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Aging impairs osteoblast differentiation of mesenchymal stem cells grown on titanium by favoring adipogenesis

ABSTRACT

Aging negatively affects bone/titanium implant interactions. Our hypothesis is that the unbalance between osteogenesis and adipogenesis induced by aging may be involved in this phenomenon.

Objective

We investigated the osteoblast and adipocyte differentiation of mesenchymal stem cells (MSCs) from young and aged rats cultured on Ti.

Material and Methods

Bone marrow MSCs derived from 1-month and 21-month rats were cultured on Ti discs under osteogenic conditions for periods of up to 21 days and osteoblast and adipocyte markers were evaluated.

Results

Cell proliferation, alkaline phosphatase (ALP) activity, extracellular matrix mineralization and gene expression of RUNX2, osterix, ALP, bone sialoprotein, osteopontin, and osteocalcin were reduced in cultures of 21-month rats compared with 1-month rats grown on Ti. Gene expression of PPAR-γ , adipocyte protein 2, and resistin and lipid accumulation were increased in cultures of 21-month rats compared with 1-month rats grown on the same conditions.

Conclusions

These results indicate that the lower osteogenic potential of MSCs derived from aged rats compared with young rats goes along with the higher adipogenic potential in cultures grown on Ti surface. This unbalance between osteoblast and adipocyte differentiation should be considered in dental implant therapy to the elderly population.

Aging; Osteoblasts; Adipocytes; Stem cells; Dental implants; Titanium

INTRODUCTION

Titanium (Ti) implants have been largely used in dentistry thanks to their physical properties and superior ability to osseointegrate22 - Albrektsson T, Brånemark PI, Hansson HA, Lindström J. Osseointegrated titanium implants. Requirements for ensuring a long-lasting, direct bone-to-implant anchorage in man. Acta Orthop Scand. 1981;52:155-70.. In addition to the implant characteristics, the clinical success of this treatment depends on several aspects such as surgical procedure, patient health conditions, and local bone quality and quantity44 - Berberi AN, Tehini GE, Noujeim ZF, Khairallah AA, Abousehlib MN, Salameh ZA. Influence of surgical and prosthetic techniques on marginal bone loss around titanium implants. Part I: immediate loading in fresh extraction sockets. J Prosthodont. 2014;23:521-7.,1010 - Holahan CM, Koka S, Kennel KA, Weaver AL, Assad DA, Regennitter FJ, et al. Effect of osteoporotic status on the survival of titanium dental implants. Int J Oral Maxillofac Implants. 2008;23:905-10.,2121 - Vehemente VA, Chuang SK, Daher S, Muftu A, Dodson TB. Risk factors affecting dental implant survival. J Oral Implantol. 2002;28:74-81..

