Abstract
MicroRNAs emerge as critical post-transcriptional regulators in bone metabolism. We have previously reported in vitro that miR-21 promotes osteogenesis, while studies have also revealed miR-21 as a regulator of osteoclastogenesis and a promoter of osteoclast differentiation in vitro. However, in vivo data are still lacking in identifying skeletal function of miR-21, particularly its effects on osteoporosis. Here, using miR-21 knockout (miR-21−/−) mice, we investigated effects of miR-21 on bone development, bone remodeling and bone loss. Unexpectedly, miR-21−/− mice demonstrated normal skeletal phenotype in development and maintained osteoblastogenesis in vivo. Besides, miR-21−/− mice showed increased receptor activator of nuclear factor κB ligand (RANKL) and decreased osteoprotegerin (OPG) through miR-21 targeting Sprouty 1 (Spry1). Nevertheless, interestingly, miR-21 deficiency promoted trabecular bone mass accrual physiologically. Furthermore, in pathological states, the protection of bone mass was prominent in miR-21−/− mice. These skeletal effects were attributed to inhibition of bone resorption and osteoclast function by miR-21 deficiency through miR-21 targeting programmed cell death 4 (PDCD4), despite the existence of RANKL. As far as we know, this is the first in vivo evidence of a pro-osteoclastic microRNA. Together, these findings clarified function of miR-21 in bone metabolism, particularly uncovering osteo-protective potential of miR-21 inactivation in osteoporosis.
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Introduction
MicroRNAs post-transcriptionally modulate osteoblastogenesis and osteoclastogenesis and are emerging as critical regulators in bone homeostasis and diseases1,2. We and others have previously reported in vitro that miR-21 promoted osteogenesis of bone marrow mesenchymal stem cells (BMMSCs) by regulating downstream targets including Sprouty 1 (Spry1) and Sprouty 2 (Spry2)3,4. Previous in vitro studies have also revealed pro-osteoclastic function of miR-21 through regulating programmed cell death 4 (PDCD4)5, a functional target of miR-216, or by targeting Fas ligand (FasL)7. In addition, it has been reported that miR-21 could regulate receptor activator of nuclear factor κB ligand (RANKL) and osteoprotegerin (OPG), the key osteoblastic mediators of osteoclastogenesis8,9, in multiple myeloma-derived BMMSCs in vitro10. Interesting questions remain to be answered are that which effect predominates physiologically in vivo, and that whether miR-21 regulates skeletal phenotypes in both physiological and pathological states.
Studies have applied targeted delivery of specific antagomirs to modulate and detect skeletal effects of individual microRNAs11,12,13. In vivo function of microRNAs in bone could be further uncovered based on gene-manipulated mouse models13,14,15. In osteoporosis, as far as we know, participations of only miR-188 and miR-34a have been revealed in transgenic mice, respectively suppressing osteogenic differentiation of BMMSCs in age-related bone loss and inhibiting osteoclastogenesis in ovariectomy (OVX)-induced osteopenia13,14. Given in vitro promotive effects of miR-21 in osteogenesis and osteoclast differentiation3,5, elucidating in knockout mice the skeletal function of miR-21, particularly in the development of osteoporosis, is in an urgent need.
In this study, we surprisingly discovered that miR-21 knockout (miR-21−/−) mice demonstrated normal skeletal phenotype in development. However, postnatally, miR-21 deficiency promoted trabecular bone mass accrual and prevented bone loss induced by OVX and during aging. Moreover, we demonstrated that these skeletal effects were attributed to inhibited bone resorption and osteoclast function in mice lacking miR-21. Thus, our results clarified physiological and pathophysiological function of miR-21 in the bone metabolism and provided first in vivo evidence of a pro-osteoclastic microRNA.
Results
miR-21−/− mice demonstrate normal skeletal phenotype in development
miR-21−/− mice were sourced directly from the Jackson Laboratory, and the deficiency of miR-21 was further confirmed systemically (Supplementary Fig. S1a) and in bone (Supplementary Fig. S1b) without affecting the neighborhood of miR-21 gene loci, the gene Vacuole membrane protein-1 (VMP1) (Supplementary Fig. S1c,d)16,17.
