Molecular and cellular characterizations of human cherubism: disease aggressiveness depends on osteoclast differentiation

This study included 7 patients (5 children and 2 adults) treated and followed in the maxillo-facial surgery department of Necker Hospital, Paris, through the MAFACE reference center for rare facial malformations. The 5 children were already part of our previously published cohort [19]. All patients gave their written informed consent for this study and for genetic analysis. Age, sex, age at diagnosis, age at first surgical treatment, radiologic extent and evolution of the lesions were recorded for each patient at the biopsy time. Medical treatment and past history were noted. Mutations in the gene encoding the binding protein SH3BP2 on chromosome 4p16.3 were sought for each patient. Direct Sanger sequencing of exons 2 to 13 of the SH3BP2 gene was performed for 7 patients. All patients underwent intraosseous cherubism granuloma curettage.

The cherubism cases were classified according to patient age at the time of surgery (children were classified as group 1, adults as group 2) and sub-classified according to their aggressiveness based on the usual radiologic classification [20] and disease evolution after surgery [19]. For the child cases, radiologic grade I with favorable evolution after surgery was classified as group 1-A (low degree of aggressiveness: radiologic grade I with a favorable evolution); 1-B (moderate degree of aggressiveness: radiologic grade II-IV with a favorable evolution); 1-C (high degree of aggressiveness: radiologic grade V-VI and/or an unfavorable evolution, recurrence or extension); the adult patients were sub-classified as 2-A (remodeling bone) and 2-B (acute exacerbation) (Table 1) [20].

Granuloma samples were obtained at the time of surgery and divided into 2 parts, one for pathological examination and the second for the biochemical and biomolecular studies outlined below. Tissues for pathological examination were fixed in 10% formalin and embedded in paraffin. Four samples of normal alveolar bone, collected during third molar extraction, were included after written informed consent as controls for biomolecular analysis.

4-μm thick sections were cut from each paraffin block. Section staining with hematoxylin/eosin/safranin (HES) was automated by using a Leica Autostainer (Nussloch, Germany): after deparaffinization (in successive baths of xylene and alcohol), staining was performed by successive baths in hematoxylin GILL2 (Thermo Shandon, Pittsburgh, PA, USA), 1% eosin (Ral Diagnostics, Martillac, France), 0.12% safranin in 1% hydrochloric acid solution (Ral Diagnostics, Martillac, France) and 95% ethanol. The sections were then mounted in synthetic resin (WVR, Radnor, PA, USA). Two pathologists blinded to clinical history scored the slides, according to the previous description of cherubism [5, 21, 22]. For each specimen, we evaluated presence of intracytoplasmic vacuoles in MGC, presence of collagen (semi quantitative evaluation: 0, +, ++, +++), cells subtype (fibroblast, round cells, MGCs) semi-quantitative evaluation (0, +, ++, +++), perivascular hyalinosis. From 5 randomly selected areas at 200 high-power field (HPF), we evaluated the number of MGC and the number of nuclei per MGC.

A TRAP activity assay was performed on paraffin-embedded tissue sections and cell cultures from granulomas on Lab-Tek™ chamber slides (Dutscher). Paraffin sections were deparaffinized and rehydrated, stained in pH 5.2 acetate buffer containing 2.5 mM Naphthol AS-TR phosphate, 0.36 M N–N dimethylformamide, 0.1 M sodium tartrate and 4 mM Fast Red TR Salt (Sigma-Aldrich). Hematoxylin was used for nuclear staining. TRAP-positive giant multinucleated (> 3 nuclei) cells were considered as osteoclasts. The number of osteoclasts (MGC > 3 nuclei) and number of nuclei per osteoclast were evaluated from five randomly selected areas (200 HPF).

