Introduction

β-catenin is a central molecule in the canonical wingless/integrated (Wnt) pathway. When Wnt ligands interact with Frizzled and low-density lipoprotein receptor-related protein 5 and 6 co-receptors, β-catenin is activated, accumulated in the cytoplasm, and translocated into the nucleus. In the nucleus, β-catenin activates transcription of downstream genes. β-catenin signaling plays important roles in bone development, postnatal bone growth, and bone remodeling. Animal studies, in which the β-catenin signaling was either inhibited or activated in chondrocytes, osteoblasts, or osteocytes, demonstrated that activation of β-catenin signaling promotes osteoblast differentiation and bone formation and inhibition of osteoclast formation and bone resorption.1,2,3,4,5,6,7 However, the detailed mechanisms of how postnatal bone growth and bone remodeling are regulated by β-catenin signaling remain unclear.

The β-catenin signaling in mesenchymal stem cells (MSCs) promoted osteoblast differentiation, inhibited chondrocyte differentiation, and enhanced endochondral ossification.8,9 For example, deletion of LRP6, the co-receptor of Wnts, in nestin-expressing cells caused bone mass decrease.10 In addition, β-catenin signaling in mature osteoblasts inhibits osteoclast formation.11,12,13 Activation of β-catenin signaling also prevented osteoblast apoptosis.14 In contrast, the function of β-catenin signaling in osteoblast precursor cells has not been fully investigated.

Without Wnt ligands interacting with the cell surface receptors, cytoplasmic β-catenin is degraded by the ubiquitin–proteasome system, mediated by the destruction complex in a phosphorylation-dependent manner. Axin1 and Axin2 are scaffolding proteins in the destruction complex and promote β-catenin phosphorylation and degradation. Upon Wnt ligand binding to Wnt receptors on the cell surface, the destruction complex is dissociated and β-catenin is then released from the destruction complex and subsequently translocated into the nucleus.

Several in vivo studies were conducted to determine the role of the β-catenin destruction complex in bone development.15,16,17 For example, Axin2 KO mice showed craniosynostosis and significantly increased trabecular bone mass.18,19 Mice lacking APC, a member in destruction complex, in osteoblasts exhibited dramatically increased bone deposition.11 Axin1 is also a scaffold protein in the destruction complex and is the negative regulator of β-catenin signaling.15,17 Axin1 was expressed ubiquitously, and the systematic deletion of Axin1 led to early embryonic lethality in mice.20 Therefore, exact functions of Axin1 at different differentiation stages during MSC differentiation have not been investigated due to the limitation of the lethality of conventional deletion of Axin1.

To determine the potential role of Axin1 in osteoblast precursor cells at postnatal stage during bone remodeling, we generated Axin1flox/flox mice21 and bred these mice with Osx-Cre mice to produce Axin1Osx conditional KO mice. We found that loss of Axin1 in osteoblast precursor cells mainly affects osteoclast formation in metaphyseal bone area.

Results

Increased expression of β-catenin in Axin1Osx KO mice

To delete Axin1 in osteoblasts, primary osteoblasts isolated from calvariae of Axin1flox/flox mice were infected with adenovirus-Cre recombinase. We found that Axin1 mRNA and protein expressions were significantly decreased in calvarial osteoblasts isolated from Axin1flox/flox mice infected with Adeno-Cre (Fig. 1a, b). In contrast, β-catenin expression was increased in these cells (Fig. 1b). We then bred Axin1flox/flox mice with Osx-Cre mice and generated Axin1Osx KO mice. We found that Axin1 expression was decreased while β-catenin expression was significantly increased in trabecular bone of tibiae of Axin1Osx KO mice (Fig. 1c). In addition, we detected Axin1 and β-catenin expression in adipocytes and perivascular cells in the bone marrow. We found that Axin1 expression was decreased while β-catenin expression was significantly increased in adipocytes (Fig. 1d). However, we did not observe obvious changes in Axin1 and β-catenin expression in perivascular cells (Fig. 1d). We also examined changes in Wnt inhibitors by determining the expression of Dkk1 and sclerostin in trabecular bone and found that expression of both Dkk1 and sclerostin was upregulated in trabecular bone area below the growth plate in Axin1Osx KO mice (Fig. 1e, f). To determine changes in skeletal structure, newborn Axin1Osx KO mice and their littermate controls were collected and performed whole body Alizarin red/Alcian blue staining. We did not observe significant changes in skeletal structure in Axin1Osx KO mice (Fig. 1g). In contrast, slightly delayed mineralization of calvarial bone was observed in newborn and 4-week-old Axin1Osx KO mice (Fig. S1).

