Reduced motility and response to SDF-1 are associated with impaired homing of CD45KO progenitors
The lower numbers of progenitors in the CD45KO BM may lead to their reduced appearance in the PB after G-CSF treatment. To examine if CD45 is directly involved in progenitor cell motility, we isolated BM subpopulations from CD45KO mice and evaluated their spontaneous and SDF-1–induced migration potential. The migration of CD45KO MNCs was significantly reduced compared with WT cells (Fig. 2 A), including both spontaneous as well as SDF-1–directional migration. Of note, no differences were observed in the expression of CXCR4, the receptor for SDF-1 (unpublished data). MNCs isolated from the BM of G-CSF–treated mice exhibited higher motility compared with untreated cells (Fig. 2 A). This high motility of G-CSF–treated WT cells correlated with their increased CD45 expression levels (Fig. 1, A and B). However, reduced migration was observed in cells obtained from CD45KO mice despite G-CSF treatment. Importantly, although normal mobilization levels were observed after 5 d of G-CSF administration, CD45KO BM MNCs still demonstrated reduced spontaneous and SDF-1 migration compared with their WT counterparts (Fig. 2 A). When CD45KO BM MNCs were allowed to migrate through a fibronectin (FN)-coated barrier, stronger reductions in their migration were observed (Fig. 2 B). These results suggest that together with their intrinsic defects in cell motility, CD45KO cells predominantly have an impaired ability to cross extracellular matrix barriers. This notion was further evident in vivo, as CD45KO MNCs showed reduced homing compared with their WT counterparts (Fig. 2 C). Next, we examined the motility potential of sorted representative subpopulations that strongly respond to G-CSF: CD11b⁺ monocytes and c-Kit⁺ enriched progenitor cells. These cell fractions were isolated from the BM of WT and CD45KO mice untreated or treated with G-CSF for 5 d. As observed with the MNC population, CD45KO CD11b⁺ monocytes showed reduced spontaneous and SDF-1–mediated migration compared with WT CD11b⁺ cells (Fig. 2 D). Similarly, CD45KO CD11b⁺ cells demonstrated reduced homing to the BM of the recipient mice (Fig. 2 E). Live cell images show that immature WT c-Kit⁺ cells responded to SDF-1 chemotactic signals by cell spreading and the formation of elongated protrusions (Fig. 2 F, left). In contrast, immature CD45KO c-Kit⁺ cells remained mostly round, forming only short cell protrusions in response to SDF-1 (Fig. 2 F, right). In vivo homing assays demonstrated the inferior homing of CD45KO c-Kit⁺ progenitors to the BM and spleen, in comparison to their WT counterparts (Fig. 2 G). Interestingly, CD45KO spleen-derived colony-forming progenitor cells also exhibited poor homing potential to the BM and spleen of recipient mice (Fig. 2 H). Additionally, in a functional repopulation assay, CD45KO spleen-derived cells showed a reduced potential to engraft the BM of WT recipients, also showing defects in primitive repopulating cells (Fig. 2 I). These results demonstrate systemic cell autonomous defects in CD45KO cell motility.

View larger version (57K): [in this window] [in a new window] [Download PPT slide]   Figure 2. Impaired migration and reduced response to SDF-1 by CD45KO progenitors. (A and B) In vitro migration of MNCs from the BM of CD45KO or WT mice either untreated or treated with G-CSF for 3 or 5 d. Cells were allowed to migrate without (spont.) or with addition of SDF-1 to the lower well. (B) Migration of WT and CD45KO BM MNCs of untreated mice through bare or FN-coated filters toward SDF-1. (C) Homing of BM MNCs derived from untreated WT and CD45KO mice to the BM and spleens of recipient NOD/SCID mice 3 h after transplantation. (D and E). In vitro migration (D) or homing assay (E) of BM CD11b+ cells sorted from the BM of untreated or G-CSF–treated WT or CD45KO mice. (F) c-Kit+ cells were sorted from the BM of WT or CD45KO mice, untreated or treated with G-CSF for 5 d and stimulated in vitro with SDF-1. Representative images demonstrate cell polarization (indicated by black arrows). Bar, 20 µm. (G) Homing of c-Kit+ cells sorted from the BM of WT or CD45KO mice to the BM of NOD/SCID recipient mice 3 h after transplantation. (H) Homing of spleen progenitor cells isolated from WT or CD45KO mice to the BM and spleens of lethally irradiated NOD/SCID/β2 recipients. (I) Percentages of engraftment in WT-recipient BM and PB transplanted with spleen-derived cells from WT and CD45KO mice. Data represent the levels of specific lineages, as indicated. Shown are the means of four recipients in each group ± SE. *, P < 0.01; **, P < 0.05.