The implantology research has been focused on the development of surface modifications that result in unique topography and chemical features that may regulate cell adhesion, proliferation and differentiation, and ultimately the interfacial tissue formation55 - Braem A, Chaudhari A, Vivan Cardoso M, Schrooten J, Duyck J, Vleugels J. Peri- and intra-implant bone response to microporous Ti coatings with surface modification. Acta Biomater. 2014;10:986-95.,66 - Castro-Raucci L, Francischini MS, Teixeira LN, Ferraz EP, Lopes HB, Oliveira PT, et al. Titanium with nanotopography induces osteoblast differentiation by regulating endogenous bone morphogenetic protein expression and signaling pathway. J Cell Biochem. 2015. doi: 10.1002/jcb.25469.
https://doi.org/10.1002/jcb.25469...
,99 - Heo YY, Um S, Kim SK, Park JM, Seo B. Responses of periodontal ligament stem cells on various titanium surfaces. Oral Dis. 2011;17:320-7.,1717 - Raimondo T, Puckett S, Webster TJ. Greater osteoblast and endothelial cell adhesion on nanostructured polyethylene and titanium. Int J Nanomedicine. 2010;5:647-52.,1818 - Rosa AL, Kato RB, Castro Raucci LM, Teixeira LN, Oliveira FS, Bellesini LS, et al. Nanotopography drives stem cell fate toward osteoblast differentiation through α1β1 integrin signaling pathway. J Cell Biochem. 2014;115:540-8.,2020 - Sverzut AT, Albuquerque GC, Crippa GE, Chiesa R, Della Valle C, Oliveira PT, et al. Bone tissue, cellular, and molecular responses to titanium implants treated by anodic spark deposition. J Biomed Mater Res A. 2012;100:3092-8.. Regarding the quality and amount of bone tissue, they are affected by various factors such as heart/vascular disease, estrogen deficiency, diabetes, and aging1212 - Khan MP, Singh AK, Joharapurkar AA, Yadav M, Shree S, Kumar H, et al. Pathophysiological mechanism of bone loss in type 2 diabetes involves inverse regulation of osteoblast function by PPARγ coactivator-1α and skeletal muscle atrogenes: adiponectin receptor 1 as a potential target for reversing diabetes-induced osteopenia. Diabetes. 2015;64:2609-23.,1515 - Macari S, Duffles LF, Queiroz-Junior CM, Madeira MF, Dias GJ, Teixeira MM, et al. Oestrogen regulates bone resorption and cytokine production in the maxillae of female mice. Arch Oral Biol. 2015;60:333-41.,1919 - Ruquet M, Maille G, Tavitian P, Tardivo D, Hüe O, Bonfil JJ. Alveolar bone loss and ageing: possible association with coronary heart diseases and/or severe vascular diseases. Gerodontology. 2014. doi: 10.1111/ger.12168.
https://doi.org/10.1111/ger.12168...
. Aging also increases the risk of bone fracture and impairs the healing process in humans and animal models88 - Giganti MG, Tresoldi I, Masuelli L, Modesti A, Grosso G, Liuni FM, et al. Fracture healing: from basic science to role of nutrition. Front Biosci. 2014;19:1162-75.,1313 - Lopas LA, Belkin NS, Mutyaba PL, Gray CF, Hankenson KD, Ahn J. Fractures in geriatric mice show decreased callus expansion and bone volume. Clin Orthop Relat Res. 2014;472:3523-32.,2222 - Yukata K, Xie C, Li TF, Takahata M, Hoak D, Kondabolu S, et al. Aging periosteal progenitor cells have reduced regenerative responsiveness to bone injury and to the anabolic actions of PTH 1-34 treatment. Bone. 2014;62:79-89.. It has been shown that the delay in fracture repair and the reduced bone volume in the healing site in aged mice is associated with a decreased proliferation of stem cells and a disrupted osteoblast differentiation1313 - Lopas LA, Belkin NS, Mutyaba PL, Gray CF, Hankenson KD, Ahn J. Fractures in geriatric mice show decreased callus expansion and bone volume. Clin Orthop Relat Res. 2014;472:3523-32.,2222 - Yukata K, Xie C, Li TF, Takahata M, Hoak D, Kondabolu S, et al. Aging periosteal progenitor cells have reduced regenerative responsiveness to bone injury and to the anabolic actions of PTH 1-34 treatment. Bone. 2014;62:79-89..

