammediator for adhesion and growth factor signals. M-CSF–initiatedsignaling modulates the ${alpha}$ _vß₃ integrin-mediated cytoskeletalreorganization in prefusion osteoclasts in the absence of c-Src,possibly via PLC- ${gamma}$ .

Key Words: ${alpha}$ _vß₃ integrins, osteoclasts, M-CSF, Src kinases, phospholipaseC ${gamma}$

Introduction

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
Acknowledgements
References

Integrins are transmembrane heterodimeric glycoproteins consistingof ${alpha}$ and ß subunits that mediate cell–cell and cell–matrixinteractions. Ligand binding to integrins activates signal transductionpathways which lead to de novo gene expression and cytoskeletalrearrangement associated with cell adhesion, spreading, andmigration (Thomas and Brugge 1997 ; Giancotti and Ruoslahti1999 ). It has been shown that integrins activate multiple signalingpathways including elevation of intracellular Ca²+, lipid turnover,and tyrosine phosphorylation. The proteins which are tyrosinephosphorylated by extracellular matrix (ECM)¹–integrininteractions include the focal adhesion kinases (FAKs) or PYK2/CAKß/RAFTK/CADTK,in certain cell types, p130^Cas, and cytoskeletal molecules suchas paxillin, tensin, and cortactin (Thomas and Brugge 1997 ; Giancotti and Ruoslahti 1999 ; Schlaepfer et al. 1999 ).

Several lines of evidence indicate that integrin-mediated signalssynergize with growth factor responses to produce the structuralchanges associated with cell migration, proliferation, and differentiation(Sastry and Horwitz 1996 ; Giancotti and Ruoslahti 1999 ; Sieg et al. 2000 ). First, many signaling molecules found inintegrin-dependent focal adhesions, such as Src or phosphatidylinositol3-kinase (PI 3-kinase), are also known to associate with tyrosinekinase growth factor receptors (Schwartz and Ingber 1994 ; Yamada and Miyamoto 1995 ). Second, adhesion of most nontransformedcells to ECM is required for cellular responses to growth factorstimulation and, in some instances, directly regulates growthfactor expression (Soldi et al. 1999 ). Third, growth factorsand integrins often reciprocally regulate cellular responsessuch as cell migration (Plopper et al. 1995 ; Filardo et al.1996 ; Sieg et al. 2000 ).

Osteoclasts are macrophage-related multinucleated cells responsiblefor the degradation of mineralized matrix (Suda et al. 1996). Their adhesion to the bone surface induces the cytoskeletalreorganization associated with activation, suggesting that recognitionof bone ECM proteins is an important step in the initiationof osteoclastic bone resorption (Duong and Rodan 1998 ). Althoughosteoclasts express ${alpha}$ ₂ß₁ and ${alpha}$ _vß₁ integrins, theirpredominant integrin is ${alpha}$ _vß₃. Disintegrins, ${alpha}$ _vß₃ blockingantibodies, and RGD peptide mimetics have been shown to inhibitbone resorption in vitro and in vivo. We reported that PYK2and p130^Cas are key effectors in the ${alpha}$ _vß₃ integrin–mediatedsignaling pathways, and their activation requires c-Src in osteoclasts(Duong et al. 1998 ; Lakkakorpi et al. 1999 ). Osteoclastsare also target cells for several cytokines and growth factors,among which macrophage colony stimulating factor (M-CSF) isessential for both osteoclast development and function (Felixet al. 1994 ). A role for M-CSF in osteoclast formation wasfirst identified in the osteopetrotic op/op mice. Subsequentreports showed that mature osteoclasts also contain the M-CSFreceptor, c-fms, which is required for the survival, spreading,and migration of these cells.

The object of this study was to investigate interactions between ${alpha}$ _vß₃ integrin–mediated and M-CSF–dependentsignaling pathways in osteoclasts. We found that Src-deficientprefusion osteoclasts (pOCs) adhered to, but failed to spreadon vitronectin (Vn)-coated surfaces. ${alpha}$ _vß₃ integrin–mediatedsignaling was abolished in these cells since several adhesion-dependentmolecules including PYK2, p130^Cas, PLC- ${gamma}$ , and paxillin were nottyrosine phosphorylated upon attachment to Vn. However, M-CSFinduced cell spreading of Src-deficient pOCs in an integrin-dependentmanner, and an inhibitor of PLC- ${gamma}$ blocked the M-CSF–dependentcell spreading. In addition, we found that in Src-deficientcells, M-CSF initiated the recruitment of ${alpha}$ _vß₃ integrinand PLC- ${gamma}$ to adhesion contacts. M-CSF also induced the associationof ${alpha}$ _vß₃ integrin with several signaling molecules includingPLC- ${gamma}$ , PI 3-kinase, and PYK2 in a Src-independent manner, whichwas blocked by a PLC inhibitor. The interaction between ${alpha}$ _vß₃and these molecules in pOCs seems to depend on the associationof PYK2 and PLC- ${gamma}$ . These data suggest that PLC- ${gamma}$ is an importanteffector of ${alpha}$ _vß₃- and M-CSF–mediated signaling pathwaysinvolved in prefusion osteoclast spreading.

Materials and Methods

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
Acknowledgements
References

Antibodies and Other Reagents
Vn and poly-L-lysine (PL) were from GIBCO BRL and Sigma-Aldrich,respectively. Antibodies to PYK2 (N-19), PLC- ${gamma}$ 1 (1249 and mAbE-12), PLC- ${gamma}$ 2 (Q20 and mAb B-10), phospho–extracellularsignal–regulated kinase (ERK) (E-4), and ERK2 (C-14) werefrom Santa Cruz Biotechnology, Inc. Antibodies to p130^Cas (mAb21), paxillin (mAb 349), PYK2 (mAb 11), and phosphotyrosine(mAb PY20) were from Transduction Labs. Anti–ß₃integrin antibodies (mAb 2C9.G2) were from BD PharMingen. Anti-Akt/PKBand anti–phospho-Akt/PKB antibodies were from New England Biolabs, Inc.Anti–phosphotyrosine antibody (mAb 4G10)was from Upstate Biotechnology. Other conjugated secondary antibodieswere from Jackson ImmunoResearch Laboratories and Amersham Pharmacia Biotech.Glutathione S-transferase (GST) fusion proteins ofPLC- ${gamma}$ 1 were from Santa Cruz Biotechnology, Inc. Collagenase wasfrom Wako Chemicals and dispase from Boehringer. 1 ${alpha}$ ,25-dihydroxyvitaminD₃ (1 ${alpha}$ ,25[OH]₂D₃) was a gift from Dr. M. Uskokovic (Hoffmann-LaRoche,Nutley, NJ). Mouse recombinant M-CSF was from R&D Systems.Wortmannin, LY294002, U73122, and PD98059 were purchased fromCalbiochem. Echistatin and polyclonal anti-ß3 integrinantibodies were generously provided by Drs. W.K. Herber andB. Bednar (Merck Research Laboratories, West Point, PA).

Animals
Balb/C mice were obtained from Taconic Farms. Heterozygote Src^+/-mice were obtained from The Jackson Laboratory and Src^-/- micewere phenotypically distinguished from their Src^+/? siblingsby lack of tooth eruption. All animals were cared and housedunder conditions approved by the Institutional Animal Care andUse Committee Guide.