View larger version (40K): [in this window] [in a new window] [Download PPT slide]   Figure 3. CD45 deficiency reduces MMP-9 levels and increases cell adhesion via activation of Src kinase. (A and B) BM or PB MNCs were isolated from CD45KO or WT mice, either untreated or treated with G-CSF for 3 d. Cells were cultured and the activity of MMP-9 in the conditioned media was detected by the gelatin zymography assay. A summary of three independent experiments and representative gel images of BM cells (A) and PB cells (B) is shown (±SD). (C) FACS analyses of the β1-activated epitope 9EG7 in untreated WT or CD45KO BM MNCs. (C, i) Representative histogram of background staining and 9EG7 expression in WT (black line) and CD45KO (gray line). (C, ii) Summary of five independent experiments (±SD). (D) Adhesion assay of WT and CD45KO BM MNCs to FN-coated wells. Shown is a summary of four independent experiments (mean ± SD). (E and F) Western blot analysis of Src phosphorylation or Src activity levels (F) in whole-cell lysates that were prepared from BM MNCs of WT or CD45KO mice, either untreated or after G-CSF injections. Histogram represents a summary of four independent experiments. Values represent the fold change of the control. (G) Western blot analysis for Erk phosphorylation. Lysates were prepared as described in E. (H) SDF-1–induced migration of WT and CD45KO BM MNCs pretreated with 1 µM of the Src inhibitor PP2 or DMSO as a control. Data represent mean ± SD values of three independent experiments and are shown as the fold increase from DMSO-treated cells. *, P < 0.01; **, P < 0.05.

CD45 deficiency leads to hyperactivation of the Src signaling pathway
Several papers have demonstrated the importance of Src kinases, the natural substrate of CD45, in integrin-mediated adhesion in various mature lymphoid and myeloid cells (27, 28). We thus examined the Src phosphorylation status and activity during steady state and in response to G-CSF administration. G-CSF stimulations of WT mice led to a reduction in Src phosphorylation and activity in BM MNCs (Fig. 3, E and F). Notably, these modulations in Src were inversely correlated with CD45 expression (Fig. 1, A and B). Interestingly, MNCs derived from the BM of untreated CD45KO mice displayed enhanced Src phosphorylation and activity (Fig. 3, E and F), and G-CSF stimulations only slightly reduced it in these CD45KO cells. Src family kinases were shown to negatively regulate the mitogen-activated protein kinase cascades, particularly extracellular signal-regulated kinase (Erk) activation (29). As Fig. 3 G shows, G-CSF treatment activated Erk protein in WT-derived BM cells, suggesting that Src kinase activity is indeed reduced. Interestingly, in the CD45KO BM, where Src kinases are hyperactive, Erk proteins are inhibited, as demonstrated by the low phosphorylation of Erk both in untreated and in G-CSF–treated mice. Finally, inhibition of Src proteins in CD45KO BM-derived cells using the PP2 inhibitor, which down-regulates the hyperactivity of Src proteins, increased migration of these CD45KO cells to a gradient of SDF-1 (Fig. 3 H). These results ultimately demonstrate the link between CD45, Src kinase activity, and the regulation of motility properties.

Impaired receptor activator of NF-B ligand (RANKL)–induced progenitor mobilization in CD45KO mice
Next, we chose to specifically stimulate CD45KO mice in vivo by injecting RANKL, which was shown to activate osteoclasts leading to preferential expansion and mobilization of immature cells (16). RANKL stimulation in WT mice increased the development of tartrate-resistant acid phosphatase–positive (TRAP⁺) osteoclasts along the endosteum of the trabecular bone, as previously shown (16). However, no increase in TRAP⁺ osteoclasts was observed in the CD45KO bones (unpublished data). We next tested progenitor cell levels in response to RANKL stimulations for 3 and 5 d. Immature WT progenitors and primitive SKL cells (Fig. 4, A and B, respectively) were expanded in the BM in response to RANKL stimulation, which was contrary to CD45KO cells. Levels of progenitors in the periphery of WT mice, such as the spleen (Fig. 4 C) or PB (Fig. 4 D), were increased, indicating progenitor mobilization. In contrast, CD45KO progenitors were not mobilized by RANKL stimulation for 3 d, and only at moderate levels after 5 d. Next, deeper investigations concerning the degradation of niche components were taken. We found only minor accumulation of soluble SCF in the PB of CD45KO mice in contrast to their WT counterparts (Fig. 4 E). Close examination of the trabecular endosteum, enriched with stem cell niches, demonstrated that in comparison to the WT BM, the niche component osteopontin was poorly degraded in CD45KO bone-lining osteoblasts after RANKL administration for both 3 and 5 d (Fig. 4 F). A broader examination of the entire BM showed a clear osteopontin-degraded product in the fluids of the WT BM after both 3 and 5 d of RANKL treatment (Fig. 4 G). However, degradation products were below the detection levels in CD45KO BM fluids, suggesting impaired osteopontin degradation (Fig. 4 G). These results indicate possible defects in CD45KO osteoclasts, resulting in their impaired response to RANKL and poor release of immature cells from the BM.