Fig. 1
figure 1

Increased β-catenin expression in Axin1Osx (KO) mice. a Axin1 expression was significantly decreased in Axin1flox/flox calvarial osteoblasts infected with Adeno-Cre (n = 3, **P < 0.01). b In Axin1flox/flox calvarial osteoblasts infected with Adeno-Cre, Axin1 protein expression was significantly decreased while active β-catenin levels were increased. c Results of IHC showed that Axin1 expression (blue arrowheads) was significantly decreased and β-catenin expression (red arrowheads) was significantly increased on the surface of trabecular bone of newborn Axin1Osx KO mice. d Expression of Axin1 and β-catenin in perivascular cells (red arrowheads) and in adipocytes (green arrowheads) in bone marrow was analyzed by IHC method. e, f Expression of DKK1 (red arrowheads) and Sclerostin (blue arrowheads) in trabecular bone was analyzed by IHC method. g Newborn Axin1Osx KO mice and Cre-negative littermates were collected and whole skeletal Alizarin red/Alcian blue staining was performed. No significant changes in skeletal structure in Axin1Osx KO mice are seen

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Delayed endochondral bone growth in Axin1Osx KO mice

We performed histological analyses and observed an expanded hypertrophic zone in tibial growth plates of newborn and 1-week-old Axin1Osx KO mice (Fig. 2a, d). In newborn Axin1Osx KO mice, the length of the hypertrophic zone is almost three times longer than that of Cre-negative mice (Fig. 2a). New bone formation in the primary ossification center was delayed in newborn Axin1Osx KO mice (Fig. 2b). In 1-week-old Axin1Osx KO mice, the length of the hypertrophic zone of Axin1Osx KO mice was significantly longer compared with that of Cre-negative controls (Fig. 2d). Large amounts of uncalcified bone with accumulated osteoid were found in the trabecular bone area below the growth plate (Fig. 2e), suggesting defects in bone remodeling in Axin1Osx KO mice. To determine if these changes are due to activation of β-catenin signaling and to compare the difference between Axin1Osx KO mice and β-catenin conditional activation mice, we generated and analyzed newborn and 1-week-old β-catenin(ex3)Osx activation mice. Compared with Axin1Osx KO mice, we did not observe obvious expansion of hypertrophic cartilage in β-catenin(ex3)Osx activation mice (Fig. 2c, f). These findings suggest that Axin1 may also act through a β-catenin-independent mechanism to regulate postnatal bone growth. In 2-week-old Axin1Osx KO mice, we observed a slightly delayed formation of a secondary ossification center (Fig. 2g). In contrast, the formation of secondary ossification centers were significantly delayed in β-catenin(ex3)Osx activation mice (Fig. 2h). In 4-week-old mice, it seems that growth plate cartilage development and the formation of a secondary ossification center were normal in Axin1Osx KO mice (Fig. 2i) or in β-catenin(ex3)Osx activation mice (Fig. 2j). Results of IHC analyses showed that extensively increased Col-X-positive hypertrophic chondrocytes were found in the metaphyseal bone area of newborn Axin1Osx KO tibiae (Fig. 2k). Similarly, extensively increased MMP13-positive cells were also found in the expanded hypertrophic zone (Fig. 2l). This phenotype was 100% penetrated in Axin1Osx KO mice.