Cell Cultures
Prefusion osteoclast-like cells (pOCs) and multinucleated osteoclast-likecells (OCLs) were prepared as described previously with slightmodifications (Duong et al. 1998 ). In brief, spleen cells isolatedfrom 2–3-wk-old Src^-/- or their normal littermates werecocultured with osteoblastic MB1.8 cells for 5–6 d inthe presence of 10 nM 1 ${alpha}$ ,25(OH)₂D₃. pOCs were released from disheswith 10 mM EDTA after removing MB1.8 cells with collagenase-dispase.Alternatively, cocultures were kept for 7–8 d to achieveOCLs and purified as described previously (Duong et al. 1998).

Cell Adhesion
After isolation, pOCs (3 x 10⁵ cells/condition) were washedtwice with serum-free ${alpha}$ -MEM containing 0.1% BSA (Sigma-Aldrich)and kept in suspension or allowed to attach to polystyrene dishescoated with Vn (20 µg/ml) or PL (50 µg/ml). After5–60 min at 37°C, an equal volume of 2x TNE lysisbuffer (20 mM Tris, pH 7.8, 300 mM NaCl, 2 mM EDTA, 2% NP-40,2 mM NaVO₃, 20 mM NaF, 20 µg/ml leupeptin, 1 TIU/ml aprotinin,and 2 mM PMSF) was added to the plates. For coimmunoprecipitation,1.5 x 10⁶ cells/condition and 1x TNE lysis buffer with 10% glycerol(10 nM Tris, pH 7.8, 300 mM NaCl, 1 mM EDTA, 1% NP-40, 1 mMNaVO₃, 10 mM NaF, 10 µg/ml leupeptin, 0.5 TIU/ml aprotinin,and 1 mM PMSF) were used. In some experiments, pOCs were reculturedfor 12 h with 1 ${alpha}$ .25(OH)₂D₃-pretreated osteoblastic MB1.8 cellsto form multinucleated OCLs, which were subsequently purifiedby removing MB1.8 cells using collagenase/dispase, as described.Clarified lysates were subjected to immunoprecipitation andimmunoblotting. Alternatively, cells were fixed and stainedfor tartrate resistant acid phosphatase (TRAP), a marker enzymeof osteoclasts (Nakamura et al. 1999 ). To quantify cell area,the periphery of each cell was outlined and the total planararea was calculated using an image analysis system (Empire ImagingAnalyzing Systems).

Immunoblotting and Immunoprecipitation
Immunoprecipitation and immunoblotting were performed as describedpreviously (Duong et al. 1998 ). In brief, lysates were precipitatedwith anti-PYK2, p130^Cas, paxillin, PLC- ${gamma}$ 1, PLC- ${gamma}$ 2, or integrinß₃ antibodies (2 µg) for 2 h at 4°C, followedby protein G–Sepharose for 1 h at 4°C. After washingfour times with lysis buffer, proteins were separated on an8% SDS-PAGE and blotted onto Immobilon-P membrane. After blockingwith 100 mM NaCl, 10 mM Tris, 0.1% Tween-20, and 2% BSA, themembrane was incubated with primary antibodies, followed byHRP-conjugated secondary antibodies and detected with the ECLchemiluminescence system (Amersham Pharmacia Biotech). Levelsof proteins in immunoblots were quantitated using an ImagingDensitometer (model GS-700, BioRad) and specific activity oftyrosine phosphorylated proteins at various time points wereestimated from the ratio of phosphorylated proteins to its proteincontent, and expressed relative to controls at time 0.

In Vitro Protein Association Assays
These experiments were performed with GST fusion proteins containingthe Src homology (SH) 3 domain, SH2 domains, both SH2 domains,and SH3 domain of PLC- ${gamma}$ 1. Multinucleated osteoclast-like celllysates (1 mg/ml) were incubated with GST fusion protein coupledwith glutathione-Sepharose beads for 2 h at 4°C. The beadswere washed three times with lysis buffer and one time withPBS, and precipitated proteins were separated by SDS-PAGE andsubjected to immunoblot analysis using anti-PYK2 antibodiesas described above.

Immunofluorescence
Src-deficient pOCs were cultured for 1 h on glass coverslips.After cells were treated with 5 nM M-CSF for another 30 min,cells were fixed with 4% paraformaldehyde, permeabilized with0.5% Triton X-100 in PBS, and incubated for 30 min at 37°Cwith polyclonal anti–ß₃ integrin (Nakamura et al.1999 ) and monoclonal anti–PLC- ${gamma}$ 1 or anti–PLC- ${gamma}$ 2 antibodies.Cells were washed with PBS and incubated for 30 min at 37°Cwith TRITC-conjugated donkey anti–rabbit IgG and FITCgoat anti–mouse IgG. Samples were viewed with a LeicaTCS SP Spectral confocal laser scanning microscope equippedwith Argon-Krypton laser (Leica Microsystems).

Cell Migration
Migration assay was performed as described by Nakamura et al.1999 , in which Src^+/? or Src^-/- pOCs were cultured on Vn-coateddishes in medium 199 (25 mM Hepes, 4 mM HCO₃^-, supplementedwith 0.1% FBS), covered with paraffin oil, and maintained at35°C using a stage heater. Osteoclasts were observed usingan inverted phase–contrast microscope coupled to a videocamera and time-lapse video recorder (one frame per 2 s). UsingM-CSF as a chemotactic stimulus, osteoclast migration was monitored.A micropipette containing M-CSF (1 nM) was positioned 200–400µm from the cells and contents were delivered by a syringepump at the rate of 4 µl/h (Harvard Apparatus). Osteoclastresponses were recorded for 4 h by time-lapse video microscopy.Images of pOCs were digitized using an analysis system (EmpireImaging Systems) and migration was quantified as the net movementof the cell centroid during a culture period of 4 h.

Results

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
Acknowledgements
References

M-CSF Induces Cell Spreading and Migration of Src^-/- Osteoclasts in an ${alpha}$ _vß₃ Integrin–dependent Manner
Fibroblasts from Src-deficient mice were shown to have a reducedrate of spreading on fibronectin (Kaplan et al. 1995 ). We foundthat the pOCs derived from Src^-/- mice exhibit a profound defectin cell spreading on Vn-coated surfaces (Fig 1). Wild-type pOCsfully spread within 60 min of plating (Fig 1, left), whereasSrc^-/- pOCs remained rounded at 60 min (Fig 1, right), and upto 120 min (data not shown). Spreading area of wild-type andSrc-deficient pOC on Vn were quantitated and are shown in Fig 1I. Initial attachment to Vn appeared to be normal in Src^-/-pOCs; however, these cells were easily detached by shaking andtapping, indicating that the firm adhesion associated with cellspreading did not occur, although the expression level of ${alpha}$ _vß₃integrins and their binding affinity were not altered in Src^-/-pOCs (Lakkakorpi et al. 2000 ). The highest number of Src^-/-pOCs attached to Vn-coated dishes was observed 60 min afterseeding.

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Figure 1. Src^-/- pOCs do not spread on Vn-coated dishes. Src^+/? (A, C, E, and G) and Src^-/- (B, D, F, and H) pOCs were plated on Vn (20 µg/ml). After culture for 5 (A and B), 15 (C and D), 30 (E and F), and 60 (G and H) min, cells were fixed and photographed. (I) To quantify cell area, the periphery of each cell was outlined and the total planar area was calculated, using an image analysis system (Empire Imaging Systems). Data are expressed as the means of ± SEM of >50 cells.