View larger version (55K): [in this window] [in a new window] [Download PPT slide]   Figure 4. CD45KO mice show impaired progenitor mobilization and endosteal modulation induced by RANKL. (A) Colony-forming progenitor cells in the BM of WT and CD45KO mice after RANKL treatment for 3 d. Values indicate fold changes compared with control mice ± SE (*, P < 0.01). (B) The percentage of SKL primitive cells in the BM of WT versus CD45KO mice after treatment with RANKL for 3 or 5 d. Values indicate the fold changes compared with control mice ± SE (*, P < 0.02; **, P < 0.05). (C) Colony-forming progenitor cells in the spleens of WT and CD45KO mice after RANKL treatment. Values indicate fold changes compared with control mice ± SE (*, P < 0.01). (D) Numbers of colony-forming progenitor cells in the PB of WT and CD45KO mice after RANKL treatment for 5 d (±SE). (E) Soluble SCF levels in the plasma of WT and CD45KO, control, or RANKL-treated mice. Values indicate the fold change in plasma SCF compared with control mice ± SE (*, P < 0.05). (F) Immunoreactivity (brown) of osteopontin in femoral metaphyseal trabecules of WT and CD45KO, control, and RANKL-stimulated mice for 3 and 5 d. Black arrowheads indicate endosteal bone-lining osteoblasts. Bars, 20 µm. (G) Western blot analysis of an osteopontin-degraded product (32 kD) in BM superannuates of WT and CD45KO mice after RANKL treatments for 3 and 5 d.

View larger version (64K): [in this window] [in a new window] [Download PPT slide]   Figure 5. Defective maturation of CD45KO osteoclasts in vitro involving impaired expression of MMPs, DC-STAMP, and Src kinase. (A) BM-derived osteoclasts from WT (top) and CD45KO (bottom) mice immunolabeled for CD45 expression (green), and stained for polymerized actin (red) and nuclear DNA (blue). Bars, 20 µm. (B) TRAP staining (purple) of BM-derived WT (top) and CD45KO (bottom) osteoclasts. Bars, 200 µm. (C and D) Semiquantitative PCR analysis for DC-STAMP mRNA levels in WT and CD45KO BM-derived cells. (C) Representative PCR image. (D) Summary of four independent experiments showing the ratio between DC-STAMP and GAPDH mRNA expression (±SE; *, P < 0.01). (E) Conditioned medium of WT versus CD45KO BM-derived osteoclasts was tested for the activity of secreted MMP-9 in a gelatin zymography assay. (F) WT and CD45KO BM-derived osteoclasts cultured with or without G-CSF were immunolabeled for expression of MT1-MMP (green), and stained for polymerized actin (red) and nuclear DNA (blue). Bar, 10 µm. (G) TRAP staining (purple) of BM-derived WT (top) and CD45KO (bottom) osteoclasts cultured in vitro in the presence of DMSO vehicle (left) or the Src inhibitor PP2 (right). Bars, 200 µm. (H) Src activity assay for osteoclast precursors incubated with 1 µM PP2 or DMSO (ctrl) for 5 d. Values indicate the fold changes of WT control mice ± SE (indicated by a horizontal line), showing a representative experiment.