The effects of aging on bone repair indicate that the process of Ti implant osseointegration could also be regulated by the age of the patient. Indeed, the number of mineralized nodules and the calcium content were reduced in osteoblasts derived from old patients compared with young patients when cultured on Ti surface2323 - Zhang H, Aronow MS, Gronowicz GA. Transforming growth factor-beta 1 (TGF-beta1) prevents the age-dependent decrease in bone formation in human osteoblast/implant cultures. J Biomed Mater Res A. 2005;75:98-105.. Corroborating this finding, the alkaline phosphatase (ALP) activity and osteocalcin (OC) expression were downregulated in osteoblasts derived from aged rats compared with young ones when they were grown on Ti surface with different surface topographies1616 - Olivares-Navarrete R, Raines AL, Hyzy SL, Park JH, Hutton DL, Cochran DL, et al. Osteoblast maturation and new bone formation in response to titanium implant surface features are reduced with age. J Bone Miner Res. 2012;27:1773-83.. Furthermore, a discrete but significant decrease in bone-to-implant contact was observed in one of the Ti surfaces placed into mouse femurs1616 - Olivares-Navarrete R, Raines AL, Hyzy SL, Park JH, Hutton DL, Cochran DL, et al. Osteoblast maturation and new bone formation in response to titanium implant surface features are reduced with age. J Bone Miner Res. 2012;27:1773-83..

Despite the clear evidences of the negative effects of aging on osteoblast and bone tissue interactions with Ti implants, the mechanisms behind this phenomenon have not been fully understood yet. Then, we hypothesized that the unbalance between osteogenesis and adipogenesis induced by aging may be one of the factors involved in the reduced osteoblast response to Ti surfaces. Thus, in the present study, we investigated the osteoblast and adipocyte differentiation of mesenchymal stem cells (MSCs) derived from bone marrow of young and aged rats cultured on Ti surface.

MATERIAL AND METHODS

Preparation of Ti discs

Discs of commercially pure grade 2 Ti (Realum, São Paulo, SP, Brazil) with 12 mm in diameter and 1.5 mm thick were polished using 320 and 600 grit silicon carbide, cleaned by sonication and rinsed with toluene and deionized H2O several times, autoclaved and air-dried as previously described1818 - Rosa AL, Kato RB, Castro Raucci LM, Teixeira LN, Oliveira FS, Bellesini LS, et al. Nanotopography drives stem cell fate toward osteoblast differentiation through α1β1 integrin signaling pathway. J Cell Biochem. 2014;115:540-8..

Cell culture

The Committee of Ethics in Animal Research approved all animal procedures performed during the experiments (Approval number: 11.1.890.53.0). Bone marrow MSCs were obtained from the tibiae of 1-month and 21-month female Wistar rats and cultured in growth medium consisting of α-MEM (Invitrogen-Gibco, Grand Island, NY, USA) supplemented with 15% fetal bovine serum (Gibco), 50 µg/mL gentamycin (Gibco), 50 µg/mL vancomycin (Acros Organics, Geel, Belgium), and 0.3 µg/mL fungizone (Gibco) until reaching subconfluence. Then, MSCs were cultured in osteogenic medium containing growth medium plus 5 µg/ml ascorbic acid (Gibco), 7 mM β-glycerophosphate (Sigma-Aldrich, St. Louis, MO, USA), and 10-7 M dexamethasone (Sigma) on Ti discs for periods of up to 21 days. During the culture period, cells were incubated at 37°C in a humidified atmosphere of 5% CO2, and the medium was changed every three days.

Cell proliferation

Cell proliferation was evaluated at days 4, 7, and 10 with 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT, Sigma-Aldrich). Cultures were incubated with 2 mL of MTT (5 mg/ml) in phosphate-buffered saline at 37°C. After 4 h, the solution was removed and 1 mL of acid isopropanol (0.04 N HCl in isopropanol) was added. After shaking for 5 min, 150 µL of this solution was used to read the optical density at 570 nm (µQuant, Bio-Tek, Winooski, VT, USA). Data were obtained in quintuplicate (n=5) and expressed as absorbance.