Fig. 2
figure 2

Delayed postnatal bone growth in Axin1Osx KO mice. a, d Results of Safranin O/Fast green staining revealed an expanded hypertrophic zone (yellow bars) in tibial growth plates of newborn and 1-week-old Axin1Osx KO mice compared with those of Cre-negative littermates. b Results of Alcian blue/Hematoxylin Orange G (AB/HO) staining showed that formation of a primary ossification center was delayed in newborn Axin1Osx KO mice (red arrow). e Results of Alcian blue staining showed that trabecular bone with large amounts of uncalcified osteoid (red arrowheads) was found in 1-week-old Axin1Osx KO mice. c, f No significant changes in the length and morphology of growth plate cartilage were seen in newborn and 1-week-old β-catenin(ex3)Osx activation mice compared with their Cre-negative littermates. g, h Results of Alcian blue staining showed a slightly delayed formation of a secondary ossification center in 2-week-old Axin1Osx KO mice. In contrast, a significantly delayed formation of a secondary ossification center (red arrow) was found in 2-week-old β-catenin(ex3)Osx activation mice. i, j Results of Alcian blue staining histology showed relatively normal hypertrophic cartilage development in 4-week-old Axin1Osx KO mice and in 4-week-old β-catenin(ex3)Osx activation mice. k, l Results of IHC showed that collagen type X (Col-X)-positive hypertrophic chondrocytes (HC) (red arrowheads) and MMP13-positive hypertrophic chondrocytes (blue arrowheads) were found in the metaphyseal bone area and in the middle of the bone marrow cavity of newborn Axin1Osx KO tibiae

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Impaired osteoclast formation in Axin1Osx KO mice

Osteoclasts in growth plate can phagocytose dying hypertrophic chondrocytes and absorb the mineralized cartilage matrix. Therefore, we analyzed changes in osteoclast formation in Axin1Osx KO mice. In newborn Cre-negative tibiae, large numbers of TRAP-positive osteoclasts were found on the metaphyseal bone area and the inner side of cortical bone (Fig. 3a). In addition, osteoclasts were also found in the ossification front, where osteoclasts invaded hypertrophic chondrocytes (Fig. 3a, lower left panel). In newborn Axin1Osx KO tibiae, TRAP-positive osteoclasts in the bone marrow cavity and ossification front were significantly decreased (Fig. 3a, right panel). Osteoclast formation in the subchondral bone of 2- and 4-week-old Axin1Osx KO tibiae was also decreased compared with that of Cre-negative tibiae (Fig. 3b). Quantification of the ratios of osteoclast numbers and trabecular bone perimeters showed reduced TRAP-positive osteoclast numbers in 4-week-old Axin1Osx KO mice (Fig. 3c). Real-time PCR and IHC results also showed decreased expression of osteoclast markers, MMP9 (Fig. 3d, e) and cathpesin K (Fig. 3f, g) in both subchondral bone and metaphyseal bone of 4-week-old Axin1Osx KO tibiae. By contrast, no obvious changes in osteoblast numbers were found in the metaphyseal bone of same-aged Axin1Osx KO mice (Fig. 4a, b). Results of calcein labeling and quantification of mineral appositional rates (MAR) showed that bone formation of cortical bone was not significantly changed in Axin1Osx KO mice (Fig. 4c, d).

Fig. 3
figure 3

Decreased osteoclast formation in Axin1Osx KO mice. a In newborn Cre-negative tibiae, TRAP-positive osteoclasts were found on metaphyseal bone surfaces (yellow arrowheads), the inner region of cortical bone (blue arrowheads) and the ossification front (red arrowheads). In newborn Axin1Osx KO tibiae, TRAP-positive osteoclasts in the bone marrow cavity and ossification front were significantly decreased. b TRAP-positive osteoclasts were decreased in the subchondral bone area of 2- and 4-week-old Axin1Osx KO tibiae. c Osteoclast numbers were quantified. The results showed significantly reduced osteoclast numbers, normalized to trabecular bone perimeters, in the subchondral bone of 4-week-old Axin1Osx KO mice compared with those of Cre-negative mice (n = 4, **P < 0.01). dg Real-time PCR and immunohistochemistry (IHC) data showed decreased mRNA and protein expressions of MMP9 (red arrowheads) and cathepsin K (purple arrowheads) in subchondral bone (middle panel) and metaphyseal bone (lower panel) of 4-week-old Axin1Osx KO tibiae. (n = 4, *P < 0.05)