Total RNA was extracted from the granuloma samples, bone controls or cell cultures using Trizol Reagent (Life technology, Saint Aubin, France) according to the manufacturer’s instructions. The total RNA yield (ng) was determined fluorometrically using a Qubit fluorometer (Life Technologies, Saint Aubin, France). Total RNA (1 μg) was reverse transcribed using SuperScript II™ reverse transcriptase (Life Technologies, Saint Aubin, France) according to the manufacturer’s instructions. Real-time quantitative PCR was carried out using SYBR-green master mix (Life Technologies, Saint Aubin, France) in a BCR Bio-Rad Opticon thermocycler (Bio-Rad, Marne La Coquette, France). PCR conditions were: 98 °C for 30 s followed by 40 cycles of 95 °C for 10 s, 60 °C for 20 s and 72 °C for 20 s. Primer sequences of all the analyzed genes are shown in (Additional file 3). Cq was transformed into quantity values using the formula (1 + Efficiency)^-Cq as previously described [23]. GAPDH, SDHA, TBP and HPRT were used as reference genes.

Samples from only 5 cherubism cases yielded cell cultures. Tumor tissues were washed in PBS. Fragments of the tumors were incubated at 37 °C for 60 min in a hyaluronidase and collagenase solution mix (1 mg/ml for each enzyme) in PBS. The number of cells was counted manually using a Mallassez counting chamber. Cells were cultured either on a dentin slice (ids, Paris, France) (at a density of 0.5 × 10⁶ cells/ml) for the resorption assay, Lab-Tek II chamber slides 1 well (ThermoScientific, Rochester, NY, USA) (at 0,6 × 10⁶ cells/cm²) for the ELISA supernatant study, or Lab-Tek II chamber slides 8 wells (at 0,6 × 10⁶ cells/cm²) for the TRAP activity assay with standard medium. After 12 h of incubation at 37 °C in a 5% CO₂ humidified atmosphere, half of the cell culture was incubated in standard medium and the other half in osteoclastogenic medium. Standard medium contained minimal essential medium (αMEM, without red phenol) and 1% Penicillin-streptomycin, 1% L-glutamine (all from Life Technologies, Saint Aubin, France) and 10% fetal calf serum (Hyclone, South Logan, UT, USA). For the Lab-Tek cultures, osteoclastogenic medium contained standard medium supplemented with RANKL at 30 ng/ml and M-CSF at 25 ng/ml (Peprotech, Neuilly-sur-Seine, France). For the dentin slices cultures, osteoclastogenic medium contained standard medium supplemented with RANKL at 60 ng/ml and M-CSF at 25 ng/ml (Peprotech, Neuilly-sur-Seine, France). Half of the cell culture was maintained for 3 days, and the other half was maintained for 7 days. In the 7-day cultures, the culture medium was changed at day 3. Supernatants were collected at day 3 and day 7 for ELISA. Cultures in Lab-Tek 8 chambers were fixed in 4% paraformaldehyde for TRAP activity measurement, and cultures in Lab-Tek 1 chambers were treated with Trizol Reagent for RNA extraction. Cultures on dentin slices were washed in distilled water and sonicated to remove cells. The slides were then stained with 0.5% toluidine blue to reveal lacunar resorption areas by light microscopy.

Whole blood (15 ml) was obtained from the French Transfusion Establishment (EFS). Blood was diluted with 1X PBS, layered on 12 ml of Ficoll (Euromedex, Souffersheim, France), and then centrifuged (× 1500 g, 10 min, room temperature, with the brake off). The PBMC layer was collected and washed in PBS, and then counted in a Malassez counting chamber. The cells were plated in Lab-Tek 8 chambers (at 0,6 × 10⁶ cells/cm²), in standard medium and osteoclastogenic medium for 14 days.

Levels of RANK-L, OPG, M-CSF, TNF-α and IL-6 in culture supernatants were determined by commercially available specific ELISAs, according to the manufacturer’s protocols (R&D Systems, Minneapolis, MN, USA). The lower and higher detection limits for each cytokine are shown in Additional file 1. It is important to note that the system only detects free, unbound RANK-L. Absorption was determined with an ELISA reader at 450 nm (Additional file 4).