To clarify skeletal effects of miR-21, we firstly investigated skeletal phenotypes of miR-21−/− embryos. To our surprise, miR-21−/− embryos at E18 appeared morphologically normal (Fig. 1a), with comparable body length to those of WT (Fig. 1b). Moreover, alizarin red staining at E18 demonstrated similar overall skeletal mineralization in WT and miR-21−/− embryos (Fig. 1c). Further observations showed that mineralized area in ribs, thoracic spines and lumbar spines of miR-21−/− embryos were as much as those of WT embryos (Fig. 1d). Quantitative analysis on L1-L4 mineralization did not detect significant difference (Fig. 1e). Also, WT and miR-21−/− embryos showed paralleled mineralized area in radius, ulna, carpus and digits (Fig. 1f,g).
Bone development is determined primarily by the bone modeling process, in which endochondral ossification is the mechanism whereby long bones are formed18,19. To further dissect the skeletal function of miR-21 in embryos, we analyzed the cartilage remnants and the ossification that are key to bone mass accrual, as previously reported15,20. Histological analyses illustrated comparable cartilaginous remnants, hypertrophic chondrocytes (Fig. 1h) and mineralization in tibia (Fig. 1i,j) of WT and miR-21−/− embryos at E18. These results indicated normal skeletal phenotype in development of miR-21−/− mice.
miR-21 regulates osteoblastogenesis and maintains bone formation in vivo
Given the normal skeletal phenotype of miR-21−/− embryos and the role of miR-21 as an osteogenesis promoter of BMMSCs in vitro3, we next examined effects of miR-21 in characteristics of BMMSCs ex vivo. We confirmed reduction of osteogenic differentiation of ex vivo miR-21−/− BMMSCs that may be attributed to SPRY1 up-regulation (Supplementary Fig. S2). However, we further discovered that primary miR-21−/− BMMSCs showed increased colony forming efficiency (Fig. 2a,b), and that miR-21−/− BMMSCs continued to show increased proliferation rate during passages (Fig. 2c). These results suggested that miR-21 inhibited colony formation and proliferation of BMMSCs despite promotion on osteogenesis.
We next investigated effects of miR-21 deficiency on osteoblastogenesis in vivo, by using toluidine blue staining for osteoblasts and calcein labeling for bone formation (Fig. 2d). Surprisingly, we revealed that number and surface of osteoblasts per bone surface were not significantly different between 3-month WT and miR-21−/− mice (Fig. 2e,f). We also revealed that bone formation parameters were comparable in WT and miR-21−/− mice (Fig. 2g,h). Furthermore, the level of a bone formation marker in serum, procollagen 1 N-terminal peptide (P1NP), in miR-21−/− mice was paralleled with that in WT mice. These findings highlighted that miR-21 maintained bone formation and osteoblastogenesis in vivo.
miR-21 deficiency promotes trabecular bone mass accrual postnatally
To further study the skeletal phenotype of miR-21−/− mice, we separately analyzed trabecular and cortical bone mass of WT and miR-21−/− mice using the micro-CT system. As shown, miR-21−/− mice had a slightly increased trabecular bone mass compared to WT mice at 3-month old (Fig. 3a). Quantifications on the trabecular bone volume (Fig. 3b) and bone mineral density (BMD) (Fig. 3c) confirmed that miR-21 deficiency promotes trabecular bone mass accrual. These changes were attributed to increases in the thickness and number of the trabecular bone (Fig. 3d,e), and a decrease in the separation of the trabecular bone (Fig. 3f), as shown by trabecular bone parameters. However, we did not detect differences in cortical bone mass between WT and miR-21−/− mice (Fig. 3g), provided the thickness and area of the cortical bone were comparable (Fig. 3h,i). Besides, WT and miR-21−/− mice showed similar body composition (Supplementary Table S1). These findings suggested that miR-21 functioned to suppress trabecular bone mass accrual postnatally.
miR-21 controls osteoclastogenesis by regulating RANKL and OPG
We next examined whether miR-21 regulates osteoclastogenesis to promote trabecular bone mass. The key osteoblastic mediators of osteoclastogenesis, RANKL8 and OPG9, were analyzed in vivo. Unexpectedly, enzyme-linked immunosorbent assay (ELISA) of serological levels demonstrated promoted RANKL and suppressed OPG by miR-21 deficiency (Fig. 4a,b), indicating stimulation of osteoclastogenesis. These effects were confirmed by corresponding changes in mRNA expression levels of RANKL and OPG in osteoblasts (Fig. 4c), and in their secretion of RANKL and OPG into culture media (Fig. 4d). Therefore, although we discovered modulatory effects of miR-21 on RANKL and OPG, these findings suggested that the increased postnatal trabecular bone mass in miR-21−/− mice was not attributed to changes of osteoclastogenesis.
