Mesenchymal Stromal Cell-Seeded Biomimetic Scaffolds as a Factory of Soluble RANKL in Rankl-Deficient Osteopetrosis.

Biomimetic scaffolds are extremely versatile in terms of chemical composition and physical properties, which can be defined to accomplish specific applications. One property that can be added is the production/release of bioactive soluble factors, either directly from the biomaterial, or from cells embedded within the biomaterial. We reasoned that pursuing this strategy would be appropriate to setup a cell-based therapy for RANKL-deficient autosomal recessive osteopetrosis, a very rare skeletal genetic disease in which lack of the essential osteoclastogenic factor RANKL impedes osteoclast formation. The exogenously administered RANKL cytokine is effective in achieving osteoclast formation and function in vitro and in vivo, thus, we produced murine Rankl-/- mesenchymal stromal cells (MSCs) overexpressing human soluble RANKL (hsRL) following lentiviral transduction (LVhsRL). Here, we described a three-dimensional (3D) culture system based on a magnesium-doped hydroxyapatite/collagen I (MgHA/Col) biocompatible scaffold closely reproducing bone physicochemical properties. MgHA/Col-seeded murine MSCs showed improved properties, as compared to two-dimensional (2D) culture, in terms of proliferation and hsRL production, with respect to LVhsRL-transduced cells. When implanted subcutaneously in Rankl-/- mice, these cell constructs were well tolerated, colonized by host cells, and intensely vascularized. Of note, in the bone of Rankl-/- mice that carried scaffolds with either WT or LVhsRL-transduced Rankl-/- MSCs, we specifically observed formation of TRAP+ cells, likely due to sRL released from the scaffolds into circulation. Thus, our strategy proved to have the potential to elicit an effect on the bone; further work is required to maximize these benefits and achieve improvements of the skeletal pathology in the treated Rankl-/- mice. Stem Cells Translational Medicine 2019;8:22-34.

RANKL‐<span class="Disease">deficient autosomal recessive osteopetrosis is a very rare skeletal genetic disease in which lack of the essential osteoclastogenic factor RANKL impedes osteoclast formation and bone resorption, and causes extremely high bone density and secondary hematological and neurological defects. At present, there is no cure for this disease. Results of this study demonstrated that RANKL‐releasing MSC‐seeded biomimetic constructs implanted subcutaneously in Rankl mice served as a source of the missing cytokine and restored the formation of TRAP+ cells in bone, thus providing proof of principle of the capacity of this approach to support cell differentiation towards the osteoclast lineage in vivo. Implementation of the experimental setting by means of recent biotechnological tools will increase the effectiveness of this strategy on the bone compartment.

Introduction

Over the last 15 years a great variety of biomimetic scaffolds, rationally designed devices with specific physicochemical properties, conceived to be seeded with cells, and used in vivo to elicit or replace a missing function that cannot be promptly restored by cells only, have been developed 1. In the bone field, biomimetic scaffolds are exploited for their osteoinductive and osteoconductive properties; in basic studies, they constitute a tool for evaluating osteogenic potential of mesenchymal stromal cells (MSCs) from different tissues in ectopic bone formation assays 2. In translational studies, a range of strategies for tissue engineering have been implemented; in the majority of cases, bone‐like scaffolds support and induce bone regeneration to replace areas of <span class="Disease">bone loss in large defects or at load‐bearing sites 3. Biomaterials may also serve as a source of bioactive soluble factors; these may be either incorporated in the scaffold during its production and released from there in specific environmental conditions, or secreted by cells seeded on these three‐dimensional (3D) structures 4, 5.

Our work intended to evaluate this latter application in the context of Receptor Activator of Nuclear Factor k B Ligand‐deficient Autosomal Recessive Osteopetrosis (RANKL‐ARO), a rare genetic skeletal disease in which lack of production of the essential osteoclastogenic molecule RANKL by cells of the stromal compartment in bone hinders osteoclast formation and bone resorption. This leads to extremely high bone density and secondary hematological and neurological defects, which further compromise the clinical picture, hence threatening the patients’ survival 6. At variance with other known forms of ARO, in which the defect is cell autonomous and early Hematopoietic Stem Cell Transplantation (HSCT) is an effective cure, in RANKL‐ARO the osteoclast defect is not cell‐autonomous, thus it cannot be rescued by HSCT 7, 8. Thus, defining a cure for RANKL‐ARO is currently an unmet medical need, whose solution is unfairly complicated owing to the extreme rarity of these patients.

Thanks to the availability of a mouse model (Rankl knockout, Rankl ) closely resembling the human disease, and to the biological activity in vivo of soluble RANKL, two different targeted therapeutic approaches have been evaluated at a preclinical level: a pharmacological and a cell‐based one 9, 10. The former consisted of the exogenous administration of soluble recombinant RANKL to Rankl mice; in our work, we evaluated different treatment schedules and identified a specific protocol able to correct the bone pathology 9. As an alternative way to provide the defective cytokine, Cappariello and colleagues assembled diffusion chambers containing osteoblasts seeded on a matrix metalloprotease 14 (MMP14)‐functionalized scaffold to facilitate RANKL shedding from the cell membrane, and implanted them in vivo 10. This strategy overcame the major limitation of the pharmacological approach, that is, the requirement for high quality (Good Manufacturing Practice, GMP‐level) recombinant RANKL for a thorough preclinical study; however, it required invasive surgery to obtain sufficient RANKL release as compared to in vivo cytokine administration.

Based on the nature of the defect in RANKL‐<span class="Gene">ARO, here we devised an approach based on Mesenchymal Stromal Cells (MSCs), multipotent stromal cells characterized by in vitro plastic adherence, colony‐forming capacity, expression of a panel of surface molecules, and ability to differentiate at least toward the osteogenic, adipogenic, and chondrogenic lineages 11. In regenerative medicine, they represent a valuable tool capable of restoring normal tissue function through the stimulation of repair mechanisms by the host's cells 12. This mainly occurs via the production of a wide range of trophic factors, also comprised of the RANKL cytokine 3, 11, 13, 14, 15. On this basis, MSCs are under evaluation for cell therapy of a range of disorders, which could be combined with gene delivery via viral vectors to elicit specific MSC properties 16.