Alkaline phosphatase (ALP) activity

Alkaline phosphatase activity was determined at days 4, 7, and 10 by measuring the release of thymolphthalein from thymolphthalein monophosphate using a commercial kit (Labtest Diagnostica SA, Lagoa Santa, MG, Brazil). Briefly, 50 μL of thymolphthalein monophosphate was mixed with 0.5 mL of 0.3 M diethanolamine buffer, pH 10.1, and kept for 2 min at 37°C before the addition of 50 μL of cell lysates obtained by five cycles of thermal shock (-20°C for 20 min and 37°C for 15 min). Then, after 10 min at 37°C, the reaction was stopped by adding 2 mL of Na2CO3 (0.09 mmol/mL) and NaOH (0.25 mmol/mL) solution, and the optical density was measured at 590 nm (µQuant, Bio-Tek). Data were obtained in quintuplicate (n=5) and expressed as ALP activity normalized by total protein content, which was determined by the Lowry method1414 - Lowry OH, Rosebrough NJ, Farr AL, Randall RJ. Protein measurement with the Folin phenol reagent. J Biol Chem. 1951;193:265-75..

Extracellular matrix mineralization

Extracellular matrix mineralization was detected at day 21 by alizarin red staining (Sigma-Aldrich). Cells were fixed in 10% formalin for 2 h at room temperature, dehydrated and stained with 2% alizarin red pH 4.2 (Sigma-Aldrich) for 10 min. For qualitative analysis, culture images were captured with a high-resolution digital camera (Canon EOS Digital Rebel Camera, Canon, Lake Success, NY, USA). Then, calcium content was evaluated using a colorimetric method. Briefly, 280 μL of 10% acetic acid was added to each well stained with alizarin red, and the plate was incubated at room temperature for 30 min under shaking. The slurry was overlaid with 100 μL of mineral oil (Sigma-Aldrich), heated to 85°C for 10 min and transferred to ice for 5 min. The slurry was then centrifuged at 20,000 g for 15 min, and 100 μL of supernatant was transferred to a microcentrifuge tube with 40 μL of 10% ammonium hydroxide to neutralize the acid. The optical density was read at 405 nm (µQuant, Bio-Tek), and data were obtained in quintuplicate (n=5) and expressed as absorbance.

Gene expression

Quantitative real-time polymerase chain reaction (PCR) was performed on day 10 to evaluate the gene expression of runt-related transcription factor 2 (RUNX2), osterix (OSX), ALP, bone sialoprotein (BSP), OC, osteopontin (OPN), peroxisome proliferator-activated receptor (PPAR-γ), adipocyte protein 2 (aP2), and resistin (RTN). Total RNA was extracted with Trizol reagent (Life-Technologies, Grand Island, NY, USA), and the concentration was determined by reading the optical density at the following different wavelengths: 260, 280, 230, and 320 nm (GE Healthcare, Milwaukee, WI, USA). Complementary DNA (cDNA) was synthesized using 1 µg of RNA through a reverse transcription reaction (Life Technologies-Applied Biosystems, Warrington, UK) according to the manufacturer’s instructions. Real-time PCR was performed in a CFX96 Real-Time PCR Detection System (Bio-Rad Laboratories, Philadelphia, PA, USA) using TaqMan (Applied Biosystems) probes for the target genes. The standard PCR conditions were 50°C (2 min), 95°C (10 min), 40 cycles of 95°C (15 s), and 60°C (1 min). The relative gene expression was calculated in relation to glyceraldehyde-3-phosphate dehydrogenase (GAPDH) expression and its respective control using the cycle threshold (Ct) method. This assay was performed in quadruplicate (n=4).

Lipid accumulation

Lipid accumulation was detected at day 21 by oil red O (Sigma-Aldrich). Cells were fixed in 10% formalin for 2 h at room temperature, washed with isopropanol 60% (Merck-Germany) and stained with 0.3% oil red O (Sigma-Aldrich) for 10 min. For qualitative analysis, culture images were captured with a high-resolution digital camera (Canon EOS Digital Rebel Camera, Canon) and the lipid accumulation was measured using a colorimetric assay. The incorporated oil red O (Sigma-Aldrich) was extracted by incubation with 100% isopropanol for 10 min under shaking at room temperature. After appropriate dilution, this solution was read at 500 nm in a plate reader μQuant (BioTek), and the data were obtained in quintuplicate (n=5) and expressed as absorbance.