To dissect the mechanism underlying miR-21 regulating RANKL and OPG in osteoblastic lineage cells, we tested if our previously established miR-21 target in BMMSCs, Spry13, is a regulator of both RANKL and OPG. Given that SPRY1 was up-regulated in miR-21-deficient osteoblastic lineage cells (Supplementary Fig. S2c,d), we applied small interfering RNA (siRNA) for SPRY1 (siSPRY1) in miR-21-deficient osteoblasts. Quantitative real-time polymerase chain reaction (qRT-PCR) analysis demonstrated successful down-regulation of SPRY1 mRNA level by siSPRY1, but not its negative control (NC) (Fig. 4e). Furthermore, siSPRY1 reduced RANKL and rescued OPG expression in miR-21-deficient osteoblasts (Fig. 4f), suggesting Spry1 is a functional target of miR-21 in regulating osteoclastogenesis.
We further explored the molecular mediator(s) downstream Spry1 to regulate RANKL and OPG, for Spry1 binding sites were not found in the promotor regions of RANKL and OPG, suggesting indirect modulating manners. Extracellular signal-regulated kinase (ERK) signaling has been reported to inhibit RANKL and promote OPG under mechanical force in fibroblasts21, and it has been proved to be regulated by miR-21 targeting Spry122,23. We confirmed in this study that siSPRY1 induced both ERK1/2 and p-ERK1/2 in miR-21-deficient osteoblasts (Fig. 4g). Using a pharmacological ERK inhibitor, PD98059, we further revealed that ERK inhibition could oppose effects of siSPRY1 on RANKL and OPG expression and moreover, the secretion, in miR-21-deficient osteoblasts (Fig. 4h,i). These findings collectively indicated that miR-21 regulates RANKL and OPG by targeting Spry1 to modulate ERK signaling in osteoblasts.
miR-21 promotes bone resorption in vivo and supports osteoclast function
The above data inspired us to further investigate whether the increased bone mass of miR-21−/− mice was directly attributed to impaired bone resorption and osteoclast function. As expected, depicted by tartrate resistant acid phosphotase (TRAP) staining, miR-21−/− mice showed inhibited bone resorption at 3-month old (Fig. 5a), which was attributed to declined parameters of the number and surface of osteoclasts in miR-21−/− mice (Fig. 5b,c). Analyses on the level of serological marker confirmed that miR-21 deficiency reduced the bone resorption rate, as shown by the cross linked C-telopeptide of type 1 collagen (CTX-1) (Fig. 5d) concentration.
To confirm effects of miR-21 in RANKL-induced osteoclast differentiation and activity, TRAP staining and resorption examination were respectively performed. We revealed that despite the existence of RANKL, miR-21 deficiency inhibited osteoclast differentiation, as shown by declined formation of TRAP+ multinucleated cells (Supplementary Fig. S3a,b). We further discovered that miR-21 deficiency reduced resorption activity of osteoclasts, as demonstrated by declined resorption pits on dentine slices (Fig. 5e,f).
PDCD4 was previously demonstrated to regulate osteoclast differentiation5 and was revealed as a direct target of miR-216. We next uncovered that the effects in miR-21−/− osteoclasts were indeed attributed to an increase of PDCD4 protein level (Fig. 5g), while the mRNA level of PDCD4 remained unchanged (Supplementary Fig. S3c), confirming miR-21 regulation of PDCD4 expression in osteoclasts at the posttranscriptional level. This targeted regulation of miR-21 on PDCD4 lead to down-regulation of both mRNA expression of c-FOS and its protein phosphorylation (p-c-fos) level (Fig. 5g, Supplementary Fig. S3d), which is a critical transcription factor for osteoclastogenesis5. In addition, we showed up-regulation of PDCD4 and down-regulation of p-c-fos in bone marrow of miR-21−/− mice (Supplementary Fig. S3e,f).