Moreover, increasing evidence showed that MSC features are strictly dependent on environmental, physical, mechanical, and chemical characteristics, and this drove the engineering of biomimetic scaffolds artificially reproducing selected natural microenvironments 17.

Of note, we recently reported the generation of wild type (WT) and Rankl murine MSC lines, and, in the latter, the restoration of RANKL production and osteogenic capacity by transduction with a lentiviral vector expressing human soluble RANKL 13. Based on the close resemblance of RANKL‐defective osteopetrosis in humans and mice, we envisage RANKL production might be similarly reestablished in patient‐derived cells.

Overall, these data provided the rationale for our novel approach: we hypothesized that MSC‐seeded scaffolds carrying either WT or transduced cells, might serve as a factory of soluble RANKL, and thus provide the cytokine in Rankl‐deficient osteopetrosis to restore osteoclastogenesis. Here, we describe the establishment of murine MSC 3D cultures on a bone biomimetic scaffold and provide proof‐of‐principle that subcutaneous implantation of these scaffolds seeded with RANKL‐expressing MSCs in Rankl mice restores formation of TRAP+ cells, bona fide osteoclasts in the bone tissue.

Materials and Methods

Cell Culture

The Human Embryonic Kidney 293 T (HEK293T) cell line was purchased from ATCC and cultured in IMDM medium supplemented with 10% fetal bovine serum (FBS; both from GIBCO, Grand Island, NY), 1% penicillin/streptomycin and 1% glutamine (Lonza, Basel, Swizerland).

Bone marrow‐derived mesenchymal stromal cells (MSCs) were isolated, cultured, and characterized as previously described from both WT and <span class="Gene">Rankl <span class="Species">mice 13. Cells were kept in a humidified 5% CO2 incubator at 37°C.

Lentiviral Transduction

The third‐generation bidirectional lentiviral vectors (LVhsRL and mock) used for HEK293T and MSCs transduction have been already described 13. Briefly, the IgK‐chain leader secretion signal followed by the extracellular region of <span class="Species">human RANKL (nucleotides 416‐954, NM_003701) was inserted into the #1074.1071.hPGK.GFP.WPRE.mhCMV.dNGFR.SV40PA plasmid backbone (gift of Prof Luigi Naldini, San Raffaele Telethon Institute for Gene Therapy, Milan), according to standard protocols. The lentiviral vectors were produced following standard procedures and in accordance with institutional and national laws (notification n. MI/IC/IMP2/12‐003).

The day before transduction, HEK293T cells were plated at a density of 104 cells/cm2 in 6‐well plate. Lentiviral transduction was performed in 1.0 ml culture medium at a multiplicity of <span class="Disease">infection (MOI) ranging from 1 to 100, in the presence of 8 μg/ml Polybrene (Sigma‐Aldrich, Saint Louis, MO); untransduced cells were treated with Polybrene only as control. After 16 hours, the medium was replaced with fresh culture medium. Transduced cells expressing GFP were analyzed by flow cytometry (FACSCantoII, BD Bioscience, Eysins, Switzerland) to assess GFP fluorescence. HEK293T cell viability was evaluated through the dye exclusion test with Trypan blue and by MTT Test, following standard procedures. Two weeks after transduction, vector copy number (VCN) was determined by qPCR as previously described 18.

<span class="Gene">Rankl MSCs were transduced with either LVhsRL or mock lentiviral vector at 20 MOI, as previously described, and maintained in MSC complete Mesencult medium (Stemcell Technologies, Vancouver, BC) 13.

RANKL Protein Analysis

Total protein extraction, gel electrophoresis, transfer, and visualization were performed according to standard Western blotting procedures. Briefly, cell lysis was done in RIPA buffer and proteins were quantified using the DC Protein Assay Kit II (Biorad, Berkeley, CA) following the manufacturer's instructions, on a Synergy H4 instrument (BioTek Instruments, Inc., Winooski, VT). Twenty‐five micrograms of protein extracts were separated on a 10% Sodium Dodecyl Sulfate Polyacrylamide Gel Electrophoresis (SDS‐PAGE) and transferred to a nitrocellulose membrane. This was incubated with human RANKL monoclonal antibody (Alexis Corporation, Lausen, Switzerland), diluted 1:1,000 in 5% milk solution, for 2 hours at room temperature, then washed, probed with a secondary antibody conjugated with HRP and developed using the Immobilon Western kit (Millipore, Darmstadt, Germany). Images were acquired using the ChemiDoc MP Imaging System equipped with Image Lab Software (Biorad).

In Vitro Osteoclastogenesis and Resorption Assay

Conditioned culture medium (CM) from <span class="CellLine">HEK293T cells transduced with either LVhsRL or the mock vector at 20 MOI underwent protein enrichment by Vivaspin column 10 MWCO (Sartorius, Goettingen, Germany) ultrafiltration according to the manufacturer's instructions, to obtain a ×50 concentrated CM with a final concentration of about 2 ng/ml hsRL.

In vitro osteoclastogenesis was induced in human PBMCs obtained from buffy coat of healthy donors by Ficoll separation or in murine WT and Rankl murine splenocytes. Briefly, 4 × 105 cells/well were cultured in 96‐well plate in αMEM medium (Sigma‐Aldrich) supplemented with 10% FBS, 1% penicillin/streptomycin, and 1% glutamine in the presence of 25 ng/ml M‐CSF, 5 ng/ml human TGFβ1 (both from Peprotech, London, UK), 1 μM Dexamethasone (Sigma‐Aldrich) and with or without 100 μl/ml of either CM for 6 or 12 days (for murine and human cells, respectively). Mature osteoclasts were stained using the Tartrate Resistant Acid Phosphatase (TRAP) Kit (Sigma‐Aldrich) following the manufacturer's instruction.