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Fig. 4
figure 4

No significant change in the bone formation in Axin1Osx KO mice. a Hematoxylin and eosin (HE) staining of trabecular bone in the metaphyseal area of 4-week-old Axin1Osx KO mice and Cre-negative controls. b Quantification of osteoblast numbers showed no significant changes in osteoblast numbers in trabecular bone in the metaphyseal area of 4-week-old Axin1Osx KO mice (n = 6). c, d Results of calcein labeling and the measurement of mineral appositional rates (MAR) showed cortical bone formation was slightly reduced in 4-week-old Axin1Osx KO mice (n = 6)

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Increased Opg expression in Axin1Osx KO mice

The ratio of Opg/Rankl is an important index reflecting changes in osteoclast formation. In the tibiae of Cre-negative mice, osteoprotegerin (OPG)-positive staining cells were observed on the trabecular bone surface (Fig. 5a). In Axin1Osx KO mice, the number and staining intensity of OPG-positive cells were significantly increased in Axin1Osx KO mice, especially on the trabecular bone surface (Fig. 5a). Osteoblasts are the important cell resource for OPG production and osteoblast precursor cells are the Osterix-expressing cells. Therefore, we examined changes in Opg and Rankl expression in primary calvarial osteoblasts of newborn Axin1Osx KO mice and Cre-negative littermate controls. In calvarial osteoblasts of newborn Axin1Osx KO mice, though both Opg and Rankl expressions were increased (Fig. 5b, c), the Opg:Rankl ratio was still significantly higher in Axin1-deficient osteoblasts than that of control osteoblasts (Fig. 5d). We then cultured wild-type (WT) bone marrow derived macrophages (BMM) cells treated with the conditioned media (CM) collected from primary osteoblasts isolated from Axin1Osx KO mice and Cre-negative mice, respectively. Osteoclast formation in the BMM cells treated with CM collected from osteoblasts of Axin1Osx KO mice was obviously decreased compared with the cells treated with CM collected from control osteoblasts (Fig. 5e). These findings were further confirmed by the results of osteoclast quantification (Fig. 5f). Nuclear factor of activated T-cells, cytoplasmic 1 (NFATc-1) and c-Fos are two key regulators of osteoclast differentiation upon receptor activator of nuclear factor kappa-Β ligand (RANKL) induction. Real-time PCR assay revealed that expression of Nfatc-1 and c-Fos was decreased in trabecular bone of Axin1Osx KO mice (Fig. 5g, h). IHC assays further demonstrated that NFATc-1- and c-Fos-expressing cells were detected in trabecular bone, and that NFATc-1 was especially highly expressed in the ossification front of the tibiae in control mice (Fig. 5i, j). The numbers of NFATc-1 and c-Fos positive cells were significantly decreased in the tibiae of Axin1Osx KO mice (Fig. 5i, j).

Fig. 5
figure 5

Alterations of OPG, NFATc-1, and c-Fos expression in Axin1Osx KO mice. a Results of IHC staining showed that more osteoprotegerin (OPG)-positive cells were observed in 4-week-old Axin1Osx KO mice, especially on the surface of trabecular bone (red arrowheads). bd In calvarial osteoblasts isolated from newborn Axin1Osx KO mice, both Opg and Rankl expression was increased, and the ratio of Opg/Rankl was significantly higher in bone marrow stromal (BMS) cells derived from Axin1Osx mice than that of Cre-negative mice (n = 4, **P < 0.01). e WT BMM cells were cultured with the conditioned medium (CM) collected from cultured calvarial osteoblasts of 4-week-old Axin1Osx KO mice and Cre-negative littermates, respectively. Osteoclast formation in the cells cultured with CM from the Axin1Osx KO calvarial cells was significantly decreased compared with that in the cells cultured with CM collected from Cre-negative osteoblasts. f Quantification results showed decreased osteoclast numbers in the Axin1Osx KO group (n = 6, **P < 0.01). g, h The total RNA was extracted from tibia of 4-week-old Cre-negative and Axin1Osx KO mice and Nfatc-1 and c-Fos mRNA expression was detected by real-time PCR (n = 4, **P < 0.01). i, j In tibiae of 4-week-old Axin1Osx KO mice, NFATc-1-positive staining cells (brown arrowheads) and c-Fos-positive staining cells (purple arrowheads) were decreased compared with those of Cre-negative control mice