To further prove the role of PDCD4 in mediating effects of miR-21 on RANKL-induced osteoclast function, we applied siRNA for PDCD4 (siPDCD4) during miR-21-deficient osteoclast differentiation. qRT-PCR analysis demonstrated successful down-regulation of PDCD4 mRNA level by siPDCD4, but not its NC (Fig. 5h). Furthermore, under the existence of RANKL, siPDCD4 rescued both differentiation and resorption activity of miR-21-deficient osteoclasts, as shown by recovered formation of TRAP+ multinucleated cells (Supplementary Fig. S3g,h) and resorption pits on dentine slices (Fig. 5i,j). In addition, mRNA expression of c-FOS was also promoted by siPDCD4 (Supplementary Fig. S3i). These findings suggested PDCD4 is a functional target of miR-21 in supporting osteoclast function, collectively indicating that miR-21 promotes bone resorption in vivo through direct control of osteoclast function by targeting PDCD4.
miR-21 deficiency blocks OVX-induced osteopenia by inhibiting osteoclast function
We next investigated the pathophysiological role of miR-21 in estrogen deficiency-induced osteoporosis. Micro-CT analysis showed that miR-21 deficiency blocked OVX-induced osteopenia (Fig. 6a), and that both trabecular and cortical bone loss were prevented (Fig. 6b,c). These effects were not attributed to a rescue in osteoblastogenesis or bone formation in miR-21−/− mice (Supplementary Fig. S4a–c). Instead, OVX-induced bone resorption was prevented by miR-21 deficiency (Fig. 6d–f). The RANKL/OPG ratio was not significantly different between ovariectomized WT and miR-21−/− mice (Fig. 6g). However, both differentiation (Supplementary Fig. S4d,e) and resorption activity (Fig. 6h,i) of osteoclasts from ovariectomized miR-21−/− mice were impaired. We further revealed up-regulation of the miR-21 target PDCD4 protein level, which suppressed c-FOS and p-c-fos expression in osteoclasts from ovariectomized miR-21−/− mice, compared to those derived from ovariectomized WT mice (Fig. 6j, Supplementary Fig. S4f,g). We also confirmed that miR-21 targeted PDCD4 to modulate p-c-fos in vivo after OVX (Supplementary Fig. S4h,i). These findings highlighted that miR-21 deficiency blocks OVX-induced osteopenia by inhibiting osteoclast function through targeting PDCD4.
miR-21 contributes to age-related osteopenia and bone loss in human
To further determine whether miR-21 contributed to the development of osteoporosis, we examined effects of miR-21 deficiency in age-related osteopenia. Micro-CT analysis showed that miR-21−/− mice did not develop age-related osteopenia (Fig. 7a), and that both trabecular and cortical bone mass were maintained (Fig. 7b,c). Impairments were still detected in osteoblastogenesis and bone formation of aged miR-21−/− mice (Supplementary Fig. S5a–c). However, age-related elevation of bone resorption was prevented by miR-21 deficiency (Fig. 7d–f), which may be attributed to targeted regulation of PDCD4 that lead to p-c-fos up-regulation (Supplementary Fig. S5d,e). In addition, the RANKL/OPG ratio was comparable between aged WT and miR-21−/− mice (Fig. 7g). These results suggested that miR-21 contributed to the development of osteopenia during aging.
To identify the correlation of miR-21 changes with bone loss, we detected serological miR-21 levels in normal and osteoporotic mice and individuals. As depicted, the mean of serological relative miR-21 levels of osteoporotic mice was 4-fold higher compared to that of normal mice, and the difference was statistically significant (Fig. 7h). Similarly in human samples, serological relative miR-21 levels of osteoporotic individuals were significantly higher compared to that of normal individuals (Fig. 7i). Further analysis identified correlation of serological relative miR-21 levels with BMD of human lumbar spine in the development of osteoporosis (Pearson’s correlation: −0.5679; p = 0.0140) (Fig. 7j). These findings highlighted skeletal effects of miR-21 in correlation with bone homeostasis.