The same culture conditions were used to perform osteoclastogenesis on dentin discs (Immunodiagnostic Systems, Ltd., Scottsdale, AZ) to evaluate osteoclast resorption activity. After 3 weeks, dentin discs were rinsed with water, scraped to remove attached cells, stained with 1% toluidine blue solution for 3 minutes, and then washed with water to visualize resorption pits. Images were acquired on an EVOS XL Inverted Microscope (Thermo Fisher Scientific, Waltham, MA) for both TRAP+ mature osteoclasts and toluidine blue stained dentin discs.

MgHA/Col Scaffold Synthesis

Equine tendon derived type I collagen, 1 wt.% in aqueous acetic buffered solution (pH 3.5), was purchased from Opocrin SpA (Modena, Italy). Phosphoric acid (H3PO4, 85 wt.%), calcium hydroxide (Ca(OH)2, 95 wt.%), magnesium chloride hexahydrate (MgCl2·6H2O, 99 wt.%), and 1,4‐butanediol diglycidyl ether (BDDGE, 95 wt.%) were purchased from Sigma Aldrich. Phosphate buffer saline (PBS, pH 7.4) was supplied by EuroClone (Milan, Italy).

Briefly, 100 g of collagen gel were dissolved into a 0.04 M phosphoric acid solution, while 0.235 g of MgCl2·6H2O were added to a 0.07 M basic calcium suspension 19, 20. The acid collagen slurry was added drop‐wise into the basic calcium and magnesium suspension, leading to the formation of Mg‐doped apatite nanocrystals uniformly distributed in the collagen matrix. After 2 hours at room temperature, the hybrid slurry was washed three times in distilled water and filtered to remove free ions. The cross‐linking reaction was carried out in the presence of 20 ml of 1 g/L of BDDGE solution for 24 hours at room temperature, followed by 24 hours at 4°C 21, 22. Afterward, the cross‐linking solution was removed and the hybrid composite was washed three times with distilled water before pouring it into polystyrene 96‐well plate. Porous 3D‐hybrid scaffolds were obtained by freezing the collagen hydrogel at −40°C and drying it at 25°C (5 Pascal, LIO 3000 PLT, Milan, Italy) for 48 hours under a constant vacuum of 0.086 mbar. Finally, the scaffolds were sterilized by gamma‐irradiation.

Scanning Electron Microscopy (SEM)

Specimens were mounted onto <span class="Chemical">aluminum stubs using black <span class="Chemical">carbon tapes and sputter coated with gold (Sputter Coater Q150TES, Laughton, UK). The specimen surface and scaffold microarchitecture were examined using high resolution SEM (FEI, Quanta 200, Cambridge, UK) under a pressure of 0.1 mTorr at an accelerating voltage of 7 or 10 kV.

Structural Characterization of MgHA/Col

The total porosity was calculated by the gravimetric (or density) method 23, according to the formula:where ρ is the scaffold density determined with the equation:in which W is the weight, D is the diameter, and H is the height of the scaffold; and the theoretical density of the material is calculated from the theoretical density and weight fraction (X A, X B,…) of each reagent:

The macropores volume percentage was calculated by the water squeezing method 24. Briefly, the scaffold was equilibrated in deionized water for 1 hour and weighed (M swollen), then squeezed to remove the water filling the pores and weighed again (M squeezed). Macropores volume was calculated using the equation:

All the values were expressed as the mean ± SEM (n = 3).

X‐Ray Diffraction (XRD)

XRD patterns of the samples were recorded on a D8 Advance diffractometer (Bruker, Karlsruhe, Germany) equipped with a Lynx‐eye position sensitive detector using Cu Kα radiation (l = 1.54178 Å) generated at 40 kV and 40 mA. XRD spectra were recorded in the 2θ range from 20° to 60° with a step size (2θ) of 0.02° and a counting time of 0.5 seconds.

Fourier Transform Infrared Spectroscopy (FTIR)

FTIR spectra were collected on a Nicolet 380 spectrometer (Thermo Fisher Scientific Inc.) with a resolution of 4 cm−1 by accumulation of 64 scans covering the 4,000 to 400 cm−1 range, using the KBr pellet method.

The pellets (13 mm Ø) were prepared by mixing 2 mg of ground sample with 100 mg of KBr in a mortar and pressing.

Inductively Coupled Plasma Optical Emission Spectrometry (ICP‐OES)

Calcium, <span class="Chemical">phosphate, and magnesium contents were determined by ICP‐OES using a Liberty 200 spectrometer (Varian, Palo Alto, CA). Twenty milligram of sample were dissolved in 50 ml of a 1 wt.% HNO3 solution prior to analysis.

Thermal Gravimetric Analysis (TGA)

The thermal properties and the ratio between collagen and <span class="Chemical">MgHA in the hybrid sample were measured using a simultaneous thermal analyzer STA 449/C Jupiter (Netzsch, Germany). Simultaneous TGA was carried out on approximately 10 mg of sample placed in <span class="Chemical">alumina crucibles, and then brought from room temperature to 1,200°C at a heating rate of 10°C/min under an airflow of 1 ml/min.

Swelling and Degradation Tests

The scaffolds were soaked in PBS, pH 7.2 in the presence of 0.1% (wt/vol) <span class="Chemical">NaN3 at 37°C. At specific time points, the samples were blotted with a piece of paper to remove surface droplets. The <span class="Disease">swelling ratio (Qs) was evaluated using the following equation:where W s is the weight of the swollen sample at a specific time point and W d the initial weight of the dried sample.

In the degradation test, the scaffolds were soaked as above, then washed twice with milli‐Q <span class="Chemical">water, freeze‐dried for 2 days and subsequently weighed. The degradation percentage (D) was evaluated using the following equation:where W i is the initial weight of the dried sample and W f the weight of the freeze‐dried sample at a specific time point.