Statistical analyses

The results are expressed as the mean±standard deviation and data obtained in three time-points were analyzed using two-way ANOVA followed by Student Newman Keuls post hoc test. Data obtained in one time-point were analyzed using Student’s t-test. For all experiments the level of significance was set at p≤0.05.

RESULTS

Cell proliferation

Cell proliferation was higher in cultures from 1-month rats compared with 21-month rats at all evaluated time-points (p=0.001 for all periods; Figure 1A). Moreover, the cell number increased (p=0.001) over time in cultures from 1-month rats, while no significant difference (p=0.127) was observed between 7 and 10 days in cultures from 21-month rats (Figure 1A).

Figure 1
Proliferation (A) and alkaline phosphatase (ALP) activity at days 4, 7, and 10 (B) and extracellular matrix mineralization at day 21 (C) of cultures from 1-month and 21-month rats grown on Ti discs. Data are presented as the mean±standard deviation (n=5). * indicates significant differences between cells from 1-month and 21-month rats within each time point (p≤0.05)

ALP activity

Cells from 1-month rats showed higher ALP activity compared with cells from 21-month rats at 7 and 10 days (p=0.001 for both time-points), while no significant difference (p=0.561) was observed at 4 days (Figure 1B). In addition, the ALP activity increased (p=0.001) over time in cultures from 1-month rats, while no significant difference (p>0.151) was observed between 4, 7, and 10 days in cultures from 21-month rats (Figure 1B).

Extracellular matrix mineralization

Extracellular calcium deposits were detected on Ti discs irrespective of cell source, with cells from 1-month rats producing the most dense and regularly distributed matrix (Figure 1C). Additionally, the calcium content was nearly five times higher (p=0.001) in cultures from 1-month rats compared with 21-month rats (Figure 1C).

Gene expression

The gene expression of all evaluated bone markers, RUNX2 (Figure 2A), OSX (Figure 2B), ALP (Figure 2C), BSP (Figure 2D), OPN (Figure 2E), and OC (Figure 2F) was higher (p=0.001 for all genes) in cultures from 1-month rats compared with 21-month rats. On the other hand, the gene expression of all evaluated adipose tissue markers, PPAR-γ (p=0.007; Figure 3A), aP2 (p=0.050; Figure 3B), and RTN (p=0.001; Figure 3C) was higher in cultures from 21-month rats compared with 1-month rats.

Figure 2
Gene expression at day 10 of the bone markers, RUNX2 (A), OSX (B), ALP (C), BSP (D), OPN (E), and OC (F) of cells from 1-month and 21-month rats grown on Ti discs. Data are presented as the mean±standard deviation (n=4). * indicates statistically significant differences between cells from 1-month and 21-month rats (p≤0.05)

Figure 3
Gene expression at day 10 of the adipose tissue markers, PPAR-γ (A), aP2 (B), and RTN (C) of cells from 1-month and 21-month rats grown on Ti discs. Data are presented as the mean±standard deviation (n=4). * indicates statistically significant differences between cells from 1-month and 21-month rats (p≤0.05)

Lipid accumulation

Lipid accumulation was detected on Ti discs irrespective of cell source, with cells from 21-month rats producing the most dense lipid droplets (Figure 3). Additionally, the lipid content was nearly twice higher (p=0.010) in cultures from 21-month rats compared with 1-month rats (Figure 4).

Figure 4
Lipid accumulation at day 21 of cultures from 1-month and 21-month rats grown on Ti discs. Data are presented as the mean±standard deviation (n=5). * indicates statistically significant differences between cells from 1-month and 21-month rats (p≤0.05)

DISCUSSION

The present study was designed to investigate if disruption of the balance between osteogenesis and adipogenesis induced by aging may be one of the factors involved in the reduced osteoblast response to Ti surfaces. Our results showed that MSCs derived from 21-month rats exhibit lower osteogenic and higher adipogenic potential compared with MSCs derived from 1-month rats when cultured on Ti surface under osteogenic conditions.