Seven patients with cherubism, five children and two adults, were investigated in this study. Patient ages ranged from 6 to 45 years old at the time of surgery (intraosseous granuloma curettage). None of the patient presented intercurrent disease or medical therapy. The children were categorized as group 1 and the adults as group 2. They were further classified according to granuloma radiological grade and evolution after surgery (Table 1, see Materials and Methods for details). Six of the patients had the same SH3BP2 mutation (c.1244 G > A; p.Arg415Gln), and one had the most common SH3BP2 mutation (c.1253 C > G; p.Pro418Arg), previously described ⁷. Noteworthy was the wide variation in cherubism aggressiveness in this patient sample.

To identify a potential cherubism biomarker, RNAs from a granuloma sample from each patient were extracted to establish a molecular profile for each patient’s granuloma. As cherubism was recently described as being an auto-inflammatory bone disease, we focused on the expression of genes involved in osteoclastogenesis (RANK, RANKL, M-CSF, OPG, NFATc1), bone formation (ALP, Osteocalcin), and inflammation (IL6, IL6R, TNFα, TNFR1, TNFR2, IL17) (Additional file 5).

All granulomas (except 1-B1) and the bone controls provided suitable material for RNA extraction and RT-qPCR analysis. The granulomas and bone expressed M-CSF, TNF-α, TNF-R1, and TNF-R2 mRNAs with no significant differences between the granuloma and bone. RANK mRNA was expressed by all samples, and significantly more expressed in samples 1-B2 (p = 0.07) and 1-C1 (p = 0.0003). RANK-L mRNA was expressed by all samples, and significantly (p = 0.0121) more expressed in sample 1-B2. OPG mRNA was expressed by all samples, and significantly (p = 0.002) more expressed in sample 2-A. The RANKL/OPG ratio was positive in all cases except sample 2-A. NFATc1 mRNA was expressed by all samples, and significantly (p = 0.0001) increased in 1-C2. Osteocalcin and ALP mRNA were expressed by all samples, and significantly more expressed in 2-A (p = 0.00001). IL6-R mRNA was expressed by control bone, 1-C1 and 2-B, with a significant increase in 1-C1 (p = 0.0287). Granulomas and control bone did not express IL-6 and IL17 mRNAs.

Biomolecular analysis showed that, in adult patient 2-A, in whom bone remodeling had occurred post-surgery, the biomolecular profile indicated bone synthesis: increased expression of osteoblast markers (ALP, osteocalcin), and a RANK-L/OPG ratio greater than 1. However, the overall results of the biomolecular analysis reflected extensive inter-tumor heterogeneity (Fig. 1a-d) and did not allow us to define specific cherubism biomarkers.

We first began with a simple histologic analysis. Hematoxylin-eosin-safranin-stained sections of six of the cherubism granulomas (excluding the remodeling case, 2-A) showed multinucleated giant cells within a collagen-rich and well-vascularized fibrous stroma (Fig. 1a-d). The granuloma histology was heterogeneous between patients, reflecting their different cherubism grades, and within each granuloma (Fig. 1a-d). Hyalinosis cuffing surrounded all vessels (Fig. 1b, d). The number of MGC varied from 0 to 35 cells per HPF (mean 6.2 ± 2.1). MGC had 3 to 23 nuclei per cell (mean 7.17 ± 1.25), and some MGC presented intracytoplasmic vacuoles (3 of 7 granulomas). Collagen was abundant (++, +++) in poor-cell- area, and rare (0, +) in rich-cell area (Fig. 1a, d). Reactive bone was seen in all tumors. Adult case 2-A (the remodeling one) showed immature bone in a fibrous stroma, without MGC (Fig. 1e). The acute exacerbation in adult case 2-B showed MGC within a collagen-rich and well-vascularized fibrous stroma, as in the child cases (Fig. 1f).