Standardization of MSC 3D Culture

Sterile <span class="Chemical">MgHA/Col scaffolds were incubated overnight at 37°C in the MSC conventional culture medium. The day after, the scaffolds were placed in 48‐well plate (1 scaffold/well). LVhsRL‐MSCs with 5 × 105 were suspended in 30 μl of standard culture medium and dropped onto each scaffold. Cell attachment was allowed for 30 minutes at 37°C and 5% CO2. Subsequently, 1 ml of cell culture medium was added to the cell‐seeded 3D scaffold system to completely cover it. To evaluate cell morphology and behavior in 3D culture, we took advantage of GFP expression by transduced MSC and collagen autofluorescence. Cell‐seeded scaffold systems were <span class="Chemical">formalin fixed at 24, 48, and 72 hours after seeding and analyzed by confocal microscopy. Images were acquired with a laser‐scanning confocal microscope (FluoView FV1000, Olympus Corp., Hamburg, Germany), with 405 and 488 nm wavelength laser excitation for collagen and GFP+‐MSC‐transduced cell, respectively. The resulting fluorescence emissions were collected in a wavelength range from 425 to 475 nm (for collagen) and from 500 to 560 nm (for GFP+ MSC‐transduced cell). Images were acquired with a 10X UPLSAPO objective (Olympus); then, processing, analysis, 3D stack reconstruction and surface rendering were performed using Imaris ×64 7.6.5 software (Bitplane, Belfast, Ireland).

For the evaluation of MSC viability and human RANKL production over time, cell‐seeded scaffolds were maintained up to 6 days and the medium changed every 2 days; conventional 2D culture of the same cells (5 × 105 cells in 6‐well plate) was concomitantly performed as a control. For both 2D and 3D cultures, at days 2, 4, and 6, cell viability of WT, mock‐transduced, and LVhsRL‐transduced Rankl MSCs was assessed through MTT assay. hsRL levels were measured after 3 days of culture by ELISA (PromoCell GmbH, Heidelberg, Germany) on the culture medium collected from LVhsRL‐transduced Rankl MSCs.

In Vivo Implantation

All mouse experimental procedures were performed in accordance with the Humanitas Institutional Animal Care and Use Committee and with international laws (authorization n.540/2017‐PR). Rankl mice were a kind gift of Prof. Yongwon Choi (University of Pennsylvania, Philadelphia, PA) 25. The colony was maintained in heterozygosis in a specific pathogen‐free facility; the litters were genotyped as described 25 and Rankl mice were fed a soft diet after weaning. The study design comprised only Rankl mice. In detail, 6 week old Rankl mice (both males and females) were randomly divided in three groups: one was implanted with LVhsRL‐transduced MSC‐seeded scaffolds, another with mock‐transduced MSC‐seeded scaffolds and the last with WT MSC‐seeded scaffold, as controls. In each group, mice were implanted with either 1 or 2 scaffolds, which were prepared following a different protocol: (a) 1 scaffold/mouse: seeding of 7 × 105 cells (WT MSC, or mock‐transduced or LVhsRL‐transduced MSC) and implantation after overnight culture at 37°C, 5% CO2; (b) 2 scaffolds/mouse: seeding of 1.5 × 106 cells/scaffold (WT MSC, or mock‐transduced or LVhsRL‐transduced MSC), 3 days culture at 37°C, 5% CO2 to allow cell penetration into the scaffold, and then implantation. In both protocols, the yield of cell seeding was calculated as a ratio between the amount of cells effectively attached to the scaffold (inferred as the difference between the number of seeded cells and that of cells left on the bottom of the well) and those initially seeded.

For the surgery, Rankl <span class="Species">mice underwent deep anesthesia (Ketamine/Xylazine) and were shaved on the back; then, under sterile conditions the skin was incised over the shoulders and a subcutaneous pouch was formed, in which the cell‐seeded scaffold(s) was (were) inserted. The incision was sewn up with wire absorbable suture; then the mice were kept warm on a special hotplate and singly housed, when they had sufficiently recovered. After 8 weeks, mice were sacrificed by CO2 asphyxiation; blood, scaffold systems, long bones, and soft tissues were collected for serological and histological evaluations.

Histological Analysis

The harvested scaffolds were fixed in 4% paraformaldehyde (PFA) and decalcified in ion exchange decal unit (Biocare Medical, Concord, CA), dehydrated and embedded in paraffin for <span class="Chemical">hematoxylin and eosin (H&E) staining and for immunohistochemistry by using anti‐GFP (Invitrogen Thermofisher; 1:200), anti‐CD31 (R&D, Minneapolis, MN; 1:1,000), and anti‐F4/80 (Biorad; 1:100) antibodies according to standard protocols.

Bones were fixed in 4% PFA for 48 hours, decalcified in 14% EDTA solution for 2 weeks and <span class="Chemical">paraffin‐embedded for TRAP staining with the Acid Phosphatase TRAP kit (Sigma‐Aldrich). TRAP+ cells were counted in at least two stained long bone sections per animal. Digital images were acquired with an Olympus XC50 camera mounted on a BX51 microscope (Olympus), and analyzed with CellF Imaging software (Soft Imaging System GmbH, Munster, Germany).

All other tissues were harvested, <span class="Chemical">formalin‐fixed, and <span class="Chemical">paraffin‐embedded for H&E staining.

hsRL Cytokine and Calcium Level Evaluation

The concentration of hsRL in the culture medium of transduced and untransduced HEK293T cells and of 2D or 3D cultured MSC was determined using the <span class="Species">human sRANKL (total) Enzyme Linked Immunosorbent Assay (ELISA) kit (PromoCell GmbH, Heidelberg, Germany). Serum total calcium levels were determined using a Ci16200 Architect Abbott instrument (Abbott Park, Green Oaks, IL).

Statistical Analysis

Statistical analysis was performed using Mann–Whitney test or t test when comparing two groups. One‐way or Two‐way Anova with Tukey's post‐test were used for multiple comparisons (GraphPad Prism 5.0, GraphPad Softwares Inc. La Jolla, CA). Statistical significance was considered when p < .05 (* p < .05, ** p < .01, *** p < .001). All the experiments were performed at least in triplicate. All data are presented as mean ± SEM.