It has been shown that the M-CSF receptor, c-Fms, is expressedin mature osteoclasts and that M-CSF induces cell spreadingand cell migration in rat primary osteoclasts and murine osteoclast-likecells (Felix et al. 1994 ). To determine whether c-Src functionis required for M-CSF–induced cytoskeletal reorganizationduring cell spreading and migration, Src-deficient and wild-typepOCs were plated on Vn-coated dishes and treated with M-CSF.To obtain optimal numbers of attached cells, we first allowedSrc^-/- cells to adhere to Vn-coated surfaces for 60 min priorto M-CSF addition. Although Src^-/- pOCs did not spread spontaneouslyon Vn, M-CSF rapidly induced Src^-/- cell spreading (Fig 2 Aand 3, first and second bars). Moreover, M-CSF induced the formationof small punctate adhesion contacts in Src^-/- pOCs, similarto podosomal adhesion structures found in wild-type cells (Fig 3B). Because a previous study found that 2.5 nM M-CSF did notinduce cell spreading of nonpurified primary Src-deficient osteoclasts(Insogna et al. 1997 ), we examined cell spreading of wild-typeand Src^-/- pOCs at 0, 2.5 and 5.0 nM M-CSF (n = 50), to ruleout a dose effect phenomenon. The cell area of untreated wild-typecells was 234 ± 41 µm² and of Src^-/- pOCs, 93 ±15 µm². M-CSF at 2.5 nM increased the cell area in wild-typeto 279 ± 16 µm² (119%) and in Src^-/- pOC to 203± 22 µm² (218%), respectively; while 5 nM M-CSFincreased cell spreading area to 318 ± 25 µm² (135%)in wild-type and 270 ± 27 µm² (290%) in Src^-/-pOC, respectively; i.e. at both doses, there was a pronouncedeffect on the spreading of Src^-/- pOCs, and not of wild-typepOCs.

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Figure 2. M-CSF induces cell spreading of Src^-/- pOCs on Vn-coated dishes. (A) Src^-/- pOCs were plated on Vn-coated dishes in the absence of serum for 60 min, cells were then treated with 5 nM M-CSF for 0 (a), 2 (b), 5 (c), 15 (d), and 30 (e) min, without or with (f) 100 nM wortmannin. (B) Src^+/? (a) and Src^-/- (b and c) pOCs were plated on Vn for 60 min, untreated (a and b) or treated with 5 nM M-CSF treatment for additional 30 min (c). Cells were fixed and stained with rhodamine-conjugated phalloidin. Bars: (A) 10 µm; (B) 5 µm.

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Figure 3. M-CSF–induced cell spreading of Src^-/- pOCs is dependent on ${alpha}$ _vß₃ integrin. Src^-/- pOCs were plated on Vn or PL in serum-free condition. After 60 min, cells were treated with 5 nM M-CSF for 30 min in the absence or presence of echistatin (1 nM). Cells were fixed and stained for TRAP activity, followed by quantitating cell area as described above. Data are presented as means ± SEM and n = 50 cells per group.

Furthermore, M-CSF–stimulated osteoclast chemotaxis ofSrc-deficient cells was not different from wild-type cells (Fig 4).In control cultures 15 out of 26 (58%) Src^+/? pOCs migratedtowards the source of M-CSF, and the net migration distanceover a 4-h period was 25.5 ± 2.0 µm (means ±SEM). Similarly, 10 out of 19 (53%) Src^-/- pOCs showed chemotacticmigration, and the net distance was 24.5 ± 2.9 µm,not significantly different from wild-type. These observationssuggest that Src function is not required for the M-CSF–inducedcytoskeletal reorganization required for osteoclast spreadingand migration.

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Figure 4. M-CSF induces cell migration of Src^-/- pOCs as well as wild-type cells. The motility of Src^+/? and Src^-/- pOCs was monitored using time-lapse video microscopy, as described in Materials and Methods. M-CSF (1 nM) was supplied through a micropipette to induce chemotaxis. Cells were observed using an inverted phase–contrast microscope coupled to a video camera and time-lapse video recorder. Images of cells were digitized using a computer-based image analysis system. Migration activity (net translocation of the cell center over a period of 4 h) was quantified (filled circles). 15 out of 26 (58%) Src^+/? cells and 10 out of 19 (53%) Src^-/- cells migrated towards the source of M-CSF. Means ± SEM (open circles) of migrating distance of wild-type and Src^-/- cells are shown.

To further examine the role of ${alpha}$ _vß₃ integrin in M-CSF–inducedSrc^-/- pOC spreading, cells were plated on Vn- or PL-coateddishes in the presence of M-CSF under serum-free conditions.As shown in Fig 3M-CSF–induced cell spreading of Src^-/-pOCs only when cells were plated on Vn, but not on PL. It shouldbe noted that wild-type pOCs plated on PL do not spread eitherin the absence or presence of M-CSF (data not shown). Moreover,M-CSF–induced Src-deficient pOC cell spreading on Vn wasblocked by the RGD-containing disintegrin, echistatin (Fig 3)which was previously demonstrated to have high binding affinityfor ${alpha}$ _vß₃ and to inhibit ${alpha}$ _vß₃-mediated spreading, migration,and sealing zone formation in osteoclasts (Nakamura et al. 1999). This finding suggested that in the absence of c-Src, M-CSF-initiatedcytoskeletal rearrangement to during cell spreading and migrationstill depends on ligand engagement of ${alpha}$ _vß₃ integrins. Wehad previously shown that tyrosine phosphorylation of PYK2 andp130^Cas, ${alpha}$ _vß₃-associated downstream signaling molecules,is significantly diminished in Src-deficient OCLs (Duong etal. 1998 ; Lakkakorpi et al. 1999 ). We therefore searchedfor potential downstream participants, which could modulatethe synergistic action of the adhesion- and M-CSF-mediated cytoskeletalreorganization in Src-deficient pOCs and evaluated include PI3-kinase and PLC.

Inhibitors of PLC and PI 3-Kinase Block Adhesion- and M-CSF–induced Cell Spreading of Src-deficient Osteoclasts
We examined the involvement of PI 3-kinase and PLC- ${gamma}$ in M-CSF–mediatedsignaling in Src-deficient cells using either wortmannin (0.1µM) or U73122 (1 µM). As shown in Fig 5 A (bars5–7) and Fig 2 F, either inhibitor blocked M-CSF–inducedcell spreading in Src^-/- pOCs. Both inhibitors also blockedthe migration of wild-type and Src-deficient cells assessedby time-lapse video microscopy (data not shown). Similarly,cell spreading of wild-type pOCs upon adhering to Vn was alsoinhibited by wortmannin (data not shown) and U73122 (Fig 5 A,bars 1 and 2). Although U73122 is widely used as a PLC inhibitor,it has been shown to interfere with non PLC-dependent signals,usually at higher concentrations (>10 µM) (Walker et al.1998 ). Nevertheless, our pharmacological findings suggest thatPI 3-kinase and PLC- ${gamma}$ may take part in both adhesion-dependentand M-CSF–mediated signaling, which leads to cytoskeletalorganization in prefusion osteoclasts.

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Figure 5. PLC and PI 3-kinase inhibitors block adhesion-induced and M-CSF–induced cell spreading of prefusion osteoclast-like cells. (A) Src^+/? pOCs (1, 2, and 4) and Src^-/- pOCs (3 and 5–8) were plated on Vn under serum-free condition. After 60 min, cells were treated with (4–8) or without (1–3) M-CSF for 30 min. U73122 (2 and 6), wortmannin (7), or PD98059 (8) was preincubated for 40 min before M-CSF was added. Cells were fixed, stained for TRAP, and the total planar area was calculated as described in Materials and Methods. Data are presented as means ± SEM; n = 50 cells per group. (B) Src^+/? and Src^-/- pOCs were kept in suspension or plated on Vn for 60 min in the absence of serum, followed by the treatment with 5 nM M-CSF for indicated periods with or without 10 µM PD98059. Lysates were blotted with anti–phospho-ERK (top), followed by anti-ERK and anti-Src (bottom). Susp., suspension; Att., attachment.