View larger version (62K): [in this window] [in a new window] [Download PPT slide]   Figure 6. Reduced osteoclast function in CD45KO mice is associated with elongated trabecular zone and irregular localization of progenitors. (A) Plasma levels of PYD indicating bone resorption in WT and CD45KO. (B) Plasma levels of osteocalcin in WT and CD45KO mice. Values represent the mean ± SE (*, P < 0.05). (C) Three-dimensional constructions of the distal femurs of WT and CD45KO mice. The red frame indicates the metaphyseal region, near the bone growing plates, and the yellow frame indicates a region 1 mm ahead toward the diaphysis (see Materials and methods). Bars, 2 mm. (D) TRAP staining of femoral bone sections. Osteoclasts stained in red (arrowheads) are shown along the metaphyseal trabecules (Tb). (E) The ratio between osteoclast surface and bone surface (Ocl.S/B.S). Data are presented as the percentage of WT cells ± SE (*, P < 0.05). (F–H) Flow cytometry analyses of BM immature Lin–/c-Kit+ progenitors (F), presented as the percentage of WT (mean ± SE), and the more primitive SKL stem cells. A representative FACS plot (G) and summary (H) indicate lower levels of these primitive cells in the BM of CD45KO mice. *, P < 0.01. (I) Flow cytometry analyses of spleen-derived immature Lin–/c-Kit+ progenitors, presented as the percentage of WT (mean ± SE). Numbers indicate higher levels of these primitive cells in the spleen of CD45KO mice, *, P < 0.01.

View larger version (21K): [in this window] [in a new window] [Download PPT slide]   Figure 7. Defective engraftment and reduced rapid mobilization in CD45KO chimeras. (A) Percentage of donor-derived WT cells in the BM of WT and CD45KO recipients. Shown is a summary of seven mice in each group (±SE; *, P < 0.01). Values demonstrate reduced engraftment levels in CD45KO hosts. (B) AMD3100-induced mobilization of donor WBCs in the PB of WT and CD45KO hosts. Values indicate fold change of mobilization index compared with PBS control mice (±SE). **, P < 0.05. (C) Rapid mobilization of WT and CD45KO donor cells. WT chimeric hosts were injected with PBS or AMD3100 and were tested for the presence of donor-derived cells in the PB. The mobilization index of specific lineages was tested, as indicated in the figure legend. Values indicate the fold change compared with PBS control mice, which are marked as a dashed line (mean ± SE). *, P < 0.01; ***, P = 0.07.

	DISCUSSION

Top ABSTRACT RESULTS DISCUSSION MATERIALS AND METHODS REFERENCES

BM-derived cells lacking CD45 have increased activation of β1 integrins and hyperinduction of adhesion properties, demonstrating that CD45 is a negative regulator of signaling cascades, inducing cell detachment and release. We found that Src kinase, the CD45 substrate, is a potential target by which CD45 regulates the migration of hematopoietic cells. Indeed, Src kinase inhibition enhanced CD45KO cell motility, demonstrating that Src activity is unbalanced in these cells. Several studies support the involvement of Src kinases in adhesion and motility properties. Src kinases were shown to regulate β1 and β2 integrins in different cells and cell lines (28, 36). Moreover, in mice deficient in members of the Src family, immature, hematopoietic Sca-1⁺ cells demonstrated increased homing (37), and primitive, BM-derived SKL cells showed enhanced G-CSF–induced mobilization that was associated with elevated MMP-9 and accelerated breakdown of vascular cell adhesion molecule 1 (38). In line with these studies, our results demonstrate the opposite effects when Src is hyperactive because of CD45 deficiency. Still, such fundamental defects in the motility of both CD45KO progenitors and maturing leukocytes strongly suggest that additional pathways are also imbalanced by the lack of CD45 function. This is especially apparent in the defective cell polarization in response to chemotactic signals of CD45KO c-Kit⁺ progenitors. Moreover, SDF-1 is considered as a survival factor for stem and progenitor cells (39). Thus, the impaired ability of immature CD45KO c-Kit⁺ cells to normally respond to SDF-1 stimulation may further explain their inferior retention in the BM.

Previously, we suggested that interactions between hematopoietic stem and progenitor cells with their BM microenvironment are mutual (5, 11). We further reveal that CD45 also plays a role in progenitor mobilization by regulating components of the BM microenvironment. Reduced progenitor expansion and release in response to RANKL activation in CD45KO mice was associated with impaired modulation of the stem cell niche regulating components osteopontin and SCF. Osteopontin was shown to negatively regulate and limit the number of endosteal stem cells (40, 41). The impaired degradation of osteopontin in the endosteum of RANKL-treated CD45KO mice may explain the low numbers and reduced expansion of progenitors and stem cells in their BM. In addition, it was previously shown that shedding of membrane-bound SCF by MMP-9 shifts stem cells from a quiescent to a proliferative state, enabling their release from the BM (9). The impaired resorption activity and the low secretion of MMP-9 by CD45KO osteoclasts may also contribute to the reduced progenitor expansion in the CD45KO BM, a prerequisite step for immature cell mobilization.