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Discussion

Osterix is the osteoblast specific transcription factor that regulates osteoblast precursor cell differentiation and inhibits cell proliferation.22,23 In Osx-expressing osteoblast precursor cells, Wnt/β-catenin signaling activation is at a low level. Osx-Cre targeting cells were established by breeding Osx-Cre mice with ROSAmT/mG reporter mice, followed by fluorescence microscopic analysis. Osx-Cre targeting cells were detected in trabecular bone and on the endosteal region of cortical bone; they were especially highly expressed in the area of metaphyseal bone that is close to the growth plate hypertrophic cartilage area.22 Consistent with these findings, when Axin1 expression was inhibited in osteoblast precursor cells using Osx-Cre transgenic mice, β-catenin-positive staining cells were also detected in trabecular bone and on the endosteal region of the cortical bone.

In this project we discovered that deletion of Axin1 in osteoblast precursor cells led to β-catenin upregulation, which further resulted in increased OPG expression. Increased OPG expression could inhibit osteoclast formation, which may be responsible for the reduction of apoptosis in hypertrophic chondrocytes and decreased resorption of mineralized cartilage matrix. Wnt/β-catenin signaling controls osteoblast and osteoclast differentiation and regulates bone mass.24,25 In our study, osteoblast numbers and bone mass were not significantly changed in Axin1Osx KO mice. In contrast, osteoclast formation was dramatically decreased when Axin1 was deleted in Osx-expressing osteoblast precursor cells. In Axin1Osx KO mice, β-catenin levels were increased in osteoblast precursor cells. It is known that inhibition of β-catenin signaling causes an increase in chondrocyte apoptosis during postnatal cartilage development.26 β-catenin, together with TCF proteins, regulates Opg expression in osteoblasts.12 Loss of β-catenin in mature osteoblasts resulted in a decreased ratio of OPG/RANKL, while accumulation of β-catenin signaling led to an increased ratio of OPG/RANKL.11,12,13 OPG is a decoy receptor that prevents RANKL/RANK interaction and inhibits osteoclast differentiation.27,28,29 Therefore, activation of β-catenin signaling in mature osteoblasts resulted in a decrease in osteoclast formation, while inhibition of β-catenin signaling caused an increase in osteoclast formation leading to severe osteopenia.11,12,13 In addition, β-catenin signaling in chondrocytes could also regulate osteoclast formation and bone resorption through regulation of OPG expression.30 In this report, we have demonstrated that deletion of Axin1 in osteoblast precursor cells led to upregulation of β-catenin signaling, increased the ratio of OPG/RANKL and prevented osteoclast formation. We also found that Rankl expression in primary calvarial osteoblasts of Axin1Osx mice was also upregulated. This is not consistent with previous reports that β-catenin signaling downregulated Rankl expression in a glucocorticoid receptor-dependent manner.27 This discrepancy may be due to the possibility that Axin1 may also affect other signaling molecules in addition to that of β-catenin. In fact, comparing differences in the histological results of newborn, 1-week-old and 2-week-old Axin1Osx KO mice with those of β-catenin(ex3)Osx activation mice, the phenotypes of the expanded hypertrophic zone and formation of the secondary ossification center are very different between Axin1 KO mice and β-catenin activation mice, suggesting that Axin1 may also act through a β-catenin-independent mechanism to regulate postnatal bone growth.