Results

Validation of a Lentiviral Vector Expressing Human Soluble RANKL

We recently produced a third generation bidirectional lentiviral vector, expressing human soluble RANKL (LVhsRL), under the minimal core element of the CMV promoter (mhCMV) and the green fluorescent protein (GFP) under the human PGK (hPGK) promoter (Fig. 1A); the vector expressing only the GFP was used as a control 13. We utilized the HEK293T cell line as commonly accepted for validation procedures 18, 26. Namely, we transduced HEK293T cells with increasing amount of lentiviral particles, from 1 to 100 MOI for both the LVhsRL and mock vector. In both conditions, the fraction of transduced cells was directly proportional to the used MOI up to MOI 20, and no significant difference was found between MOI 20, 50 and 100, as assessed through GFP fluorescence by cytofluorimetric analysis (Fig. 1B, left plot); so the transduction efficiency of the two vectors was comparable. Mean Fluorescence Intensity (MFI) of GFP+ cells was comparable at MOI 1–20, and higher at MOI 50 and 100 with both vectors (Fig. 1B, right plot), likely due to higher viral integration in these latter conditions. In addition, cell viability and growth, measured through the MTT test at 24, 48 and 72 hours posttransduction, inversely correlated to the used MOI, as expected (Fig. 1C). At all the time points, RANKL concentration was significantly higher in the supernatant of LVhsRL‐transduced as compared to untransduced cells, as expected. In particular, in a short timeframe (within 3 days after transduction), no difference was observed between 1, 5, and 10 MOI. At 20, 50, and 100 MOI RANKL production significantly higher as compared to lower MOIs at all the time points. At 48 and 72 hours after transduction, cytokine levels were greatly reduced at MOI 50 and 100 (Fig. 1D), likely due to decreased cell viability at these MOIs; no such effect was observed at MOI 20. Then, we selected the conditions 10, 20, and 50 MOI for long‐term culture (up to 12 days after transduction). In this period, cells of all experimental settings recovered as inferred by measuring RANKL production, which was sustained and proportional to the used MOI, as assessed both in the cells by Western blot and in the supernatant by ELISA assay (Fig. 1E). The achieved VCN was similar between LVhsRL‐transduced and mock‐transduced cells, with values of 4.56, 8.45, and 16.16 for cells transduced with the LVhsRL vector at 10, 20, and 50 MOI, and 3.02, 4.74, and 16.58 for cells transduced with the mock vector at the same MOIs.

Figure 1

Validation of a lentiviral vector expressing human soluble RANKL (hsRL). (A) Schematic representation of the lentiviral vector for the expression of hsRL. (B) Quantization of HEK293T cell transduction with the LVhsRL and mock vector at increasing MOI, expressed as percentage of GFP+ cells (left) and as GFP mean fluorescence intensity (MFI; right). (C) Evaluation of cell growth rate over time of untransduced and transduced HEK293T cells, by MTT assay. (D) Quantization of hsRL production over time by untransduced and transduced HEK293T cells, by ELISA assay on the corresponding supernatants. Only statistics between different time points of the same MOI is indicated. (E) Quantization of hsRL in protein extracts (left) and in supernatants (right) of untransduced and transduced HEK293T cells 2 weeks after transduction. * p < .05; ** p < .01, *** p < .001.

Overall, these results showed that the LVhsRL vector was able to transduce effectively HEK293T cells and to achieve sustained soluble <span class="Gene">RANKL production. In addition, based on these data and foreseeing the usage of transduced cells shortly after transduction, we reasoned that 20 MOI provided an optimal balance between cell viability and RANKL production; therefore, the following experiments were performed at this MOI.

Functional Evaluation of the RANKL Cytokine Produced by Transduced HEK293T Cells

To assess whether the RANKL cytokine expressed by the lentiviral vector was biologically active, we verified whether it was capable of inducing osteoclast differentiation from <span class="Species">mouse and human precursor cells; in fact, human RANKL is known to be effective on precursors from both species 27, 28. In detail, the conditioned media (CM) of LVhsRL‐transduced HEK293T cells (MOI 20) was used in a standard osteoclastogenesis assay in place of the recombinant RANKL cytokine; the CM of mock‐transduced HEK293T cells was used in parallel, as a negative control. In this regard, it is worth mentioning here that the RANKL concentration in LVhsRL‐transduced HEK293T supernatants was lower than that used in standard osteoclastogenesis protocols (i.e., 37.13 ± 0.8 pg/ml as compared to 20–100 ng/ml 29, 30). Therefore, the CM from both LVhsRL‐transduced and mock‐transduced cells was concentrated by a factor of 50, achieving an hsRL concentration of 2.32 ± 0.28 ng/ml in the LVhsRL‐CM, prior to application to the osteoclastogenesis assay.

Then, WT or Rankl <span class="Species">murine splenocytes and human peripheral blood mononuclear cells (PBMCs) from a healthy donor were cultured either on plastic or dentin discs in the presence of M‐CSF and with or without the concentrated CM. At the end of the differentiation protocol, in the presence of RANKL‐containing CM, osteoclasts formed from both murine and human precursor cells and resorbed dentin, as demonstrated by TRAP and toluidine blue staining, respectively. On the other hand, no differentiation was achieved in the presence of the concentrated mock CM (Fig. 2). The most obvious explanation to this result was that hsRL present in the LVhsRL CM endowed this supernatant with a pro‐osteoclastogenic capacity.

Figure 2

Functional evaluation of hsRL produced by transduced HEK293T cells. Osteoclastogenesis and resorption assays from (A) human PBMCs and (B) murine WT and Rankl splenocytes in the presence of M‐CSF and ×50 concentrated conditioned medium from mock‐transduced and LVhsRL‐transduced HEK293T cells (left and right plots, respectively). Mature osteoclasts were identified by TRAP staining, while resorption pits were visualized by staining dentin discs with toluidine blue. Scale bars: 200 μm (A); 400 μm (B).

Overall, these data confirmed that the <span class="Gene">RANKL cytokine expressed by the lentiviral vector was functional in vitro.