Osteoclasts derived from hematopoietic precursors in the BM of CD45KO mice show abnormal morphology and function both in vitro and in vivo, reflecting mild osteopetrosis. Of note, osteoclasts derived from precursors in the spleen exhibited the same defective phenotype (unpublished data), although the numbers of hematopoietic progenitors were higher in the CD45KO spleens. This demonstrates that the decreased osteoclast numbers are not caused by the lack of progenitor cells but rather an intrinsic defect in osteoclast differentiation. Our investigations further showed that CD45 regulates osteoclast formation via controlling Src kinase activity and DC-STAMP expression. In support of our findings, previous reports showed that osteoclasts derived from DC-STAMP^–/– mice were TRAP⁺ MNCs exhibiting a reduced bone-resorbing activity (17). Interestingly, DC-STAMP^–/– osteoclasts demonstrated enhanced Src expression, suggesting a link between these two regulators (17). Thus, our data propose a role for the CD45–Src axis in osteoclast fusion and maturation. In addition, low expression of MMPs in CD45KO osteoclasts showed that by regulating MMP-9 and MT1-MMP expression, CD45 is eventually involved in osteoclast motility and bone degradation activity (42, 43). These defects in osteoclasts may thus explain the poor mobilization observed in CD45KO mice. However, distinguishing between the environmental versus hematopoietic effects using chimera models revealed a parallel and perhaps additive impact of both compartments on progenitor retention and mobilization potentials.

The abnormal phenotype and activity of CD45KO osteoclasts are associated with lower numbers of trabecules in the femoral metaphysis, a region known to harbor stem cells (32). Mouse models of severe osteopetrosis exhibit extramedular hematopoiesis, demonstrating lower levels of stem and progenitors cells in the BM caused by several bone structure defects, and higher levels of progenitor cells in the spleen (33, 44). CD45KO mice demonstrated a similar phenotype of the primitive SKL pool size and location driven by multiple defects of both the CD45KO primitive cells and their osteoclast progeny. The reduction in CD45KO primitive cells in the BM is complementary to previous findings showing that Lyn^–/– mice (members of the Src kinase family) display higher numbers of primitive SKL cells in the BM (45), demonstrating the central role of the CD45–Src cascade in stem cell retention. Our findings indicate that stem and progenitor cells can modulate their CD45 expression and signaling via Src kinase, influencing their retention, survival, and motility. Moreover, CD45KO spleen progenitors, which are not directly influenced by osteoclasts, exhibited poor mobility and repopulation potentials, and an unusual distribution of these progenitors was observed between the spleen and the PB. However, previous studies showed that in normal settings, spleen progenitors reside in equilibrium with the blood, suggesting no barrier between these organs (46), as opposed to the BM (6, 46). Hence, progenitor accumulation in the spleen may also be affected by the impaired intrinsic ability of CD45KO spleen progenitors to traffic to the circulation. Additional factors may also be involved, including increased survival and/or proliferation of these progenitor cells in extramedullary locations such as the spleen.

Our results suggest that hematopoietic stem cells and their leukocyte progeny have dual CD45-mediated self-regulation modes: their motility, proliferation, and adhesion are autonomously and dynamically regulated. In addition to stem cell regulation by the niche, functional CD45 is needed for osteoclast development and activity, which indirectly affect hematopoiesis and the progenitor pool size via interactions with the bone and BM stromal cells. This notion of a dynamic cross talk between all components of the system is also supported by a recent study, which shows that primitive signaling lymphocyte activation molecule stem and progenitor cells can directly regulate osteoblast development (47). Collectively, our results reveal that hematopoietic stem and progenitor cells are involved in regulating their own levels and the dynamic BM microenvironment via their osteoclast progeny, which require modulated CD45 activity.

	MATERIALS AND METHODS

Top ABSTRACT RESULTS DISCUSSION MATERIALS AND METHODS REFERENCES

 
Mice.
All experiments were approved by the animal care committee of the Weizmann Institute. The experiments were performed on CD45 exon 6–deficient mice (provided by T. Mak, University of Toronto, Toronto, Canada), which were bred and maintained under defined flora conditions at the Weizmann Institute. Age- and sex-matched C57BL/6 (CD45.2) mice (Harlan) were used as a WT control. All mice used were 6–8 wk of age at the onset of the experiments.