During the endochondral bone formation process, hypertrophic chondrocytes in the growth plate undergo apoptosis and the mineralized cartilage matrix was absorbed, followed by bone formation. At the ossification front, hypertrophic chondrocytes directly contact with osteoclasts. Findings with annexin-V labeling confirmed that osteoclasts could remove dying chondrocytes by phagocytosis.31 Meanwhile, osteoclasts are also capable of absorbing the mineralized cartilage matrix.32,33 Mice lacking TRAP resulted in an expanded hypertrophic zone and disordered hypertrophic chondrocyte columns that extended into the trabecular bone region.34 Mice lacking RANK showed an even more severe phenotype of an expanded hypertrophic zone. The bone marrow cavity was almost filled with unabsorbed cartilage.35,36 In Axin1Osx KO mice, we also found an expanded hypertrophic zone and unabsorbed cartilage in the bone marrow cavity, which may be caused by decreased osteoclast formation. Meanwhile, large numbers of Col-X-positive prehypertrophic and hypertrophic chondrocytes and MMP13-expressing terminally differentiated hypertrophic chondrocytes were found in the expanded hypertrophic zone of the growth plate as well as in the bone marrow cavity. This suggests that the terminal apoptosis of chondrocytes was inhibited or delayed due to the loss of Axin1 in osteoblast precursor cells. Although Osterix was also detected in a subset of chondrocytes,37,38 in Axin1Osx KO mice, β-catenin upregulation was found in the chondrocytes located in the upper part of the proliferative zone, but not in the hypertrophic zone. However, the phenotypes of the expanded hypertrophic zone and unabsorbed cartilage matrix observed in Axin1Osx KO mice may not be primarily caused by the alteration of β-catenin signaling in hypertrophic chondrocytes. The evidence that the phenotype of the expanded hypertrophic zone was not observed in β-catenin activation mice further suggest that the phenotype observed in early postnatal Axin1 KO mice was not caused by the activation of β-catenin signaling. The detailed mechanism of Axin1 regulation of postnatal bone growth needs to be further investigated.

In conclusion, loss of Axin1 in osteoblast precursor cells led to activation of β-catenin signaling, which in turn upregulated OPG expression and increased the ratio of OPG/RANKL. Osteoclast formation was then inhibited by OPG, which is responsible for decreased apoptosis of hypertrophic chondrocytes and reduced resorption of the mineralized cartilage matrix. However, it is not totally clear whether only a small portion of osteoblast precursor cells was affected leading to the changes in β-catenin signaling in those cells. This possibility needs to be further investigated.

Materials and methods

Animals

The use of animals was approved by Shanghai Laboratory Animal Use Committee. The generation of Axin1flox/flox mice has been reported in previous studies.21 Osx-Cre mice were obtained from the Jackson Laboratory. Axin1Osx conditional KO mice were generated by crossing Axin1flox/flox mice with Osx-Cre transgenic mice (Osx-Cre;Axin1flox/flox). β-catenin(ex3)flox/- mice have been used in our previous studies.30,39

Isolation and culture of calvarial osteoblasts

The periosteal layers on both sides of the skull of 3-day-old mice were removed. The calvariae were transferred into a 50 mL conical tube and digested in 1 mg·mL−1 collagenase A (Roche, Basel, Switzerland) in serum-free αMEM in a 37 °C water bath for 15 min. After two repeated digestions in fresh collagenase A solution, the retained mixtures of collagenase A and cells were filtered into a new tube. The cell suspensions were mixed, centrifuged, and resuspended in αMEM with 10% FBS and 50 μg·mL−1 ascorbic acid. The suspension was finally plated in six-well culture plates at a density of 2 × 105 cells per well. The media were changed every other day.

Adenovirus mediated deletion of Axin1 in primary calvarial osteoblasts

Primary osteoblasts were isolated from calvariae of Axin1flox/flox mice and cultured in αMEM with 10% FBS in six-well plates. When cells reach 40% density, Adeno-Cre or Adeno-GFP (Hanbio, Shanghai, China) was added to the culture medium at a concentration of 2 × 108 plaque-forming unit (PFU) per mL. The culture medium was changed 24 h after infection. The cells were collected 40 h after virus infection for real-time PCR and western blot assays.