The capacity to expand is a key feature of the osteoblastic cells in order to colonize the implant surface, and distinct results are reported regarding the effect of aging on cell proliferation33 - Baker N, Boyette LB, Tuan RS. Characterization of bone marrow-derived mesenchymal stem cells in aging. Bone. 2015;70:37-47.. Here, we observed a relevant decrease in the proliferation activity of cells from 21-month rats compared with 1-month rats cultured on Ti surface at all evaluated time-points. According to this result, a reduced cell number in osteoblast cultures derived from the calvaria of old rats compared with young ones was observed1616 - Olivares-Navarrete R, Raines AL, Hyzy SL, Park JH, Hutton DL, Cochran DL, et al. Osteoblast maturation and new bone formation in response to titanium implant surface features are reduced with age. J Bone Miner Res. 2012;27:1773-83.. In contrast, MSCs from young and aged rats exhibited similar proliferation rate when cultured on polystyrene in a non-inducing differentiation medium77 - Geißler S, Textor M, Kühnisch J, Könnig D, Klein O, Ode A, et al. Functional comparison of chronological and in vitro aging: differential role of the cytoskeleton and mitochondria in mesenchymal stromal cells. PLoS One. 2012;7(12):e52700.. Such discrepancies may be related to the use of cells in different stages of differentiation and culture conditions, since the studies were conducted with either osteoblastic cells in osteogenic medium or MSCs in growth medium.

Another relevant characteristic of osteoblastic cells to interact with implants is the ability to complete the differention process and to synthesize an extracellular matrix that will be subsenquently mineralized. In this study, all evaluated markers of osteoblast genotype and phenotype expression were higher in cultures derived from 1-month rats compared with 21-month rats, including gene expression of RUNX2, OSX, ALP, BSP, OPN and OC, ALP activity and extracellular matrix mineralization. Corroborating our findings, a reduced number of mineralized nodules and calcium content were noticed in osteoblasts derived from old patients compared with young ones grown on Ti surface2323 - Zhang H, Aronow MS, Gronowicz GA. Transforming growth factor-beta 1 (TGF-beta1) prevents the age-dependent decrease in bone formation in human osteoblast/implant cultures. J Biomed Mater Res A. 2005;75:98-105.. Furthermore, a low osteogenic potential induced by aging was demonstrated in vivo in mice and in vitro in cells from rats in response to different Ti surfaces1616 - Olivares-Navarrete R, Raines AL, Hyzy SL, Park JH, Hutton DL, Cochran DL, et al. Osteoblast maturation and new bone formation in response to titanium implant surface features are reduced with age. J Bone Miner Res. 2012;27:1773-83..