Stress-induced mobilization.
Mice received a daily s.c. injection of 300 µg/kg G-CSF (Filgrastim; Roche) for 3 or 5 consecutive days and were killed 4–6 h after the last injection. Single injections of 12.5 mg/kg LPS (Escherichia coli serotype O111:B4; Sigma-Aldrich) were administrated i.p. Mice were killed 16 h after injection. 2 µg of mouse RANKL (R&D Systems) was injected into 5–6-wk-old WT and CD45KO mice, s.c. over the femur, twice a day for the first 3 d followed by 2 d of rest, or for 5 consecutive days.

Homing assay.
5 x 10⁶ mouse BM MNCs per mouse, or 2.5 x 10⁶ CD11b⁺ or c-Kit⁺ sorted cells per mouse, were prelabeled with CFSE dye (5 µM/10⁷ cells; Invitrogen) and i.v. injected into NOD/SCID mice. Recipient mice were killed after 3 h, and the number of CFSE⁺ cells that reached the BM and spleens of recipient mice was determined by FACS. The homing of progenitor cells was examined as previously described (48) and modified using spleen cells by injecting 20 x 10⁶ total spleen cells into lethally irradiated (600 cGy from a cesium source) NOD/SCID/β2^–/– mice. A fraction of the injected cells was plated in colony assays to quantify the number of injected CFU-Cs. Recipients were killed 18 h after injections, and fractions of BM and spleen (1–2 x 10⁶ cells) were plated in methylcellulose medium to find the numbers of functional CFU-Cs (progenitors) that lodged to these organs. Homing efficiency was calculated as the percentage of homed progenitors out of the number of injected CFU-Cs in total spleen or four bones.

Repopulation and rapid mobilization in chimera models.
Recipient C57BL/6 (CD45.2) or CD45KO (CD45.2) mice were irradiated (600 cGy from a cesium source) and injected 4 h later with 10⁶ total BM cells derived from B6.SJL donors (CD45.1). Alternatively, C57BL/6 recipients were transplanted with 1–10 x 10⁶ CD45KO BM or 10⁶ spleen-derived cells from B6.SJL or CD45KO mice. PBS (as a control) or 5 mg/kg AMD3100 (Sigma-Aldrich) was injected s.c into chimeric mice 5 wk after transplantation. Engraftment levels and mobilization of donor WBCs in the PB were evaluated 1 h after AMD3100 injections using different combinations of cell staining and were analyzed by FACS. B6.SJL cells in different hosts were detected by tracing CD45.1⁺ cells, followed by staining with anti–CD45.1-PE/CD45.2-FITC (eBioscience). Detection of CD45KO cells in C57BL/6 hosts was performed by staining with Lineage⁺/CD45.2 antibodies (eBioscience), evaluating donor cells as CD19⁺, CD11b⁺, and Gr1⁺, which are CD45^– cells. Mobilization index refers to the ratio between BM engraftment level and the amount of donor-derived cells in the circulation.

Colony-forming assay.
PB samples were subjected to Ficoll separation. Total BM and spleen cells or PB MNCs were seeded (1.5 x 10⁴, 5 x 10⁵, and 2 x 10⁵ cells/ml, respectively) in semisolid cultures, as previously described (15). Colonies were scored 7 d later under an inverted microscope (CK2; Olympus), applying morphological criteria.

Flow cytometry analysis.
Membrane expression of different molecules on mouse BM and PB MNCs was detected by flow cytometry, using one- or two-step staining procedures. CD45 expression was assessed with FITC anti–mouse CD45.2 (BD Biosciences). CD45 expression on lineage-specific populations was determined by double staining using anti–CD45-PE (BD Biosciences) and antibodies for lineage markers (CD4- and CD11b-FITC, and c-Kit–allophycocyanin; eBioscience). The percentage of SKL cells in the BM and PB was tested by staining MNCs, as previously described (16). Activated mouse β1 was detected by using anti-CD29 (clone 9EG7; BD Biosciences) and secondary PE–donkey anti–rat (Jackson ImmunoResearch Laboratories). After staining, cells were washed and analyzed on a FACSCalibur (Becton Dickinson) using CellQuest software.