Interestingly, PD98059, a mitogen-activated protein (MAP) kinasekinase inhibitor, had little effect on the spreading of Src^-/-pOCs (Fig 5 A, bars 5 and 8), although activation of ERK1 and2 were induced by attachment to Vn-coated surface and by M-CSFtreatment in wild-type pOCs using phospho-ERK–specificantibodies (Fig 5 B, right). However, these kinases were notactivated by either pathway in Src^-/- pOCs (Fig 5 B, left).These findings suggest that adhesion- and M-CSF–dependentactivation of the MAP kinases require c-Src in pOCs. However,in Src-deficient prefusion osteoclasts their activation didnot correlate with M-CSF–induced cytoskeletal rearrangement.

Adhesion-mediated Protein Tyrosine Phosphorylation Is Impaired in Src-deficient Osteoclasts
Initial events triggered by integrin engagement of ECM ligandsinclude recruitment and phosphorylation of numerous signalingand cytoskeletal molecules, leading to cytoskeletal reorganization.We previously reported on the role of PYK2 and p130^Cas in the ${alpha}$ _vß₃ integrin–mediated signaling pathways (Duonget al. 1998 ; Lakkakorpi et al. 1999 ) and on the involvementof PI 3-kinase in osteoclast adhesion and spreading (Lakkakorpiet al. 1997 ). Since U73122 blocked the adhesion- and M-CSF–dependentcell spreading of pOCs, we examined the tyrosine phosphorylationlevels of PLC- ${gamma}$ 1 and 2 in pOCs upon adhesion to Vn. Src^+/? orSrc^-/- pOCs were either left in suspension or plated on Vn-coateddishes. Cell lysates were analyzed by Western blotting withantiphosphotyrosine antibodies after immunoprecipitation. Inwild-type cells, PYK2, p130^Cas, paxillin, and both PLC- ${gamma}$ 1 and2 became tyrosine phosphorylated paralleling the time courseof cell spreading, i.e., peaking at 30 min after plating (Fig 6A). These data indicate that PLC- ${gamma}$ 1 and 2 are downstream effectorsof the integrin-mediated signaling pathway. Furthermore, tyrosinephosphorylation of these molecules after cell adhesion was absentin Src^-/- pOCs (Fig 6 B), supporting the morphological observationsshown in Fig 1. The data thus implicated Src tyrosine kinaseas playing an essential role in osteoclast function by mediatingintegrin-dependent signaling triggered by ligand engagement.

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Figure 6. Adhesion-induced tyrosine phosphorylation of PYK2, Cas, paxillin, and PLC- ${gamma}$ in Src^+/? and Src^-/- prefusion osteoclast-like cells. (A) Src^+/? pOCs were kept in suspension for 60 min or plated on Vn-coated dishes for the indicated periods in the absence of serum. Total cell lysates were immunoprecipitated (IP) with anti-PYK2, anti-Cas, anti–paxillin, anti–PLC- ${gamma}$ 1 and 2, and anti-Src antibodies, followed by immunoblotting with anti–phosphotyrosine (pTyr) antibody (left). The same membranes were reblotted with anti-PYK2, anti-Cas, anti–paxillin, anti–PLC- ${gamma}$ 1 and 2, and anti-Src antibodies (right). (B) Src^+/? or Src^-/- pOCs were kept in cell suspension or plated on Vn for 60 min. Total cell lysates were subjected to immunoprecipitation as described above. S, suspension; A, attached. (C) Src^+/? or Src^-/- pOCs (1.0 x 10⁶ cells) were either plated on Vn-coated dishes for 60 min (lanes 1 and 3) or re-cultured with equal number of vitamin D3-treated MB1.8 cells on tissue culture dishes to generate OCLs (lanes 2 and 4). After 12 h, OCLs were purified as described in Materials and Methods. Cell lysates were immunoprecipitated with anti-paxillin, followed by blotting with p-Tyr and anti-paxillin. Arrowhead shows the position of paxillin.

We previously observed tyrosine phosphorylation of paxillinin attached and spread Src^-/- OCLs under steady state conditions(Duong et al. 1998 ). However, in this study, we found thatin Src^-/- pOCs, paxillin was not tyrosine phosphorylated immediatelyfollowing adhesion (Fig 6 B). In order to reconcile these observations,we re-cultured wild-type or Src^-/- pOCs with osteoblastic/stromalMB1.8 cells for 12 h to form OCLs, and compared them with thesame number of pOCs both plated on Vn-coated dishes for 60 min.Levels of tyrosine phosphorylated paxillin were analyzed inOCLs, after removal of MB1.8 cells, and pOCs. As shown in Fig 6C, paxillin was indeed tyrosine-phosphorylated in Src-deficientOCLs (lane 4) as compared to Src^-/- pOCs (lane 3). It shouldbe noted that we consistently observed low yields of Src-deficientOCLs after enzymatic treatment, which is probably due to reducedspreading, as previously reported (Duong et al. 1998 ). Nevertheless,our observations suggest that in spread Src-deficient OCLs atsteady state paxillin is phosphorylated, probably as a consequenceof their interaction with the osteoblasts/stromal cells.

M-CSF Induces Tyrosine Phosphorylation of PLC- ${gamma}$ and Activation of PI 3-Kinase in Src-deficient Osteoclasts
As shown above, M-CSF induces spreading in Src^-/- prefusionosteoclasts in an ${alpha}$ _vß₃-dependent manner. Therefore, weexamined the downstream effectors involved in M-CSF–dependentsignaling in the absence of c-Src. Wild-type and Src-deficientpOCs were plated on Vn-coated dishes for 1 h to achieve maximalactivation of the adhesion-induced signals, and were then treatedwith M-CSF at the indicated time (Fig 7). Although M-CSF appearedto further induce adhesion-dependent tyrosine phosphorylationof PYK2, p130^Cas, and paxillin in wild-type cells, tyrosinephosphorylation of these molecules was not detected in M-CSF–treatedSrc-deficient pOCs (Fig 7 A). In contrast, M-CSF rapidly inducedtyrosine phosphorylation of PLC- ${gamma}$ 2 (Fig 7 A) and PLC- ${gamma}$ 1 (datanot shown) within 0.5 min in these cells, which gradually returnedto basal levels after 60 min, suggesting that tyrosine phosphorylationof both PLC- ${gamma}$ isoforms by M-CSF is Src independent. The M-CSF-inducedPLC phosphorylation was found to be transient, as compared tothat of ${alpha}$ _vß₃-dependent PLC phosphorylation in Src^+/? pOCs(Fig 6 A).

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Figure 7. M-CSF–induced intracellular signaling in Src^-/- prefusion osteoclast-like cells. Src^+/? and Src^-/- pOCs were kept in suspension or plated on Vn for 60 min in the absence of serum, followed by treatment with 5 nM M-CSF for the indicated periods with or without PI 3-kinase inhibitors. (A) Total cell lysates were immunoprecipitated with anti-PYK2, anti-Cas, antipaxillin, and anti-Src, and blotted with antiphosphotyrosine (pTyr, left), anti-PYK2, anti-Cas, antipaxillin, and anti-Src antibodies (right). (B) Lysates were immunoprecipitated with anti–PLC- ${gamma}$ 2, blotted with anti-pTyr (top), then with anti–PLC- ${gamma}$ 2 antibodies (middle). Part of the total cell lysates were used for immunodetection of c-Src (bottom). (C) Lysates were immunoprecipitated with anti-Akt/PKB, blotted with anti–phospho-Akt/PKB, or anti-Akt/PKB antibodies. S, suspension; A, attached.