The reduced osteoblast differentiation of MSCs grown on Ti surface induced by aging was paralleled by an increased genotype and phenotype expression level of adipocyte markers, such as higher gene expression of PPAR-γ, aP2, and RTN, and more lipid accumulation, the later not reported in studies investigating the effect of aging on the interaction between osteoblasts and Ti1616 - Olivares-Navarrete R, Raines AL, Hyzy SL, Park JH, Hutton DL, Cochran DL, et al. Osteoblast maturation and new bone formation in response to titanium implant surface features are reduced with age. J Bone Miner Res. 2012;27:1773-83.,2323 - Zhang H, Aronow MS, Gronowicz GA. Transforming growth factor-beta 1 (TGF-beta1) prevents the age-dependent decrease in bone formation in human osteoblast/implant cultures. J Biomed Mater Res A. 2005;75:98-105.. In contrast with this finding, it was reported that there were no differences between MSCs from young and aged rats in terms of osteoblast and adipocyte differentiation; however, this study evaluated cells obtained from 3-week and 12-month rats cultured on polystyrene under osteogenic and adipogenic conditions, respectively77 - Geißler S, Textor M, Kühnisch J, Könnig D, Klein O, Ode A, et al. Functional comparison of chronological and in vitro aging: differential role of the cytoskeleton and mitochondria in mesenchymal stromal cells. PLoS One. 2012;7(12):e52700.. It is worth noting that, in our study, cells were cultured only in osteogenic medium on Ti surface, indicating that even in a non-adipogenic milieu aging may disrupt the balance between osteoblast and adipocyte differentiation in favor of adipogenesis. Also, it has been shown that adipocytes inhibit the osteoblast phenotype expression by releasing tumor necrosis factor alpha to the tissue environment11 - Abuna RP, Oliveira FS, Santos TS, Guerra TR, Rosa AL, Beloti MM. Participation of TNF-α in inhibitory effects of adipocytes on osteoblast differentiation. J Cell Physiol. 2016;231:204-14.. These findings are of relevance from the clinical perspective as the process of Ti implant osseointegration occurs in a more osteogenic environment than in an adipogenic one.

The unbalance between osteoblast and adipocyte differentiation induced by aging could be related to the extracellular signal-regulated kinase 1/2 (ERK 1/2) that acts as a switch for the reciprocal regulation of osteogenesis and adipogenesis by modulating RUNX2 and PPAR-γ expression and/or activity1111 - Jung HS, Kim YH, Lee JW. Duration and magnitude of extracellular signal-regulated protein kinase phosphorylation determine adipogenesis or osteogenesis in human bone marrow-derived stem cells. Yonsei Med J. 2011;52:165-72.. While ERK 1/2 phosphorylation is sustained during osteoblast differentiation, it is transient and decreased during adipocyte differentiation of human MSCs, suggesting that a reduced ERK 1/2 activation favors adipogenesis1111 - Jung HS, Kim YH, Lee JW. Duration and magnitude of extracellular signal-regulated protein kinase phosphorylation determine adipogenesis or osteogenesis in human bone marrow-derived stem cells. Yonsei Med J. 2011;52:165-72.. However, further studies are necessary to investigate the participation of ERK 1/2 on the reduced osteoblast differentiation of MSCs cultured on Ti surface induced by aging.

CONCLUSIONS

The results of our study indicate that the reduced osteogenic potential of MSCs derived from aged rats compared with young ones goes along with the increased adipogenic potential in cultures grown on Ti surface. In this context, the unbalance between osteoblast and adipocyte differentiation should be taken into consideration in dental implant therapy to the older-adult population.

ACKNOWLEDGMENTS

This research was supported by a grant from FAPESP - São Paulo Research Foundation (grant no. 2012/01291-6) and from CNPq - National Council for Scientific and Technological Development (grant no. 153364/2012-2). Fabiola S. Oliveira, Milla S. Tavares, and Roger R. Fernandes are acknowledged for their technical assistance during these experiments.