Production of a 3D Biomimetic Scaffold

We recently reported on the generation and characterization of murine bone marrow‐derived WT and Rankl MSCs, and the transduction of these latter with LVhsRL and mock lentiviral vectors 13. In the framework of the present study, to favor MSC survival and proliferation, and enhance their functional properties, we set up a 3D culture. In detail, we generated a scaffold made of Magnesium‐doped hydroxyapatite/collagen I (MgHA/Col), which could ideally mimic the physicochemical characteristics of the bone. The 3D hybrid composites were synthetized through a biomineralization process allowing nucleation of biomimetic HA nanoparticles on type I collagen fibers during their self‐assembly guided by pH changes. SEM analysis showed the porosity and the whole hybrid's structure at low magnifications, and the formation of nanostructured and homogeneously distributed apatite nanocrystals aligned on collagen fibers, at high magnification (Fig. 3A). The assessment of the porosity of the hybrid composite with two different methods highlighted a total porosity close to 95% comprising nanopores and micropores and about 60% of macropores suitable for cell proliferation (Fig. 3B). TGA analysis revealed a weight ratio of the MgHA/Col hybrid composite 60/40 (Fig. 3C), so very close to the composition of the natural bone tissue 31. FTIR spectra of the hybrid composite MgHA/Col and of an hydroxyapatite (HA) synthetized in the same condition and selected as reference material, revealed the presence of typical peaks of collagen together with those of apatite in the biomineralized material. In detail, the peaks at about 1,000 cm−1 and 600 cm−1 correspond to the apatite, while those between 1,300 cm−1 and 1,650 cm−1 correspond to the alpha‐helical structure of collagen at amide I, II, and III. In particular, the shift from 1,340 cm−1 to 1,337 cm−1 was because of the stretching of COOˉ groups of collagen, indicating the active interaction of collagen functional groups with the positively charged apatite crystals (Fig. 3D).

Figure 3

Characterization of 3D biomimetic MgHA/Col scaffold. (A) Scanning Electron Microscopy micrographs at different magnifications, showing scaffold porosity and micro‐architectures of the hybrid composite. (B) Porosity and chemical composition of the hybrid MgHA/Col scaffold. (C) TGA, (D) FTIR, and (E) XRD analysis. In plots D and E, the solid line indicates the MgHA/Col, while the dashed one the HA. (F) Evaluation of the swelling ratio and (G) percentage of degradation of MgHA/Col scaffolds overtime.

XRD analysis of the hybrid <span class="Chemical">MgHA/Col and of the reference HA showed the typical peaks of low crystalline apatites; however, the mineral phase synthetized through the biomineralization process produced wider peaks. This indicated that the presence of <span class="Chemical">Mg2+ ions and the template and structural confinement action of collagen fibers led to the formation of a less crystalline and thus more biomimetic mineral phase (Fig. 3E).

ICP analysis confirmed the presence of Magnesium in the final composite with evidence of a partial substitution of Calcium with Magnesium in the apatite lattice. In particular, ICP showed that about 70 wt.% of the initial nominal concentration of Mg2+ ions substituted Ca2+ in the apatite lattice, and that the Ca/P ratio of the MgHA nucleated on collagen was in the typical range of low crystalline apatite (1.45–1.60), as expected (Fig. 3B). Finally, this material had high hydrophilicity and very low‐degradation rate, thanks to the stability conferred by the crosslinking action of BDDGE 20 (Fig. 3F, 3G). Overall, these properties made our scaffold particularly suited for in vitro and in vivo experiments.

MSC Culture on MgHA/Col Scaffolds

As above explained, our strategy is based on the use of MSC. Thus, we exploited WT and <span class="Gene">Rankl MSC lines previously generated and afterward transduced at MOI 20 according to the validation experiments 13. For the present purpose, we first studied MSC behavior on the produced scaffolds in terms of cell morphology and interactions, attachment to the collagen fibers and invasion. To this end, we took advantage of GFP expression by transduced MSCs, on one hand, and of collagen autofluorescence, on the other. Initially, cells appeared to distribute on top of the scaffold, showing their typical “fibroblast‐like” shape, to organize and firmly attach along the collagen fibers. As early as 48 hours after seeding, they had entered the scaffold and begun to colonize it; in addition, cell proliferation and cell‐to‐cell contacts appeared to increase over time. On the other hand, the scaffold itself was modified and remodeled over time by the invading cells (Fig. 4A).

Figure 4

Characterization of MSC culture on MgHA/Col scaffolds. (A) Confocal analysis of LVhsRL‐transduced Rankl MSC‐seeded scaffolds at different time points; blue color corresponds to collagen fibers, green to MSCs. Scale bar: 200 μm (B) Assessment of WT, mock‐transduced and LVhsRL‐transduced Rankl MSC proliferation in 2D versus 3D culture overtime by MTT assay. Cell growth is expressed as fold increase compared to time 0. Statistics is referred to comparison of 2D versus 3D for each group. Cell growth fold increase data ± SEM are reported in Supporting Information Table 1. (C) Evaluation of hsRL concentration in the supernatant of LVhsRL‐transduced Rankl MSCs in 2D versus 3D culture by ELISA assay. * p < .05; ** p < .01.

Then, we compared cell proliferation in 2D versus 3D culture on the produced scaffold. At all time points, cell growth, determined as fold increase as compared to day 0, was greater in 3D than in 2D cultures, irrespective of the genotype, or vector used for transduction (Fig. 4B and Supporting Information Table S1). Furthermore, the amount of cytokine produced by the LVhsRL‐transduced cells upon 3D culture was significantly higher as compared to the 2D setting (Fig. 4C); in contrast, the <span class="Gene">RANKL cytokine was absent in mock‐transduced <span class="Gene">Rankl MSCs culture medium, as expected ([13] and data not shown).

Overall, these data demonstrated that our <span class="Chemical">MgHA/Col scaffold was a good substrate for MSCs culture: seeded cells adhered nicely and interacted with the provided support and extensively colonized it; moreover, their viability was maintained and proliferation was increased over time. Thus, the cytokine production was significantly enhanced.