PI 3-kinase activity was previously reported to be requiredfor PLC- ${gamma}$ activation (Falasca et al. 1998 ; Gratacap et al.1998 ). In this study, LY294002, a selective PI 3-kinase inhibitor,inhibited M-CSF–mediated tyrosine phosphorylation of PLC- ${gamma}$ 2(Fig 7 B), indicating that PI 3-kinase is an upstream mediatorof PLC- ${gamma}$ activation in osteoclasts. Given the limitations ofthis cell system, including relatively small cell numbers andshort survival of purified osteoclast-like cells in culture,which precluded direct determination of PI 3-kinase activity,we examined the activation of Akt/PKB as a downstream targetof PI 3-kinase in these cells (Downward 1998 ). Indeed, in Src^-/-pOCs (Fig 7 C, right) as well as in wild-type cells (Fig 7 C,left), M-CSF–induced phosphorylation of Akt/PKB, whichwas blocked by the PI 3-kinase inhibitors, wortmannin (Fig 7C, left), and LY294002 (data not shown). We also noted an increasedlevel of Akt proteins in Src-deficient pOCs (Fig 7c). Usingimaging densitometry, the ratio of Akt protein levels in Src^-/-to wild-type pOCs was estimated to be 1.7-fold. Furthermore,the specific activity of tyrosine phosphorylated Akt in wild-typeand Src^-/- pOCs upon treatment with M-CSF, at peak levels (2min) relative to basal levels (0 min), were estimated to be4.4 and 3.9, respectively. This indicated that although Aktproteins appeared to be induced in the absence of c-Src in pOCs,the extent and time course of M-CSF-induced phosphorylationof Akt were similar in wild-type and Src-deficient prefusionosteoclasts (Fig 7c). Interestingly, the time course of PLCphosphorylation (Fig 7b) is coincident with M-CSF-induced activationof PI 3-kinase (Fig 7c). Since LY294002 blocked PLC- ${gamma}$ phosphorylation(Fig 7b), these data indicated that in Src-deficient pOCs, M-CSFactivates PI 3-kinase, which subsequently leads to PLC- ${gamma}$ activation.Taken together, these findings implicate PI 3-kinase and PLC- ${gamma}$ in the M-CSF-dependent cytoskeletal organization in Src-deficientosteoclasts, which further induces ligand engagement of ${alpha}$ _vß₃integrins, formation of adhesion contacts and cell spreadingas shown in Fig 2 A.

M-CSF–induced Recruitment of Downstream Mediators to ß₃ Integrins in Src-deficient Osteoclasts, Is Similar to Adhesion-dependent Recruitment in Wild-Type Cells
Since previous reports demonstrated the association of ${alpha}$ _vß₃integrins with c-Src and PI 3-kinase in osteoclasts (Hruskaet al. 1995 ; Lakkakorpi et al. 1997 ), we examined by coimmunoprecipitationwith anti–ß₃ integrin antibodies the adhesion-dependentassociation of ${alpha}$ _vß₃ with PLC- ${gamma}$ , PI 3-kinase, c-Src, andPYK2. In pOCs, cell adhesion to Vn increased the associationof ß₃ integrins with PLC- ${gamma}$ 2, PI 3-kinase, PYK2, and c-Src(Fig 8 A, lanes 1 and 2, 5 and 6, 9 and 10, and 13 and 14, respectively).These data suggest that integrin–ligand engagement inducesnot only tyrosine phosphorylation of these signaling moleculesbut also their association with the integrin receptor.

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Figure 8. M-CSF–induced association of ${alpha}$ _vß₃ integrin with signaling molecules in Src^-/- prefusion osteoclast-like cells. (A) Cell adhesion and M-CSF induce the association of ß₃ integrins with signaling molecules in pOCs. Src^+/? and Src^-/- pOCs (1.5 x 10⁶ cells per condition) were plated on PL- or Vn-coated dishes. After culture for 60 min, Src^-/- cells were treated with or without 5 nM M-CSF for 5 min. Total cell lysates were immunoprecipitated (IP) with anti–ß₃ integrin antibodies, followed by immunoblotting (IB) with anti–PLC- ${gamma}$ 2 (lanes 1–4), anti-PYK2 (lanes 5–8), anti–PI 3-kinase (lanes 9–12), anti–c-Src (lanes 13–16), and anti–ß₃ integrin (lanes 17–20). The molecular masses of marker proteins (in kD) are on the left. Positions of c-Src (arrowhead) and of p85 subunit of PI 3-kinase (asterisk) are as indicated. (B) PLC and PI 3-kinase inhibitors block M-CSF–induced association of ${alpha}$ _vß₃ integrin with signaling molecules in Src-deficient pOCs. Src^-/- pOCs (1.5 x 10⁶ cells per condition) were plated on Vn as described above, followed by incubation with either U73122 (1 µM) or LY294002 (50 µM) for 40 min, then with 5 nM M-CSF. Lysates were immunoprecipitated with hamster anti–murine ß₃ integrin antibodies (lanes 2–4, 6–8, 10–12, and 14–16) or control hamster IgG (lanes 1, 5, 9, and 13), followed by blotting with anti–PLC- ${gamma}$ 2 (lanes 1–4), anti-PYK2 (lanes 5–8), anti–PI 3-kinase (lanes 9–12), or anti–ß₃ integrin (lanes 13–16). p85 subunit of PI 3-kinase (small arrowheads). C, control hamster IgGs.

On the other hand, in Src-deficient pOCs plated on Vn, PLC- ${gamma}$ 2,PI 3-kinase, and PYK2 were only weakly coimmunoprecipitatedwith the ß₃ integrins (Fig 8 A, lanes 3, 7, and 11), indicatingthat Src kinase is important for the adhesion-dependent recruitmentof various downstream mediators to the integrin receptor. However,association of ${alpha}$ _vß₃ integrins with PLC- ${gamma}$ 2, PI 3-kinase,and PYK2 was promoted in Src^-/- pOCs by treatment with M-CSF(Fig 8 A, lanes 3 and 4, 7 and 8, and 11 and 12). These datasuggest that in the absence of c-Src, M-CSF–induced activationof PLC- ${gamma}$ 2 and PI 3-kinase was sufficient to further the recruitmentof PYK2 to ${alpha}$ _vß₃ receptors independent of tyrosine phosphorylation.

Additional evidence for the role of PLC and PI 3-kinase in theM-CSF–dependent association of ${alpha}$ _vß₃ integrins withtheir downstream effectors was provided by the fact that eitherU73122 or LY294002 disrupted the recruitment of PLC- ${gamma}$ 2, PYK2,and PI 3-kinase to ß₃ integrins in Src-deficient pOCs(Fig 8 B). These data supported the pharmacological findingssuggesting that PI 3-kinase and PLC take part in both, adhesion-and M-CSF-dependent signaling. The findings also suggest thatM-CSF modulates ${alpha}$ _vß₃ integrin-dependent signaling via activationof PI 3-kinase and PLC- ${gamma}$ , leading to cytoskeletal reorganizationand formation of integrin-associated adhesion contacts in osteoclasts.

To further test the involvement of ${alpha}$ _vß₃ integrins in M-CSF–dependentspreading of Src^-/- pOCs, we examined the localization of ${alpha}$ _vß₃in M-CSF–treated cells. As shown in Fig 9, ß₃ integrins(a and d, in green) colocalized with F-actin (Fig 9 b, red)as well as PLC- ${gamma}$ 2 (Fig 9 e, red). Colocalization of ß3integrins and PLC- ${gamma}$ were found in adhesion contacts of the M-CSF-treatedSrc-deficient pOCs plated on Vn (Fig 9 c and f, in yellow).