Sorting for CD11b⁺ and c-Kit⁺ cells.
Total BM cells from untreated mice or mice treated with G-CSF for 5 d were stained using anti–CD11b-FITC and anti–c-Kit–APC. Cells were sorted to these two populations simultaneously using a FACSAria (Becton Dickinson). Cells were washed and tested applying in vitro and in vivo assays.

Migration assay.
Chemotaxis assays were performed in Costar transwells (6.5-mm diameter, 5-µm pore size; Corning). Upper filters were untreated (bare) or precoated overnight with 25 µg/ml FN at 4°C (Millipore). 10⁵ mouse BM MNCs were added to the upper filters and were allowed to migrate toward 50 ng/ml SDF-1 (PeproTech) for 2 h. Migrating cells were counted using a FACSCalibur. CD45KO BM MNCs were pretreated with 1 µM of the Src inhibitor PP2 (EMD), or as a control with the PP2 solvent DMSO for 30 min at 37°C. The cells were then washed and submitted to migration toward 50 ng/ml SDF-1 and analyzed as described.

Cell polarization microscopy images.
Response to 200 ng/ml SDF-1 of c-Kit⁺–sorted cells was observed using a 40x objective (NA = 1.35; Olympus) on uncoated µ slides (Integrated BioDiagnostics). Phase-contrast images were acquired using scientific-grade charge-coupled device (CCD) camera (LIS-700; Applitech) and processed by the DeltaVisionRT system using SoftWoRx software (Applied Precision).

Adhesion assay.
96-well plates were coated by overnight incubation with 25 µg/ml FN at 4°C, washed with PBS, and blocked with 0.1% BSA. 2.5 x 10⁵ WT or CD45KO BM MNCs per well were allowed to adhere to the plates for 16 h at 37°C in serum-free RPMI 1640. Nonadherent cells were washed twice in PBS. Adherent cells were collected in 200 µl PBS buffer plus 0.5 mM EDTA. The number of adherent cells was determined by FACS analysis using a FACSCalibur.

MMP-9 zymography.
Zymography assay was performed as previously described (4), with the following modifications. BM and PB MNCs were incubated in vitro at 37°C (10⁵ cells per 100 µl of serum-free RPMI 1640) for 40 h. For measurement of osteoclast-secreted MMP-9, total BM cells were cultured with M-CSF and RANKL, as previously described (16). The resulting conditioned medium was collected and loaded (10 µl) on 10% SDS-PAGE gels containing 1 mg/ml gelatin.

Immunoblotting.
Whole-cell lysates were prepared from BM MNCs of WT or CD45KO mice, intact or after G-CSF injections for 3–5 d. Lysates were obtained by a 15-min incubation with modified RIPA buffer (20 mM Hepes [pH 7.3], 150 mM NaCl, 10% glycerol, 0.1% SDS, 1% Triton X-100, 2 mM EDTA, 2 mM EGTA, 0.5% deoxycholate, 50 mM βGP, and 50 mM NaF) freshly supplemented with 1% protease inhibitor cocktail (Sigma-Aldrich) and 0.2 mM pervanadate (Sigma-Aldrich). 50 µg of total protein was separated on 10% SDS-PAGE and transferred to nitrocellulose membranes. The membranes were blocked with TBST (5 mM Tris, 154 mM NaCl, 0.1% Tween-20 [pH 7.6]) containing 5% milk and probed with rabbit anti–human/mouse phospho-Src (Invitrogen), rabbit anti–human/mouse ERK1 (pThr²⁰²/pTyr²⁰⁴) and ERK2 (pThr¹⁸⁵/pTyr¹⁸⁷; Sigma-Aldrich), or rabbit anti–total ERK1/2 (Sigma-Aldrich), as a control for total protein. Osteopontin expression was evaluated in BM superannuates, separated on 10% SDS-PAGE (20 µg). Polyclonal anti–mouse osteopontin antibodies (R&D Systems) were used to detect the 32-kD degraded product, as previously described (49).