We already reported evidence showing that a similar cell‐scaffold construct was well tolerated and osteoinductive in immunodeficient mice 13. Here, we verified the in vivo biocompatibility of the cell‐seeded MgHA/Col scaffold and the effect of lentivirally mediated RANKL production in the Rankl mouse. In detail, Rankl mice underwent subcutaneous implantation of a scaffold seeded with 7 × 105 cells, which were either LVhsRL‐transduced or mock‐transduced Rankl MSCs or WT MSCs, as controls; the seeding efficiency was about 90%. After surgery, the animals were monitored for 2 months; in this timeframe, no sign of distress was apparent. At necropsy, the scaffold, long bones, spine, and selected tissues were harvested and processed for histological analysis. Hematoxilin‐Eosin (H&E) staining of the scaffolds showed that, irrespectively of the specific type of seeded cells, they were well colonized by live cells and extensively vascularized; the presence of vessels was confirmed by immunostaining for CD31 (Fig. 5A, left plots). This evidence supports the hypothesis that soluble factors produced by the implanted MSCs, also comprising the RANKL cytokine, could reach the general circulation, thus possibly eliciting a biological effect. Of note, the cells populating the scaffolds were at least in part of donor origin, as demonstrated by GFP positive immunohistochemical staining in scaffolds initially seeded with transduced cells (Fig. 5B, left plots); it could be reasonably inferred, even though we have not formally proven, that the same will have occurred in WT MSC‐seeded scaffolds. In addition, a large number of cells found on the scaffolds were represented by F4/80+ macrophages from the host (Supporting Information Fig. S1).

Figure 5

Histological analysis of MSC‐seeded MgHA/Col scaffolds after 2 months implantation in Rankl mice. (A) Hematoxylin–Eosin staining and CD31 immunostaining on serial sections of decalcified scaffolds from the different groups of treatment. Scale bar: 100 μm. (B) GFP immunostaining on sections of decalcified scaffolds from the different groups of treatment. Scale bar: 50 μm.

Next, we assessed whether the implanted cell‐scaffold constructs affected the skeletal phenotype of Rankl mice. TRAP staining revealed the presence of TRAP+ cells specifically in the bone of Rankl mice implanted with a WT or LVhsRL‐transduced Rankl MSC‐seeded scaffold, while no TRAP+ cells were found in Rankl mice implanted with a mock‐transduced Rankl MSC‐seeded scaffold (Fig. 6A, left plots, and 6B), in accordance with previous reports on the absence of TRAP+ cells in the Rankl mouse model 9. This suggests that the hsRL molecule secreted by WT and LVhsRL‐transduced Rankl MSCs can induce to a certain extent formation of TRAP+ cells, which could be reasonably regarded as cells of the osteoclast lineage.

Figure 6

Evaluation of the effect of cell‐constructs implantation on the bone phenotype of Rankl mice. (A) TRAP staining on long bone of Rankl mice belonging to the different treatment groups. Scale bars: 50 μm (left); 20 μm (right). (B) Number of TRAP+ cells per bone section of treated Rankl mice. nd: not detected. (C) Measurement of serum total calcium concentration in treated Rankl mice. The red dashed line indicates the average concentration in age matched wild type mice. * p < .05.

To enhance the effect at the cellular level, we performed another group of experiments, in which 1.5 × 106 cells where seeded on each scaffold, with a seeding efficiency of about 80%, and 2 scaffolds were implanted in each Rankl mouse; after sacrifice we carried out the same evaluations as above. Histological analysis of the harvested cell‐scaffold constructs showed abundant vascularization and a more prominent presence of cells, comprising also of GFP+ ones, as expected based on the higher number of cells initially seeded (Fig. 5, right plots). Within the bone tissue, we found a clear increase in TRAP+ cells in the bone of Rankl mice implanted with WT MSC‐seeded scaffolds and even more in those implanted with LVhsRL‐transduced Rankl MSC‐seeded scaffolds, as compared with mice of the same treatment group with a single scaffold. On the other hand, TRAP+ cells were still completely absent in the control group (i.e., Rankl mice plus mock‐transduced Rankl MSC‐seeded scaffolds), as expected (Fig. 6A, right plots, and 6B). Serological analysis of bone‐related parameters showed a significant increase of total calcium in mice implanted with WT‐transduced and LVhsRL‐transduced Rankl MSC‐seeded scaffolds, even though physiological levels were not reached (Fig. 6C). Nonetheless, independent of the type of implanted construct, the classic osteopetrotic features were still present in the treated Rankl mice, as shown by H&E staining: bone was very dense, with cartilage remnants, and no clear evidence of remodeling and very few marrow cells (Fig. 7). Accordingly, no difference was found in serum TRAP activity among the groups (data not shown).

Figure 7

Histological analysis of bone after 2 months MSC‐seeded MgHA/Col scaffolds implantation in Rankl mice. H&E staining on sections of decalcified femurs from the different groups of treatment. Scale bar: 500 μm.

We also evaluated whether the in vivo implantation of these constructs, and in particular the continuous release of hsRL by LVhsRL‐transduced cells, caused any side effect. At sacrifice, no gross abnormality potentially related to the performed procedure was observed, nor were pathological signs found by standard histological analysis of selected organs, including liver, kidney, and lung (Supporting Information Fig. S2).

Discussion

The combination of biomaterials mimicking bone extracellular matrix and MSCs or engineered MSCs is a valid option for regenerative medicine and for cell‐based tissue engineering therapies 32.

In particular, MSCs might serve as long‐lasting reservoir of biologically active compounds 33, 34.

Accordingly, here we used a biocompatible hybrid scaffold composed of type I collagen and Magnesium‐doped HA, seeded with either murine WT or Rankl MSCs‐transduced with a lentiviral vector restoring RANKL production, and implanted in Rankl mice, to provide mice the missing essential osteoclastogenic factor. A scaffold with the same composition had been already used and reported to support in vivo MSC osteogenic differentiation 13, 35. In the present work, this composite was produced through an ad hoc modified procedure that allowed achieving features of natural bone on the mandatorily reduced scale (i.e., the same size as the well of a 96‐well plate) required by the small size of Rankl mice 9. Cross‐linked collagen type I fibrils, the main component of the osteoid in vivo, served as templates onto which the inorganic elements settled, thus forming a mineralized bone matrix. The presence of Mg2+ ions inside the nucleated HA lattice and the chemical interaction between the mineral and the organic phase constrained the nucleation of apatite and reduced its crystallinity. These features made the obtained hybrid highly biomimetic, especially with respect toyoung and immature bone, and favored its biological properties. In fact, previous studies 2, 13, 35 and the present work demonstrated that this kind of scaffold was bioactive, biodegradable, biocompatible, and easily recognized by cells, thanks to the high hydrophilicity and porosity, particularly in terms of macropores, which fostered cell adhesion, colonization, proliferation, and RANKL cytokine production, in agreement with reports in literature referring to different contexts 36, 37. Moreover, once implanted subcutaneously in mice, these scaffolds were extensively vascularized; in line with other findings 38, 39, this should have favored graft‐host interaction and MSCs survival, and supported the systemic distribution of soluble factors, likely comprising also RANKL, produced by the implanted cells.