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Figure 9. Colocalization of ${alpha}$ _vß₃ integrin and PLC- ${gamma}$ in M-CSF treated Src^-/- prefusion osteoclasts. Src^-/- pOCs were plated on Vn-coated glass coverslips for 1 hr, then treated with 5 nM M-CSF for 30 min. Cells were fixed double stained with polyclonal anti-ß3 integrin and monoclonal anti-PLC- ${gamma}$ 1 or PLC- ${gamma}$ 2 antibodies. Pseudocolored confocal microscopic images of ß3 integrins (a, d, in green) and double staining of PLC- ${gamma}$ 1 (b, in red) or PLC- ${gamma}$ 2 (e, in red). Colocalization (c, f, in yellow) appears to be more prominent in the adhesion contacts organized at the spreading edge of the cells. Images merged from optical sections of 4.7 µm thickness at the adhesion surface of the cells. Bar, 10 µm.

Adhesion- and M-CSF–dependent Association of PYK2 and PLC- ${gamma}$ in Osteoclasts
We next examined which molecular interactions are importantfor the convergence of the integrin- and M-CSF–dependentsignals in prefusion osteoclasts in the absence of c-Src. Sincewe were previously unable to demonstrate stable interactionsof PYK2 and PI 3-kinase in OCLs (Duong et al. 1998 ), we examinedthe association of PYK2 with PLC- ${gamma}$ in these cells. Both anti–PLC- ${gamma}$ 1and 2 antibodies coprecipitated PYK2 (Fig 10 A) and anti-PYK2antibodies pulled down PLC- ${gamma}$ 2 (Fig 10 B), supporting the in situassociation of the two proteins in OCLs. Furthermore, upon adhesionto Vn a stronger association of PYK2 and PLC- ${gamma}$ was observed thanin cells plated on PL (Fig 10 C). Moreover, in the presenceof U73122 the association of PYK2 and PLC- ${gamma}$ 2 was reduced to thelevel observed in cells on PL (Fig 10 C). These findings suggestthat in osteoclasts, both integrin-dependent activation of PYK2and PLC- ${gamma}$ 2 and the phospholipase activity itself might be importantfor the stable interaction between these molecules.

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Figure 10. M-CSF–dependent association of PLC- ${gamma}$ 2 and PYK2 in osteoclasts. Src^+/? pOCs were cultured on Vn-coated dishes for 60 min in the absence of serum. (A) Total cell lysates were immunoprecipitated (IP) with anti–PLC- ${gamma}$ 2 (lane 1) and anti–PLC- ${gamma}$ 1 (lane 2), followed by blotting with anti-PYK2 (left), anti–PLC- ${gamma}$ 2 (middle), or anti–PLC- ${gamma}$ 1 (right) antibodies. (B) Lysates were immunoprecipitated with anti-PYK2 mAb 11 (lane 1) and anti-PYK2 N-19 antibodies (lane 2), followed by blotting with anti–PLC- ${gamma}$ 2 (left) or anti-PYK2 (right). (C) Src^+/? pOCs were cultured on PL or Vn for 60 min with or without 1 µM U73122. Lysates were immunoprecipitated with anti–PLC- ${gamma}$ 2 and blotted with anti-PYK2 (left), and anti–PLC- ${gamma}$ 2 (right) antibodies. (D) Lysates of Src^+/? OCLs were incubated with GST fusion proteins containing NH₂- and COOH-terminal SH2 domains or SH3 domains of PLC- ${gamma}$ 1 and blotted with anti-PYK2 antibodies (top) or incubated with GST fusion proteins of NH₂- or COOH-terminal domains or kinase (K) domain of PYK2 and blotted with anti–PLC- ${gamma}$ 2 antibodies (bottom). (E) Src^-/- pOCs (1.5 x 10⁶ cells per condition) were plated on Vn and treated without and with M-CSF. Adhesion of Src^+/? pOCs on Vn was used as control. Lysates were immunoprecipitated with anti–PLC- ${gamma}$ 2 and blotted with anti-PYK2, followed by anti–PLC- ${gamma}$ 2 antibodies (left) or immunoprecipitated with anti-N terminal PYK2 and blotted with anti–PLC- ${gamma}$ 2, followed by anti-PYK2 antibodies (right). Molecular weight markers (in kD) are as indicated on the left. Positions of PYK2 (arrowhead) and of PLC- ${gamma}$ (asterisk) are as indicated.

To partially characterize the domains of PLC- ${gamma}$ which mediatebinding to PYK2, GST fusion proteins encoding the NH₂- and COOH-terminalSH2 domains or the SH3 domain of PLC- ${gamma}$ 1 were incubated with lysatesprepared from OCLs. GST fusion protein containing the COOH-terminalSH2 domain and the SH3 domain of PLC- ${gamma}$ bound to PYK2 from OCLlysates (Fig 10 D, top), suggesting that PLC- ${gamma}$ could bind toeither a tyrosine phosphorylated moiety or to a proline-richregion of PYK2. Conversely, the COOH-terminal domain containingproline-rich regions of PYK2 was found to bind to PLC- ${gamma}$ 2 (Fig 10D, bottom), supporting the above observations on both theadhesion (phosphorylation)-dependent association of PYK2 andPLC- ${gamma}$ , as well as their constitutive interaction. Additionalstudies will be conducted to further analyze the structuralfeatures that are important for the interaction of these twomolecules.

Since we found that both integrin-dependent activation of PYK2and PLC- ${gamma}$ 2 and its phospholipase activity were important fortheir interaction in wild-type pOCs, we thus proceeded to examinethe direct interaction of PYK2 and PLC- ${gamma}$ 2 in M-CSF–treatedSrc-deficient pOCs. Although PYK2 is not tyrosine phosphorylatedin Src^-/- pOCs (Fig 7 A), direct interaction of PYK2 and PLC- ${gamma}$ 2was induced in response to M-CSF (Fig 10 E). This observationwas reproduced in three separate experiments and supports therole of PLC activity in the integrin- and M-CSF–mediatedassociation with their downstream mediators (Fig 8a and Fig b).Furthermore, these data suggest that the direct associationof PYK2 and PLC- ${gamma}$ might play an important role in both M-CSF–and adhesion-dependent signaling pathways in prefusion osteoclasts.

Discussion

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Abstract
Introduction
Materials and Methods
Results
Discussion
Acknowledgements
References

Src kinases play an important role in cell adhesion and migration,in cell cycle control, and in cell proliferation and differentiation(Thomas and Brugge 1997 ). Moreover, novel roles for Src kinasesin the control of cell survival and angiogenesis have recentlyemerged (Schlessinger 2000 ). In this study, we examined integrin-and M-CSF–mediated signaling pathways involved in theadhesion and migration of osteoclast precursors, using Src^+/?and Src^-/- pOCs formed in vitro. The findings indicate thatc-Src is essential for integrin-initiated signaling in thesecells upon ligand engagement, since the absence of c-Src causesimpairment in cell spreading associated with significant reductionin tyrosine phosphorylation of several adhesion/signaling moleculesincluding PYK2, p130^Cas, paxillin, and PLC- ${gamma}$ . The involvementof Src family kinases in integrin-mediated signaling pathwayhas been reported in Src^-/- Yes^-/-Fyn^-/- triple mutant cells(Klinghoffer et al. 1999 ) and macrophages derived from Hck^-/-Fgr^-/-Lyn^-/- triple mutant mice (Meng and Lowell 1998 ). Tripledeletions of Src family kinases are required to block the integrin-dependentsignals in these cells, probably due to functional overlap.On the other hand, in Src-deficient fibroblasts, the vitronectinreceptor-mediated traction forces during cell migration wererecently demonstrated to be selectively modulated by c-Src (Felsenfeldet al. 1999 ).