Discussion
Critical function of individual microRNAs in bone is emerging to be revealed13,14,15. Previous in vitro studies have shown that miR-21 regulates osteoclast differentiation5,7, osteoclastogenesis10 and osteogenesis of BMMSCs3,4. In the present study, we further discovered in vivo the protection of bone mass in miR-21−/− mice that was attributed to an inhibition of osteoclast function. Our results clarified skeletal function of miR-21 and provided first in vivo evidence of a pro-osteoclastic microRNA.
microRNAs post-transcriptionally modulate properties of both osteoclastic and osteoblastic lineage cells1,2. Function of microRNAs in osteoblastogenesis has been well established by numerous in vitro reports and several in vivo studies1,2,11,13,15,24. However, a few individual microRNAs have been demonstrated to regulate osteoclastogenesis2,5, among which only miR-34a was uncovered based on transgenic mouse models as a key osteoclast suppressor to confer skeletal protection14. Notably, miR-34b/c were revealed to specifically regulate osteoblastogenesis in bone15,24. This skeletal functional diversity of microRNAs from one family was further supported by findings of miR-21. miR-21 was previously reported as an osteogenesis promoter of BMMSCs by in vitro studies3,4 and in applied researches targeting miR-21 or downstream effectors to promote bone formation25,26. miR-21 was also documented in vitro as a microRNA expression signature of RANKL-induced osteoclast differentiation5 and to oppose pro-apoptotic effect of estrogen on mature osteoclasts7. In addition, it has been reported that miR-21 could regulate RANKL and OPG, the key osteoblastic mediators of osteoclastogenesis8,9, in multiple myeloma-derived BMMSCs in vitro10. Here, we clarified that the function of miR-21 in promoting osteoclast function predominated in vivo, despite that it maintained osteoblastogenesis, inhibited RANKL and promoted OPG physiologically. As far as we know, this is the first in vivo evidence of a pro-osteoclastic microRNA based on gene-manipulated animal models.
Correlations of microRNA function with bone diseases have just begun to emerge. With the targeted delivery of specific antagomirs to bone cells, inhibition of miR-148a, miR-188 and miR-214 restored bone mass in osteoporotic mice11,12,13. In transgenic mice, miR-188 was further revealed to regulate the switch between osteoblast and adipocyte differentiation in age-related bone loss13. Moreover, miR-34a overexpression in mice blocks osteoporosis and osteolytic bone metastasis14. In our previous research, we found that miR-21 in BMMSCs was regulated by tumor necrosis factor-alpha (TNF-α) in estrogen deficiency-induced bone loss ex vivo3. In this study, we further uncovered that lack of miR-21 in mice blocked osteopenia induced by OVX and during aging, suggesting protection of bone mass by miR-21 deficiency in pathological states. Our results also indicate the potential therapeutic effects of miR-21 inhibition on osteoporosis, which may be of clinical significance to investigate in future studies. We additionally demonstrated that serological miR-21 up-regulation was directly correlated with reduced BMD in human samples. Seeliger et al. also documented that expression of circulating and bone tissue miR-21 elevated in patients with osteoporotic fractures27. These findings highlighted potential values of miR-21 as both a therapeutic target and a biomarker for osteoporosis. For now, the source of serological miR-21 and its links with bone cells are still unknown, although we have detected the highest expression level of miR-21 in bone marrow among various tissues (data not shown). Our findings pave an avenue for further mechanistic researches on osteoclast-specific loss-of-function of miR-21 and miR-21 overexpression in skeletal disorders.