Because, based on a mouse model, cherubism is considered to be an auto-inflammatory disease [16, 17], we characterized the immune cells to look for an indication of chronic inflammation. Some mononuclear cells were lymphocytes, CD5⁺. Among these lymphocytes, most were CD8+ T lymphocytes, some were CD4⁺ cells, and fewer still were CD20⁺ cells (Table 3, Fig. 2a, b, e, f). In addition, our analysis showed that the cells that expressed CD68⁺ (antigen expressed by myeloid cells) could be mononucleated or multinucleated (Table 3, Fig. 2c, g). In addition, all MGC expressed CD68.

To determine if CD68⁺ multinucleated cells were osteoclasts, we performed a TRAP activity assay. Some MGC CD68⁺ cells were positive for TRAP. The aggressive tumor of patient 1-C showed a high number of TRAP-positive MGC (considered as osteoclast-like cells when TRAP positive with more than 3 nuclei) (Fig. 2d, h, Table 3). Then, to address the role of the RANK/RANKL/OPG triad in cherubism and in the development of these MGC osteoclast-like cells, we studied the expression of these proteins essential for osteoclastogenesis [24]. RANK was expressed in both stromal cells and MGC (Fig. 3a). We found that stromal cells expressed osteoprotegerin (OPG) near the MGC (Fig. 3b). In areas without MGC, some stromal cells of granulomas 1-B2 and 1-C1 expressed RANK-L (Fig. 3c). In the most aggressive cherubism, cases 1-C1 and 1-C2, and in acute adult cherubism, case 2-B, MGC expressed both nuclear and cytoplasmic NFATc1 (Fig. 3d) (Table 2).

Other cells present were supposed to be fibroblasts as they were CD5⁻, CD68⁻, AE1/AE3⁻, vimentin +, and spindle shaped (Fig. 2, Table 3).

Finally, because inflammatory cytokines have been implicated in cherubism [14, 25], we analyzed cytokine receptor expression on the granulomas. No expression of TNF-R1–2 was observed. A few stromal cells from cases 1-A, 1-C1, and 2-B expressed IL6-R (data not shown).

Overall, the histopathological analysis revealed great heterogeneity of cherubism granulomas, in part due to the aggressiveness of the disease; and the unexpected and atypical expression of the RANK/RANKL/OPG triad in cherubism granulomas (low expression of RANKL by cells outside the MGC area; high expression of OPG around the MGC; variable expression of RANK by both MGC and stromal cells) (Table 2). Consistent with an auto-inflammatory bone disease [16, 17], lymphoid cells were present (CD5⁺), most of which were CD8+ lymphocytes; however, immature macrophages (CD68⁺ mononuclear cells), mature macrophages (CD68⁺, multinucleate, TRAP-) and osteoclasts (TRAP+, multinucleate with > 3 nuclei) were observed. TRAP activity, NFATc1 staining and the number of nuclei in CD68⁺ cells, strongly suggesting an osteoclastic phenotype, seem to be associated with the aggressiveness of cherubism. In non-aggressive cherubism, CD68⁺ cells displayed a macrophage phenotype, whereas in aggressive cases, CD68⁺ cells displayed osteoclast characteristics (> 3 nuclei, TRAP+, nuclear NFATc1+).

To analyze the osteoclastic characteristics of the granuloma MGC and determine if the cells are hypersensitive to RANK-L and M-CSF, as demonstrated in the cherubism mouse model [14], we enzymatically digested the granulomas, cultured the cells in standard and osteoclastogenic media, and compared their characteristics with those of osteoclasts obtained from healthy-donor PBMC-ifferentiation cultures (control) (Figs. 4 and 5).