Osteoclasts abundantly express c-Src, as well as very low levelsof c-fyn, c-yes, and c-lyn (Horne et al. 1992 ). However, theabsence of c-Src is sufficient to abolish bone resorption invivo, without reducing osteoclast number (Soriano et al. 1991), suggesting that these members of the Src kinase family donot compensate for the absence of c-Src in osteoclast function,both in vivo and in vitro (Horne et al. 1992 ). Indeed in Src^-/-pOCs, we found no change in protein levels of c-yes and c-lyn,and a very small increase (<2-fold) in c-fyn expression,and could not detect these members of c-Src family kinases inimmunoprecipitates of ${alpha}$ _vß₃ integrins (data not shown).Nevertheless, we show in this study that c-Src is not requiredfor M-CSF–induced cytoskeletal reorganization in prefusionosteoclast-like cells. M-CSF induces cell spreading and migration,along with tyrosine phosphorylation of PLC- ${gamma}$ 2 in Src^-/- pOCs,although it did not induce tyrosine phosphorylation of PYK2and p130^Cas under the same conditions. We previously observedtyrosine phosphorylation of paxillin in attached and spreadSrc^-/- OCLs (multinucleated osteoclast like cells) under steadystate conditions (Duong et al. 1998 ). In this study, we examinedadhesion-mediated signaling immediately following the attachmentof Src^-/- pOCs and found that paxillin is not tyrosine phosphorylatedduring initial adhesion process. To resolve this apparent inconsistency,we re-cultured Src^-/- pOCs with osteoblastic/stromal cells toform OCLs, and found that paxillin was indeed tyrosine phosphorylatedin these attached cells under steady state conditions. Thisobservation suggests that in OCLs paxillin is phosphorylatedby an alternative kinase probably in response to stimuli receivedfrom osteoblasts/stromal cells.

Our observations are consistent with a recent report showingthat PDGF-mediated signaling is similar in Src^-/- Yes^-/-Fyn^-/-triple mutant fibroblasts and the wild-type controls (Klinghofferet al. 1999 ). In addition, our in vitro findings of M-CSF–inducedcell spreading and migration of Src^-/- prefusion osteoclastscould be relevant to in vivo observations on Src-deficient mice,where osteoclasts are multinucleated and adhere to the bonesurface. The ability of Src-deficient osteoclasts to spreadand migrate in vivo (Boyce et al. 1992 ) could reflect the influenceof M-CSF or other growth factors. Moreover, transgenic expressionof kinase-deficient Src in Src^-/- mice rescued osteoclast function,indicating that Src may function in part as an adaptor to recruitdownstream signaling molecules (Schwartzberg et al. 1997 ).Our findings apparently differ from a previous report showingthat M-CSF did not induce cell spreading in Src-deficient osteoclastsderived from Src knockout mice (Insogna et al. 1997 ). The differencecould be due to use in that study of adherent multinucleatedprimary osteoclasts in the presence of serum and bone marrowstromal cells. The present study used purified prefusion osteoclast-likecells under serum-free condition, in which M-CSF-mediated signalingcould be enhanced.

The data presented here support the role of PLC- ${gamma}$ in integrin-dependentregulation of cytoskeletal organization. This is supported byinduction of PLC- ${gamma}$ tyrosine phosphorylation upon cell adhesionand inhibition of cell spreading in wild-type osteoclasts bya PLC inhibitor. These observations are consistent with previousstudies showing that integrin–ECM interactions inducetyrosine phosphorylation of PLC- ${gamma}$ 1 (Langholz et al. 1997 ) andPLC- ${gamma}$ 2 (Asselin et al. 1997 ). It was also recently reportedthat phosphorylation of PLC- ${gamma}$ 1 at the tyrosine residue 783 isimportant for regulation of cytoskeletal organization in fibroblasts(Yu et al. 1998 ; Pei and Williamson 1998 ), while PLC- ${gamma}$ 1 canserve as a substrate of c-Src in in vitro kinase assays (Liaoet al. 1993 ; Nakanishi et al. 1993 ). Furthermore, PLC- ${gamma}$ 1–nullfibroblasts exhibit a more round-up morphology than their normalcounterparts (Ji et al. 1997 ). Taking advantage of the crucialrole of c-Src in osteoclasts, we demonstrated that in thesecells PLC- ${gamma}$ is downstream of c-Src, since adhesion does not inducetyrosine phosphorylation of PLC- ${gamma}$ 1 and 2 in Src-deficient pOCs.

This study points to interactions between adhesion- and growthfactor–initiated signal transduction, which seem to playa role in cell spreading and migration. There are several possiblemechanisms for synergy between adhesion and growth factor signalingpathways (Schwartz and Ingber 1994 ; Yamada and Miyamoto 1995), for example activation of common downstream effectors. Wesuggest that in prefusion osteoclasts PLC- ${gamma}$ is one of the downstreammolecules, activated by adhesion- and M-CSF–dependentsignals, that lead to cytoskeletal reorganization. PLC- ${gamma}$ is activatedeither by cell attachment in a Src dependent manner or by M-CSF-treatmentwhich is not Src dependent. The role of PLC is supported bypharmacological evidence showing that PLC inhibitors block bothadhesion- and M-CSF–induced cell spreading. Previous studieshave implicated MAP kinases as candidates for this cross-signaling(Chen et al. 1994 ; Zhu and Assoian 1995 ); however, in osteoclasts,M-CSF did not activate MAP kinases ERK1 and 2 in Src^-/- pOCs,and the MAP kinase kinase inhibitor, PD98059, had little effecton M-CSF–induced cell spreading of Src-deficient prefusionosteoclasts.

Another likely mechanism for the synergy between adhesion- andgrowth factor–mediated signaling pathways is the physicalinteraction (clustering) of key components of both pathways,allowing the convergence of the two (Thomas and Brugge 1997; Giancotti and Ruoslahti 1999 ). Coclustering of integrinsand growth factor receptors appears to require association withthe cytoskeleton and recruitment of downstream signaling molecules.Aggregation of these molecules has been thought to bring bothadhesion- and growth factor-mediated signaling closer to a thresholdof manifest activity (Giancotti and Ruoslahti 1999 ). Recentreports have documented the physical interaction of ${alpha}$ _vß₃with the insulin, PDGF or VEGF receptors in fibroblasts (Woodardet al. 1998 ; Soldi et al. 1999 ). More recently, FAK was demonstratedto be an important proximal link between PDGF and EGF receptorsand ß1 integrins during fibroblast chemotactic migration(Sieg, et al. 2000 ). Interestingly, for chemotactic cell motilityFAK kinase activity is dispensible, while phosphorylation atFAK Y397, the Src-kinase binding site, and the integrity ofthe actin cytoskeleton are required for PDGF/EGF- and integrin-mediatedcell migration (Sieg, et al. 2000 ).