Src activity assay.
Whole-cell lysates were prepared from BM MNCs and sorted CD11b⁺ cells. Alternatively, lysates were prepared from osteoclast precursors grown for 5 d in the presence of RANKL and 20 ng/ml M-CSF supplemented with 1 µM PP2 or DMSO vehicle. Lysis was performed using HNTG lysis buffer (20 mM Hepes [pH 7.5], 150 mM NaCl, 1% Triton X-100, 10% glycerol, 1 mM EDTA, 1 mM EGTA, 50 mM NaF) freshly supplemented with 1% protease inhibitor cocktail, 0.2 mM pervanadate, and 0.5 mM okadaic acid (A.G. Scientific). Src kinases were immunoprecipitated by incubating cell lysates with 1 µg of anti–v-Src antibodies (EMD) for 2 h at 4°C. Protein G plus agarose beads (Santa Cruz Biotechnology, Inc.) were added to the mixture and incubated for an additional 12 h at 4°C. Immunocomplexes were precipitated after three washes with HNTG wash buffer (20 mM Hepes [pH 7.5], 150 mM NaCl, 0.1% Triton X-100, 10% glycerol, 1 mM EDTA, 1 mM EGTA, 50 mM βGP, 50 mM NaF, 1 mM sodium orthovanadate) and a final wash with Src kinase buffer (20 mM MOPS, 5 mM MgCl₂). Src kinase activity was tested using a tyrosine kinase activity assay kit (Millipore) according to the manufacturer's instructions. Src activity in BM samples was calculated in correlation to the total amount of Src that was precipitated in each sample stated by immunoblot assay.

µCT imaging and trabecular morphometry.
Femurs from CD45KO and WT control mice were removed, disarticulated from the pelvic bone and tibia, cleaned of soft tissues, and stored at –20°C. After thawing at room temperature, bones were scanned using a µCT device (eXplore Locus SP; General Electric) with custom software (version 5.2.2; MicroView). Scanning was performed with 80-kV x-ray voltage, 80-µA current, 400-ms integration time, and 8-µm pixel size. Based on preliminary work, two volumes of interest (VOI) were defined (Fig. 6 C). The first VOI consisted of the distal metaphyseal region, defined as starting at a distance of 32 image slices (250 µm) from the growth plate in the direction of the diaphysis, and extending a further 220 slices (1.75 mm) in the same direction. The second proximal metaphyseal VOI started from the end of the previous VOI and extended a further 125 slices (1 mm) in the same direction. The trabecular volume was separated from the surrounding cortical shell by manual segmentation, and a direct three-dimensional model (50) was used to evaluate the Tb.N.

Osteoclast immunocytochemical staining.
Total BM cells were seeded on glass cover-slips (10⁶ cells/1 ml) and cultured for 6 d in -MEM supplemented with 20 ng/ml M-CSF (PeproTech) and RANKL that were changed every other day. Where indicated in the figures, culture medium was supplemented with 200 ng/ml G-CSF (Filgrastim; Roche). Samples were fixed with 3% paraformaldehyde (Merck), permeabilized with 0.5% Triton X-100 (Sigma-Aldrich), and immunolabeled at room temperature in a humidified chamber with FITC-conjugated anti-CD45.2 (eBioscience) or rabbit anti–mouse/human MT1-MMP polyclonal antibody (Millipore), followed by secondary goat anti–rabbit–Alexa Fluor 488. TRITC-phalloidin and DAPI (Sigma-Aldrich) were added. Images were acquired using scientific-grade CCD camera and processed by the DeltaVisionRT system using SoftWoRx software.

TRAP staining of bone sections and osteoclasts.
TRAP staining of bone sections and osteoclasts was performed as previously described (16). For osteoclast formation in vitro, BM cells were seeded in 96-well plates (10⁵ cells/0.2 ml) and cultured with M-CSF and RANKL, as previously described (16). In some experiments, the culture medium was supplemented with 1 µM of the Src inhibitor PP2 or its vehicle DMSO in the respective concentration.

Immunohistochemistry of osteopontin and SDF-1.
Bone sections were prepared and stained as previously described (16).

ELISA for mouse SCF.
Blood plasma samples were obtained from control and RANKL-treated mice and tested for SCF by ELISA, as previously described (16).

ELISA for PYD and osteocalcin.
We tested plasma PYD (Metra; Quidel Corp.) and osteocalcin (Biomedical Technologies, Inc.) on frozen plasma samples according to the manufacturers' instructions.

Semiquantitative RT-PCR for DC-STAMP.
We prepared cDNA from mouse BM cells using standard protocols. We performed semiquantitative PCR analysis for DC-STAMP expression for 35 cycles: 95°C for 1 min, 60°C for 1 min, and 72°C for 1 min. We used the following primer sequences: 5'-GGGTCTCAACACCACGAACT-3' and 5'-GACTCTGTTTGCCCAGCTTC-3' (251 bp).

Statistical analysis.
Significance levels of the data were determined by the Student's t test using Microsoft Excel.