Interestingly, in the present study, we discovered ex vivo that miR-21 inhibited colony formation and proliferation of BMMSCs, while we confirmed its promotion on osteogenesis. Similarly, in mesenchymal stem cells derived from fetal amniotic fluid and adult adipose, overexpression of miR-21 in vitro suppressed proliferation while enhancing the differentiation potential28,29,30. The discrepancy of miR-21 effects in different functional aspects of BMMSCs lead to maintained bone formation and osteoblastogenesis in miR-21−/− mice, as shown by our findings. Previous studies have also revealed that miR-23a has limited roles in bone formation in vivo31, in spite of its involvement in osteogenic differentiation in vitro32. Another important finding of the present study is that miR-21 reduced RANKL and induced OPG secretion physiologically, but these effects were not observed in pathological states. In multiple myeloma-derived BMMSCs, it has recently been reported that miR-21 directly targeted to reduce OPG and indirectly promoted RANKL by targeting the signal transducer and activator of transcription 3 (STAT3) pathway, suggesting inhibition of osteoclastogenesis by miR-2110. During bone mass accrual physiologically, we discovered in osteoblasts that miR-21 targeted Spry1 to regulate ERK signaling, thus suppressing RANKL and elevating OPG, indicating promotion of osteoclastogenesis by miR-21. The discrepancy of miR-21 effects on RANKL and OPG might be attributed to the distinguished physiological or pathological states, mature or progenitor cells, and in vivo or in vitro differences that leads to activation of different functional targets and signaling pathways. For example, the miR-21-Spry1-ERK axis was documented pivotal under stress22, and ERK signaling has been reported to regulate RANKL and OPG under mechanical force21, which is of great significance to maintain bone homeostasis in vivo33,34. Therefore, considering that the dynamic regulation of an individual microRNA (miR-21) on its potential targets may vary depending on the experimental conditions/microenvironments, direct in vivo elucidation of its functional importance based on gene-manipulated animals is of necessity.
In summary, we discovered in vivo the prevention of bone loss in miR-21−/− mice that was attributed to an inhibition of osteoclast function. Our findings clarified skeletal function of miR-21 and provided first in vivo evidence of a pro-osteoclastic microRNA that regulates bone mass accrual and contributes to the development of osteoporosis.
Methods
Animals
All experimental protocols were approved by the Fourth Military Medical University. All animal experiments conducted in this research were performed in accordance with the guidelines of the Fourth Military Medical University Intramural Animal Use and Care Committee and met the NIH guidelines for the care and use of laboratory animals. WT C57BL/6 mice and miR-21−/− mice were sourced directly from the Jackson Laboratory. For embryonic experiments, WT (n = 6) and miR-21−/− (n = 6) embryos were separated at E18. For skeletal phenotype analysis during bone mass accrual, WT (n = 6, 3 female and 3 male) and miR-21−/− (n = 6, 3 female and 3 male) mice were sacrificed at 3-month old15. For skeletal phenotype analysis post estrogen deficiency, 2-month female WT and miR-21−/− mice underwent either a bilateral OVX (n = 6/genotype) or a Sham (n = 6/genotype) operation by the dorsal approach under general anesthesia3. Mice were modeled for 1 month and sacrificed at 3-month old. For age-related skeletal phenotype analysis, WT (n = 6, 3 female and 3 male) and miR-21−/− (n = 6, 3 female and 3 male) mice were sacrificed at 16-month old13. The mice were maintained with good ventilation and a 12-h light/dark cycle, and were kept feeding and drinking ad libitum.
Micro-CT analysis
For trabecular and cortical bone mass evaluation in mice, a desktop micro-CT system (eXplore Locus SP, GE Healthcare, USA) was employed35,36,37. At sacrifice, the left femora were isolated and fixed overnight in 4% paraformaldehyde. The distal femoral metaphysis were scanned at a resolution of 8 μm, a voltage of 80 kV, and a current of 80 μA. The region of interest (ROI) of the trabecular bone was defined from 0.1 mm to 2.6 mm away from the epiphysis. Cortical ROI was defined in the midshaft, from 3.5 mm to 4.0 mm away from the epiphysis. Data were analyzed with the Micview V2.1.2 software. Quantification of trabecular bone was performed using parameters of bone volume per tissue volume (BV/TV), BMD, trabecular thickness (Tb.Th), trabecular number (Tb.N), and trabecular separation (Tb.Sp)3. Quantification of cortical bone was performed using parameters of cortical thickness (Ct.Th) and cortical area fraction (Ct.Ar/Tt.Ar)38.