In the case of prefusion osteoclasts, our data suggest thatM-CSF can modulate the localization of ${alpha}$ _vß₃ and its interactionwith downstream effectors in a c-Src–independent manner.This is supported by the following findings: first, M-CSF–inducedcell spreading of Src^-/- pOCs depends on attachment to Vn; second,echistatin, an ${alpha}$ _vß₃ integrin antagonist, blocks M-CSF–inducedcell spreading; third, in M-CSF–treated Src^-/- pOCs, ß₃integrin localizes to adhesion contacts along with PLC; andfourth, association of ${alpha}$ _vß₃ with PYK2, PI 3-kinase, andPLC- ${gamma}$ in Src^-/- prefusion osteoclasts is M-CSF dependent andPYK2 binds directly to PLC- ${gamma}$ . These findings suggest that activationof M-CSF receptors result in the recruitment of intracellularsignaling molecules to ${alpha}$ _vß₃ integrins at adhesion contacts.Furthermore, in Src-deficient cells, M-CSF induces the associationof ß₃ integrin engaged by its extracellular ligand withsignaling molecules including PI 3-kinase, PLC- ${gamma}$ , and PYK2, independentof PYK2 tyrosine phosphorylation. These interactions are blockedby PLC or PI 3-kinase inhibitors. Therefore, our data suggestthat activation by either integrin ligands or growth factorsresults in the physical recruitment of key components of thesepathways to adhesion contacts. On the other hand, we could notconvincingly demonstrate the presence of M-CSF receptors inthe ${alpha}$ _vß₃-associated immunocomplexes (data not shown). Weare presently investigating further the possible physical associationof M-CSF receptor with ${alpha}$ _vß₃ integrin in osteoclasts duringchemotactic migration.

The observations on PI 3-kinase are consistent with previousreports showing that growth factor receptors, e.g., PDGF (Kinashiet al. 1995 ), thrombopoietin (Zauli et al. 1997 ), insulin(Guilherme et al. 1998 ), EGF (Adelsman et al. 1999 ), and VEGF(Soldi et al. 1999 ) stimulate integrin-mediated cell adhesionthrough a PI 3-kinase–dependent pathway. In the case ofosteoclasts, the association of ${alpha}$ _vß₃ integrins with PI3-kinase has been reported (Hruska et al. 1995 ; Lakkakorpiet al. 1997 ). Present findings suggest that PLC- ${gamma}$ is a downstreameffector of PI 3-kinase, involved in the regulation of integrin-dependentsignaling by growth factors. Consistent with these observations, Shibayama et al. 1999 reported recently that U73122 blocksIL-3–induced ${alpha}$ ₄ß₁ and ${alpha}$ ₅ß₁ integrin activationin Baf3 cells.

An obvious question is how M-CSF–dependent activationof PI 3-kinase and PLC- ${gamma}$ modulate integrin function. FAK wasdemonstrated to bind to peptides that mimic the ß₁ integrincytoplasmic domains (Shaller et al. 1995 ). In addition, Plopperet al. 1995 reported that RGD-coated beads pulled down themolecular complex that contains FAK, c-Src, and PLC- ${gamma}$ in capillaryendothelial cells. Recently, Zhang et al. 1999 reported thatPLC- ${gamma}$ 1 can associate with FAK. This association is mediated bytyrosine-397 in FAK and the COOH-terminal SH2 domain of PLC- ${gamma}$ 1and is dependent on cell adhesion. We found that PYK2, a memberof the FAK family kinases, is highly expressed in osteoclastsand is tyrosine phosphorylated in a c-Src–dependent mannerupon ${alpha}$ _vß₃-mediated adhesion (Duong et al. 1998 ). In addition,PYK2 localizes to podosomes, the primary adhesion structuresin osteoclasts (Duong et al. 1998 ). In this study, PLC- ${gamma}$ wasfound to associate with PYK2 independent of PYK2 phosphorylation,probably via the SH3 domain of PLC- ${gamma}$ and the proline-rich domainstoward the COOH-terminal region of PYK2. Importantly, this interactionwas further enhanced upon osteoclast adhesion to Vn, possiblyvia interaction of the COOH-terminal SH2 domain of PLC- ${gamma}$ withtyrosine-402 in PYK2 (Schlaepfer et al. 1999 ). This interactionis sensitive to the PLC- ${gamma}$ inhibitor. Taken together, these datasuggest that in osteoclasts either integrin- or M-CSF–mediatedsignals result in recruitment of PYK2 and PLC- ${gamma}$ to the integrin-associatedcomplex at adhesion sites. Furthermore, our data also suggestthat PYK2 may function as an adaptor recruiting other integrin-associatedmolecules, including p130^Cas and PLC- ${gamma}$ , during M-CSF-inducedSrc^-/- osteoclast spreading and migration. In part, this observationis supported by a previous study in which kinase-deficient c-Srcwas implicated to function as an adaptor, when its transgenicexpression rescued osteoclast function in Src^-/- mice (Schwartzberget al. 1997 ).

Questions that remain to be answered relate to how PI 3-kinaseand PLC- ${gamma}$ can mediate cell spreading and migration in responseto growth factors and cytokines. PI 3-kinase-mediated activationof PLC- was suggested to be important for PLC membrane targeting(Falasca et al. 1998 ). One candidate molecule might be PKC,which is activated by DAG, a product of PLC- ${gamma}$ (Kolanus and Seed1997 ). In FG human carcinoma cells, Klemke et al. 1994 demonstrateda link between activation of EGF receptor tyrosine kinase, PKC,and integrin-dependent cell spreading. The pleckstrin homologydomain of PLC- ${gamma}$ was shown to preferentially recognize 3-phosphorylatedphosphoinositides, including PtdIns(3)P, PtdIns(3,4)P₂, andPtdIns (3,4,5)P₃ (PIP3) and to lesser extent PtdIns(4,5)P₂ (PIP2)(Falasca et al. 1998 ; Kavran et al. 1998 ). Recent studiesrevealed the cytoplasmic distribution of PtdIns(3)P to endosomes,and PtdIns(3,4)P₂ and PIP3 to plasma membranes, and implicatedroles of these PI 3-kinase products in regulation of variousprocesses, including endosome fusion and motility, phagocytosis,pinocytosis, regulated exocytosis, and cytoskeletal organization(Czech 2000 ). Recently, the local concentration of PIP2 wassuggested to control adhesion strength of the actin-based cytoskeletonto plasma membrane, which also define cell shape and cell movement(Raucher et al. 2000 ). Interestingly, the localized adhesionenergy in NIH3T3 cells was shown to be reduced by either EGFor PDGF, known stimuli that activate PLC- ${gamma}$ , and this reductioncould be blocked by U73122 (Raucher et al. 2000 ). Together,these studies suggest that PLC- ${gamma}$ and PI 3-kinase, which mediatethe cytoskeletal structure by changing local concentrationsof PIP2, PIP3, DAG, and calcium, could indirectly modulate integrinfunction.

In summary, we have demonstrated that in prefusion osteoclasts:(a) c-Src is essential for integrin "outside-in" signaling;(b) c-Src is not necessary for M-CSF–mediated cytoskeletalreorganization; (c) PLC- ${gamma}$ is a common downstream mediator foradhesion and growth factor signals; and (d) M-CSF–initiatedsignaling modulates the ${alpha}$ _vß₃ integrin–ligand interactionand the recruitment of signaling molecules to adhesion structures,possibly via PLC- ${gamma}$ activation.

Footnotes

¹ Abbreviations used in this paper: ECM, extracellular matrix;ERK, extracellular signal–regulated kinase; FAK, focaladhesion kinase; GST, glutathione S-transferase; MAP, mitogen-activatedprotein; M-CSF, macrophage colony stimulating factor; OCL, multinucleatedosteoclast-like cell; PI 3-kinase, phosphatidylinositol 3-kinase;PL, poly-L-lysine; pOC, prefusion osteoclast-like cell; SH,src homology; TRAP, tartrate-resistant acid phosphatase; Vn,vitronectin.

Acknowledgements

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Original Article

Convergence of vß3 Integrin– and Macrophage Colony Stimulating Factor–mediated Signals on Phospholipase C in Prefusion Osteoclasts

Convergence of ${alpha}$ _vß₃ Integrin– and Macrophage Colony Stimulating Factor–mediated Signals on Phospholipase C ${gamma}$ in Prefusion Osteoclasts