Real-time PCR assay

Total RNA was extracted from primary calvarial osteoblasts using a RNeasy mini kit (Qiagen, Hilden, Germany). DNAse I-treated total RNA was reverse transcripted using a RT reagent kit (Takara Bio, Tokyo, Japan). The cDNA was amplified by PCR in a total volume of 20 μL reaction solution containing 10 pmol·L−1 primers (primer names and sequences are listed in Table 1).

Table 1 Names and sequences of PCR primers
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Whole skeleton Alizarin red and Alcian blue staining

After removing skin and adipose tissues, the skeletons were fixed in 95% ethanol for 2 days followed by fixation in acetone for another day. The skeletons were then stained with 0.015% Alcian blue and 0.005% Alizarin red for 3 days. Pictures were taken after most of the soft tissue was digested in 1% potassium chloride solution.

Histological analysis

Tibial samples were fixed in 4% paraformaldehyde, decalcified, dehydrated, and embedded in paraffin. 4-μm thick serial midsagittal sections of tibias were cut and stained with Alcian blue/HEG (ABH) and Safranin O/Fast green (SOF). Histomorphometric analysis was performed using an Olympus BX50 microscope (Olympus, Tokyo, Japan) and Image-Pro Express software (Media Cybernetics, Rockville, MD, USA). TRAP-positive osteoclast numbers were quantified.

Calcein labeling assay

1 mg·mL−1 calcein in saline was injected into 3-week-old mice (i.p. injection, 10 mg·kg−1) followed by a second injection 4 days later. Tibiae of 4-week-old mice were fixed in 4% paraformaldehyde and dehydrated in a series of ethanol (75%–100%). Samples were embedded in methyl methacrylate and 100-μm thick serial midsagittal sections were cut. The fluorescence signal of the cortical bone was observed using an Olympus BX50 microscope (Olympus). The distances of two calcein labels were measured with DP Manager software (Olympus) to determine the MAR.

TRAP staining

Paraffin sections of newborn, 2- and 4-week-old tibias were rehydrated and incubated with a 0.4 mg·mL−1 Napthol-Ether solution/basic stock incubation solution at 37 °C for 30 min. A 0.04 g·mL−1 sodium nitrite solution and a 0.05 g·mL−1 pararosaniline dye/2 N hydrochloric acid solution was mixed and added to the basic stock incubation solution and the paraffin sections were incubated in this mixture for 10 min.

Immunohistochemistry (IHC) staining

Paraffin sections of 4-week-old tibiae were rehydrated and digested in 0.1% trypsin for 10 min at the room temperature, and then treated with 3% H2O2 for 20 min. Sections were incubated with primary antibodies in PBS overnight at 4 °C. Col-X, MMP13, MMP9, cathepsin K, OPG, DKK1, and sclerostin antibodies were obtained from Abcam (Cambridge, MA, USA). Axin1 and β-catenin antibodies were obtained from Sigma (St. Louis, MO, USA). NFATc-1 and c-Fos antibodies were obtained from Santa Cruz Biotechnology (Santa Cruz, CA, USA). Negative control sections were incubated with IgG (Beyotime Biotechnology, Shanghai, China). A Polink-2 plus polymer HRP detection kit (PV-9001, ZSGB-BIO, Shanghai, China) was used for incubation with secondary antibody and horseradish peroxidase (HRP)-streptavidin.

In vitro osteoclast differentiation assay

BMM cells were isolated from long bone of 1-month-old WT mice and plated into 24-well culture plates at a density of 4 × 105 cells per well and cultured in αMEM with 10% FBS. Cells were treated with 20 ng·mL−1 macrophage colony-stimulating factor (M-CSF) for 3 days, and then switched to the medium with 10 ng·mL−1 M-CSF and 50 ng·mL−1 RANKL for 7 days. To test Axin1Osx CM, BMM cells were treated with CM collected from cultured calvarial osteoblasts isolated from Axin1Osx KO mice and Cre-negative controls for 7 days. The culture medium was changed every 3 days. TRAP staining was performed using a TRAP assay kit (Sigma, St. Louis, MO, USA).

Statistical analysis

An unpaired Student’s t test was performed for experiments involving two groups. P < 0.05 was considered statistically significant.