Five of the seven cases (1-B1, 1-B2, 1-C1, 1-C2, and 2B) yielded material suitable for granuloma cell culture. Cases 1-B2 and 1-C2 were only cultured in osteoclastic medium, and analyzed at day 7. In culture, TRAP-positive MGC with greater than 3 nuclei were considered as osteoclasts (Fig. 4). At day 14, the number of control osteoclasts/HPF varied from 0 to 6 (mean 3.6 ± 0.38), the number of nuclei per osteoclast varied from 3 to 6 (mean 3.2 ± 0.26), and the cell size varied from 49 μm to 122 μm (mean 88.2 μm ± 32) (Fig. 4).

Interestingly, in standard medium (i.e., without osteoclastogenic cytokines), the granuloma osteoclasts (day 7) were comparable in terms of both number/HPF (p = 0.053) and size (p = 0.09) to those in the control osteoclast culture (day 14, in osteoclastic medium), but showed a greater number of nuclei (p = 0.002) versus the control osteoclast culture (day 14, in osteoclastic medium) (Figs. 4 and 5). In addition, from day 3 to day 7, granuloma osteoclast number/HPF, number of nuclei per osteoclast, and osteoclast size increased (Additional file 9). This suggests that the cells from the cherubism granuloma are able to differentiate into osteoclasts even without M-CSF and RANKL supplementation to the culture medium.

In osteoclastic medium, granuloma osteoclasts (day 7) were comparable in terms of number/HPF (p = 0.75) compared to the control osteoclast culture (day 14), but they were larger (p = 0.02) and tended to have more nuclei (p = 0.03). In addition, from day 3 to day 7, granuloma osteoclast number/HPF, number of nuclei per osteoclast, and osteoclast size increased (Additional file 9). This suggests that cells of cherubism granulomas have a greater ability to fuse (Figs. 4 and 5).

Finally, in standard and osteoclastogenic media, granuloma cell cultures on bone slides generated resorption pits (Fig. 5), which seemed to be more prevalent when the cells were cultured in osteoclastogenic medium.

The results of the granuloma cell culture studies showed that the MGC could be considered as fully functional osteoclasts, as they are multinucleated (> 3 nuclei), TRAP-positive, and able to resorb bone. Granuloma cells can differentiate into osteoclasts and maturate without RANK-L and M-CSF medium supplementation (as evidenced by the increase in osteoclast number and size, and the number of nuclei between day 3 and day 7). However, these cells are still sensitive to RANK-L and M-CSF, because in osteoclastogenic medium the granuloma cells differentiate further into osteoclasts and the osteoclasts maturate from day 3 to day 7, and they generate more pits than when cultured in standard medium.

It must be noted that these cell cultures were not pure MGC cultures. Thus, the results of standard medium cultures suggest that granuloma cells might secrete cytokines which stimulate osteoclast differentiation, maturation and fusion. In addition, we cannot rule out that some MGC might have been present at the start of the culture.

The main cytokines involved in auto-inflammatory bone diseases [16] are TNF-α, IL-1β, IL-17 and IL-6. Therefore, we next examined the levels of these cytokines in the culture supernatants by using ELISA (Fig. 6).

TNF-α was detected in the supernatant of all cultures (from 0 to 8 ng/ml, depending on the patient and culture conditions). IL-6 was detected in the supernatant of all cultures at higher levels than for TNF-α (from approx. 2 to 147 ng/ml, depending on the patient and culture conditions). IL-17 was not detected. OPG was detected in the supernatant of all cultures (from 5 to almost 150 ng/ml), whereas unbound RANK-L levels were generally lower than OPG levels (from barely detectable to 151 ng/ml), leading to a RANK-L/OPG ratio of less than 1 in most cases (Fig. 6).

Although in the culture supernatant the RANK-L/OPG ratio disfavors osteoclastogenesis, we demonstrated an increase in the number and size of the MGC in culture. The cytokine analysis showed that OPG and RANK-L are not playing their usual role in the osteoclastic differentiation of these granuloma cells, because even with the apparently unfavorable RANK-L/OPG ratio (< 1), the number of osteoclasts increased. Instead, IL-6 might stimulate osteoclast differentiation and maturation.