Bone histology and histomorphometry
Embryos at E18 were separated, photographed by a stereomicroscope (SZX9, Olympus, Japan), and measured for body length. For whole-mount skeletal mineralization examination, skeletons were dissected, fixed in 95% ethanol for 5 days, placed in acetone for 2 days, stained in 0.0005% alizarin red solution (Sigma-Aldrich, USA) at 37 °C for 3 days, cleared, and photographed by a stereomicroscope (SZX9, Olympus, Japan), according to standard protocols with minor modifications15,39. Quantification was performed using the ImageJ 1.47 software for percentages of mineralized area in the lumbar spines and digits, as stated15. For histological observations on cartilaginous and mineralized tissue in skeleton, after isolation of embryos, tibiae were dissected, fixed with 4% paraformaldehyde, and sagittally sectioned without decalcification (RM2125, Leica, Germany). Alcian blue (Sigma-Aldrich, USA) and von Kossa staining were performed using standard protocols15. Quantification was performed using the ImageJ 1.47 software from at least five microscopic fields.
For bone formation examination, double calcein labeling was performed according to previous studies with minor modifications3,37,40. At 16 day and 2 day prior to sacrifice, mice received double intraperitoneal injection of 20 mg/kg calcein (Sigma-Aldrich, USA). Calcein was dissolved at a concentration of 2 mg/ml in PBS supplemented with 1 mg/ml NaHCO3 (Sigma-Aldrich, USA), and was injected at 10 μl/g each time away from light. Necessary precautions were taken to ensure that the injected fluid was never accidentally placed in intestine, and that successful administration of double calcein labeling was accomplished in all mice. At sacrifice, the right femora were isolated, fixed in 80% ethanol, and embedded in methyl methacrylate without decalcification. The specimens were sagittally sectioned into 30-μm sections using a hard tissue slicing machine (SP1600, Leica, Germany) away from light. Both double-labeled and single-labeled cortical endosteum surfaces were evaluated by a fluorescence microscope (STP6000, Leica, Germany) with an excitation wavelength of 488 nm. Quantification was performed based on at least five photographs using the parameters of mineral apposition rate (MAR) and mineralized surface per bone surface (MS/BS). Bone formation rate (BFR) was calculated as MAR × MS/BS, according to standard methods40.
For osteoblast and osteoclast/bone resorption examination, toluidine blue and TRAP staining was respectively performed, as stated before15,40. At sacrifice, left tibiae were isolated, fixed with 4% paraformaldehyde, decalcified with 10% ethylene diamine tetraacetic acid (EDTA) (pH, 7.2–7.4), and embedded in paraffin. 5-μm sagittal serial sections of proximal metaphyses were prepared (RM2125, Leica, Germany). The sections were either stained by 1% toluidine blue (Sigma-Aldrich, USA) dissolved in PBS for 30 min, or underwent TRAP staining using a commercial kit according to the manufacturers’ instructions (Sigma-Aldrich, USA). Osteoblast quantification was determined using parameters of number of osteoblasts per bone surface (N.Ob/BS) and osteoblast surface per bone surface (Ob.S/BS). Similarly, osteoclast/bone resorption quantification was determined using parameters of number of osteoclasts per bone surface (N.Oc/BS) and osteoclast surface per bone surface (Oc.S/BS). Quantification was performed using the ImageJ 1.47 software from at least five microscopic fields.
Immunohistochemistry
Left tibiae were also used for in situ detection of miR-21 targets in bone marrow, according to published methods13. Sections were deparaffinized, treated by 0.25% trypsin (MP Biomedicals, USA) for 30 min at 37 °C for antigen retrieval, washed, and treated with 3% hydrogen peroxide for 20 min at 37 °C. Sections were blocked with 5% BSA (Sigma-Aldrich, USA) in PBS for 2 h in room temperature. Sections were then stained with either a rabbit anti-mouse PDCD4 primary antibody (Cell Signaling Technology, USA) or a rabbit anti-mouse p-c-fos primary antibody (Cell Signaling Technology, USA) overnight at 4 °C at both concentrations of 1:100, followed by a goat anti-rabbit secondary antibody (Cell Signaling Technology, USA) for 30 min in room temperature at a concentration of 1:200. Subsequently, an HRP-based Dako REALTM EnVisionTM Detection System (Dako, Denmark) was used to detect the immunoactivity, followed by counterstaining with hematoxylin (Sigma-Aldrich, USA). Negative control experiments were performed by omitting the primary antibodies. Quantification of number of positive stained cells over total area was performed using the ImageJ 1.47 software from at least five microscopic fields.