REFERENCES

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    - Baker N, Boyette LB, Tuan RS. Characterization of bone marrow-derived mesenchymal stem cells in aging. Bone. 2015;70:37-47.
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    - Braem A, Chaudhari A, Vivan Cardoso M, Schrooten J, Duyck J, Vleugels J. Peri- and intra-implant bone response to microporous Ti coatings with surface modification. Acta Biomater. 2014;10:986-95.
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    - Castro-Raucci L, Francischini MS, Teixeira LN, Ferraz EP, Lopes HB, Oliveira PT, et al. Titanium with nanotopography induces osteoblast differentiation by regulating endogenous bone morphogenetic protein expression and signaling pathway. J Cell Biochem. 2015. doi: 10.1002/jcb.25469.
    » https://doi.org/10.1002/jcb.25469
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    - Giganti MG, Tresoldi I, Masuelli L, Modesti A, Grosso G, Liuni FM, et al. Fracture healing: from basic science to role of nutrition. Front Biosci. 2014;19:1162-75.
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    - Heo YY, Um S, Kim SK, Park JM, Seo B. Responses of periodontal ligament stem cells on various titanium surfaces. Oral Dis. 2011;17:320-7.
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    - Jung HS, Kim YH, Lee JW. Duration and magnitude of extracellular signal-regulated protein kinase phosphorylation determine adipogenesis or osteogenesis in human bone marrow-derived stem cells. Yonsei Med J. 2011;52:165-72.
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    - Khan MP, Singh AK, Joharapurkar AA, Yadav M, Shree S, Kumar H, et al. Pathophysiological mechanism of bone loss in type 2 diabetes involves inverse regulation of osteoblast function by PPARγ coactivator-1α and skeletal muscle atrogenes: adiponectin receptor 1 as a potential target for reversing diabetes-induced osteopenia. Diabetes. 2015;64:2609-23.
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    - Lopas LA, Belkin NS, Mutyaba PL, Gray CF, Hankenson KD, Ahn J. Fractures in geriatric mice show decreased callus expansion and bone volume. Clin Orthop Relat Res. 2014;472:3523-32.
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    - Lowry OH, Rosebrough NJ, Farr AL, Randall RJ. Protein measurement with the Folin phenol reagent. J Biol Chem. 1951;193:265-75.
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    - Macari S, Duffles LF, Queiroz-Junior CM, Madeira MF, Dias GJ, Teixeira MM, et al. Oestrogen regulates bone resorption and cytokine production in the maxillae of female mice. Arch Oral Biol. 2015;60:333-41.
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    - Olivares-Navarrete R, Raines AL, Hyzy SL, Park JH, Hutton DL, Cochran DL, et al. Osteoblast maturation and new bone formation in response to titanium implant surface features are reduced with age. J Bone Miner Res. 2012;27:1773-83.
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    - Raimondo T, Puckett S, Webster TJ. Greater osteoblast and endothelial cell adhesion on nanostructured polyethylene and titanium. Int J Nanomedicine. 2010;5:647-52.
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    - Rosa AL, Kato RB, Castro Raucci LM, Teixeira LN, Oliveira FS, Bellesini LS, et al. Nanotopography drives stem cell fate toward osteoblast differentiation through α1β1 integrin signaling pathway. J Cell Biochem. 2014;115:540-8.
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    - Ruquet M, Maille G, Tavitian P, Tardivo D, Hüe O, Bonfil JJ. Alveolar bone loss and ageing: possible association with coronary heart diseases and/or severe vascular diseases. Gerodontology. 2014. doi: 10.1111/ger.12168.
    » https://doi.org/10.1111/ger.12168
  • 20
    - Sverzut AT, Albuquerque GC, Crippa GE, Chiesa R, Della Valle C, Oliveira PT, et al. Bone tissue, cellular, and molecular responses to titanium implants treated by anodic spark deposition. J Biomed Mater Res A. 2012;100:3092-8.
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    - Vehemente VA, Chuang SK, Daher S, Muftu A, Dodson TB. Risk factors affecting dental implant survival. J Oral Implantol. 2002;28:74-81.
  • 22
    - Yukata K, Xie C, Li TF, Takahata M, Hoak D, Kondabolu S, et al. Aging periosteal progenitor cells have reduced regenerative responsiveness to bone injury and to the anabolic actions of PTH 1-34 treatment. Bone. 2014;62:79-89.
  • 23
    - Zhang H, Aronow MS, Gronowicz GA. Transforming growth factor-beta 1 (TGF-beta1) prevents the age-dependent decrease in bone formation in human osteoblast/implant cultures. J Biomed Mater Res A. 2005;75:98-105.

Publication Dates

  • Publication in this collection
    Jul-Aug 2016

History

  • Received
    16 Feb 2016
  • Reviewed
    30 Mar 2016
  • Accepted
    31 Mar 2016
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