Another strength of our approach is the optimization of murine MSC transduction with a lentiviral vector establishing continuous production of human soluble RANKL 13, which promoted osteoclastogenesis in vitro. Implantation of cell‐seeded scaffolds in Rankl mice led to TRAP+ cells formation in knock‐out mice receiving the implant of a single LVhsRL‐producing cell construct, indicating that the released cytokine was functional in vivo, too. In parallel, a similar result was not observed either in vitro or in vivo in the presence of mock‐transduced Rankl MSCs, further proving that the biological response elicited was dependent on the RANKL molecule expressed by the viral vector. We could not formally demonstrate the presence of hsRL in the sera of Rankl mice implanted with LVhsRL‐expressing constructs, but this was not surprising, as in other experimental settings a short half‐life of exogenous RANKL in the circulation has been reported 9, 27.

No major side effect of these implants was observed over the 2 month follow‐up period or at necropsy, indicating that this treatment was safe. On the other hand, the biological effect attained in Rankl mice was limited and no amelioration of the osteopetrotic phenotype was observed. These results prompted us to conceive a strategy that could possibly enhance the benefit gained on the skeletal tissue of Rankl mice by increasing the amount of cytokine delivered in vivo. To reach this goal, we increased the number of cells seeded on each scaffold and the number of cell constructs implanted in each mouse, even though no more than two of them could be inserted in the subcutaneous pouch on the back of Rankl mice because of their severe growth retardation 9. These changes to the protocol led to an increase in TRAP+ cell formation in the bones of Rankl mice receiving RANKL‐producing cell constructs, but again the skeletal defect was not improved. Thus, at present the pharmacological administration of soluble RANKL appears to be the most effective treatment for RANKL ARO 9, 10. Possible reasons for the failure of the approach herein described to correct the ARO‐phenotype of Rankl mice could be the limited amount of cytokine produced by WT and LVhsRL‐transduced Rankl MSCs 13; in the latter case, this was dependent on the used MOI. Another possible explanation could be the extensive colonization of the scaffold by immune cells of the host, in particular a high number of macrophages, which might have eliminated a significant fraction of the cells originally seeded 40. More substantial modifications of the protocol, than those used in the present study, would be necessary to improve the outcome of this approach. For example, we might consider increasing hsRL production by transduced cells, by using a higher MOI; using telomerase overexpression in LVhsRL‐transduced Rankl MSCs to augment their proliferation 41; implanting a higher number of scaffolds or larger scaffolds (as far as this is technically feasible in these small mice); using a biomimetic smart scaffold functionalized to enhance MSC attachment 42; isolating the system from the host cells by means of newly developed cell encapsulation systems, thus preventing its disruption 43. The optimization of these aspects might be pursued, for example, by exploiting the emerging technology of rechargeable devices containing 3D printed cell‐seeded functionalized scaffolds 44, which has already achieved promising results in other fields. Thus, the integration of the strengths of our strategy with these new tools will likely achieve a net improvement.

Conclusion

In this work, we have utilized a lentiviral vector for the stable expression of hsRL, which sustained in vitro human and mouse osteoclast differentiation. We have transduced Rankl MSCs and set up conditions for their 3D culture on an MgHA/Col biomimetic scaffold. In particular, the chemical and physical properties of this scaffold enhanced MSC proliferation and hsRL production. After implantation of these MSC‐seeded constructs in Rankl mice, TRAP+ cells formed in bone, thus providing proof of principle of the capacity of this approach to support cell differentiation towards the osteoclast lineage in vivo. Optimization of the experimental setting exploiting also the most recent biotechnological tools will increase the efficacy of this strategy on the bone compartment. As a perspective, we might pursue further implementation of this system using patients‐derived cells for a future possible autologous cell and gene therapy approach.

Author Contributions

C.M.: Conception and design, data collection and analysis, manuscript writing, and final approval; E.C., E.P., S.M., M.E.: Data collection and analysis, final approval of manuscript; A.I.: Data collection and analysis, final approval of manuscript; E.F.: Data analysis, final approval of manuscript; F.S.: Provision of study material, final approval of manuscript; R.v.H.: Data collection, final approval of manuscript; M.S.: Provision of study material, data collection and analysis, manuscript writing and final approval; A.T.: Provision of study material, final approval of manuscript; A.V.: Conception and design, financial support, final approval of manuscript; C.S.: Conception and design, data interpretation, manuscript writing, and final approval.

Disclosure of Potential Conflicts of Interest

The authors indicated no potential conflicts of interest.

Supporting Information Figure S1. Histological analysis of macrophages populating MSC‐seeded MgHA/Col scaffolds after 2 months implantation in Rankl mice. F4/80+ immunostaining on sections of decalcified scaffolds from the different groups of treatment. Scale bar: 200 μm; for the inset 100 μm.

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Supporting Information Figure S2. Histological analysis of the lung tissue after 2 months MSC‐seeded MgHA/Col scaffolds implantation in Rankl mice. H&E staining on sections from the different groups of treatment shows the presence of lymphoid aggregates, linked to the reported lack of lymph nodes in this mouse model. The fraction of lung parenchyma occupied by these structures was comparable in all groups and unchanged as compared to the untreated Rankl mouse. Scale bar: 500 μm.

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Supporting Information Table S1. Cell growth of WT, mock‐transduced and LVhsRL‐transduced <span class="Gene">Rankl MSC in 2D versus 3D culture overtime by MTT assay. Cell growth is expressed as mean fold increase values ± SEM compared to day 0.

Click here for additional data file.