ELISA
Collected murine serum underwent ELISA using murine ELISA kits according to the manufacturers’ instructions (R&D Systems, USA)38. Markers of bone resorption (CTX-1), bone formation (P1NP), RANKL and OPG were detected for their serological levels. Ratio of RANKL/OPG was calculated. RANKL and OPG were also detected for their concentrations in conditional media of osteoblasts.
Human sample
Human sample collection and experiments were performed according to the Declaration of Helsinki in its newest version and published methods27,41. Serum specimens were obtained from patients with informed consent in Xijing Hospital that was pre-approved by the Fourth Military Medical University. Healthy donors and donors with postmenopausal osteoporosis were recruited. Exclusion criteria were tumors; diabetes; thyroid and parathyroid diseases; history of long-term hormone therapy; severe disorders in the digestive system; history of long-term immobilization; Cushing’s disease; history of liver and renal diseases; inflammation or auto-immune/inflammatory diseases; history of anti-osteoporotic medication; other metabolic endocrine diseases. The classification of osteoporosis was based on clinical dual-energy X-ray absorptiometry (DXA) for BMD of the lumbar spine. The characteristics of the included healthy donors (n = 9, female) and donors with postmenopausal osteoporosis (n = 9, female) were presented in Supplementary Table S2.
Serum sample processing and microRNA extraction
For human serum samples, donors were fasted for food and liquids overnight. 5-mL whole blood was sampled via median cubital vein in the morning. For murine serum samples, before necropsy, the peripheral whole blood was collected from the retro-orbital venous plexus at 500 μL under general anesthesia. The serum were isolated by centrifuging at 3000 rpm 10 min followed by 12000 rpm 10 min at 4 °C. microRNAs from serum were extracted using the miRNeasy Serum/Plasma Kit according to the manufacture’s recommendations (Qiagen, Germany), followed by phenol-chloroform extraction, as described27. cDNA synthesis was performed using reverse transcription primers from the Bulge-loopTM miRNA Primer Sets specific for murine and human miR-21 and RNU6 designed by RiboBio (Guangzhou, China), and PrimeScriptTM RT Reagent Kit (Takara, Japan)42,43.
Statistical analysis
Murine data are represented as the mean ± standard errors of the mean. Statistical significance was evaluated by two-tailed Student’s t test for two-group comparison, and by one way analysis of variation (ANOVA) followed by Newman-Keuls post-hoc tests for multiple comparisons. Human data are given as box plots showing 5th, 50th and 95th percentiles, and minimum to maximum ranges. Two-tailed Mann-Whitney U test was used to determine the significance. Pearson’s test was used to determine the correlation between BMD and miR-21 expression. All the statistical tests were performed using SPSS 17.0 software. Values of P < 0.05 were considered as statistically significant.
Additional Information
How to cite this article: Hu, C.-H. et al. miR-21 deficiency inhibits osteoclast function and prevents bone loss in mice. Sci. Rep. 7, 43191; doi: 10.1038/srep43191 (2017).
Publisher's note: Springer Nature remains neutral with regard to jurisdictional claims in published maps and institutional affiliations.
Change history
14 December 2022
A Correction to this paper has been published: https://doi.org/10.1038/s41598-022-25782-2
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Acknowledgements
This work was supported by grants from The National Natural Science Foundation of China (31301062 and 81271013).
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Study design: X.-R.Y. and Y.J. Study conduct: C.-H.H. and B.-D.S. Data collection: C.-H.H., B.-D.S., F.-Y.D. and S.Y. Data analysis: C.-H.H. Data interpretation: C.-H.H., B.-D.S., S.Y., P.Z. and Y.J. Drafting manuscript: C.-H.H. Revising manuscript: C.-H.H., B.-D.S., C.-X.Z. and Y.J. Approving final version of manuscript: X.-R.Y. and Y.J. C.-H.H. and Y.J. are responsible for the integrity of data analysis.
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Hu, CH., Sui, BD., Du, FY. et al. miR-21 deficiency inhibits osteoclast function and prevents bone loss in mice. Sci Rep 7, 43191 (2017). https://doi.org/10.1038/srep43191
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DOI: https://doi.org/10.1038/srep43191
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