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ISRN Stem Cells
Volume 2013 (2013), Article ID 138704, 9 pages
Low-Frequency Mechanical Stimulation Modulates Osteogenic Differentiation of C2C12 Cells
1Soft Tissue Biophysics Laboratory, Department of Chemical Engineering, McGill University, 3610 University Street, Montreal, QC, Canada H3A 0C5
2Faculty of Dentistry, McGill University, Montreal, QC, Canada H3A 0C5
Received 12 December 2012; Accepted 19 January 2013
Academic Editors: A. Chapel, C. Dong, S. M. Hwang, and B. Machalinski
Copyright © 2013 Ghazaleh Khayat et al. This is an open access article distributed under the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
Mechanical stimulation influences stem cell differentiation and may therefore provide improved lineage specification control for clinical applications. Low-frequency oscillatory mechanical stimulation (0.01 Hz) has recently been shown to suppress adipogenic differentiation of mesenchymal stem cells, indicating that the range of effective stimulation frequencies is not limited to those associated with locomotion, circulation, and respiration. We hypothesized that low-frequency mechanical stimulation (0.01 Hz) can also promote osteogenic cell differentiation of myoblastic C2C12 cells in combination with BMP-2. Results indicate that low-frequency mechanical stimulation can significantly enhance osteogenic gene expression, provided that differentiation is initiated by a priming period involving BMP-2 alone. Subsequent application of low-frequency mechanical stimulation appears to act synergistically with continued BMP-2 exposure to promote osteogenic differentiation of C2C12 cells and can even partially compensate for the removal of BMP-2. These effects may be mediated by the ERK and Wnt signalling pathways. Osteogenic induction of C2C12 cells by low-frequency mechanical stimulation is therefore critically dependent upon previous exposure to growth factors, and the timing of superimposed BMP-2 and mechanical stimuli can sensitively influence osteogenesis. These insights may provide a technically simple means for control of stem cell differentiation in cell-based therapies, particularly for the enhancement of differentiation toward desired lineages.
Stem cell differentiation to bone is important to growth, development, and tissue maintenance; understanding of the cellular processes underlying osteogenesis is necessary for the development of cell-based therapies. Growth factor stimulation of stem cells is an initiating event which activates transcription factors that subsequently drive lineage specification. Bone-inducing agents  called bone morphogenetic proteins (BMPs) [2, 3] comprise a superfamily of growth factors that drive bone differentiation and adult bone maintenance. Among the BMP superfamily, BMP-2 is known to have a critical role in inducing osteogenic differentiation of mesenchymal stem cells . Genes which are direct targets of BMP-2 include the transcription factors Runx2 and osterix, the matrix-associated proteins osteopontin and osteocalcin, and the osteogenic enzyme alkaline phosphatase . It has also been established that the time course and duration of growth factor stimulation can have important effects on differentiation , and moreover BMP-2 efficacy is dose dependent .
In addition to the growth factor stimulation, mechanical stimulation can also affect osteogenic differentiation of stem cells [8, 9]. Intracellular signalling pathways induced by mechanical stimulation in neurosensory and vascular cells can induce physiological responses which are much more rapid  than those induced by growth factors which can require minutes to hours . Furthermore, downstream signalling events overlap between the two types of stimulation, potentially resulting in interactions between chemical and mechanical cues [12, 13]. Mechanical stimulation utilizing amplitudes and frequencies consistent with the fundamental frequencies of locomotion (0.1–1 Hz) can induce osteogenic differentiation [14, 15]. However, stimulation frequencies below this range have not been extensively studied in the context of osteogenesis, though they have been found effective in modulating differentiation of mesenchymal stem cells . Since lower-frequency mechanical stimulation is often technically easier to apply, study of the effects of low-frequency mechanical stimulation may create new avenues for integration of mechanical stimulation into protocols for stem cell differentiation in cell-based therapies.
Since mechanotransduction alone can enhance bone formation [17, 18] while BMP-2 is known to effectively drive osteogenesis, our goals were to explore the extent to which the complementary mechanisms interact during during osteogenic differentiation. Specifically, these stimuli were applied either together or in different sequences to elucidate their relative importance as osteogenesis progresses. The murine myoblastic C2C12 cell line (of mesenchymal origin), which can differentiate into muscle, adipocyte, or osteoblastic lineages , was used. These cells have recently been shown to be sensitive to the sequence and timing of BMP-2 exposure during osteogenesis , making them an ideal candidate for testing interactions with mechanical stimulation as well.
2. Materials and Methods
2.1. Cell Culture
The cell line C2C12 (ATCC CRL-1772; American Type Culture Collection, Manassas, VA) was maintained on 10 cm diameter petri dishes in growth medium consisting of Dulbecco’s modified Eagle medium (DMEM; Invitrogen, Burlington, ON) supplemented with 10% fetal bovine serum (FBS; Invitrogen) and 1% Penicillin-Streptomycin (Invitrogen) at 37°C in a humidified atmosphere of 5% CO2 in air. Cells between passages 5 to 10 were used in all experiments. Cells were seeded on modified (as will be shown) high extension silicone rubber (HESR) culture dishes and maintained overnight for an attachment period. Seeding was performed using cells on HESR dishes expanded to 20 cm2. After the 24-hour attachment period, cells were typically 60–80% confluent and experiments were initiated.
2.2. Preparation of Silicone Rubber Culture Surfaces
High extension silicone rubber culture dishes (Cytomec GmbH, Spiez, Switzerland) were modified to promote cell adhesion as previously described . Briefly, unstretched HESR dishes were coated with 30% sulphuric acid for 15 min and then washed thoroughly with deionized water. Then surfaces were silanized with 1% (3-aminopropyl) triethoxysilane for 2 hours at 70°C and washed thoroughly again. Surfaces were then functionalized with 5% (wt/vol) glutaraldehyed for another 15 min and washed. Next, surfaces were disinfected by rinsing with 70% ethanol, washed with phosphate buffered saline (PBS), mounted in a mechanical device (as will be shown), expanded to 20 cm2 culture surface area, and coated with protein by incubation with 50 μg/mL collagen type I in PBS overnight. On the next day, HESR surfaces were washed again with PBS prior to cell seeding.
2.3. Mechanical Stimulation
Mechanical stimulation was applied using an iris-like device (Cytomec) within which HESR culture dishes were mounted [16, 20] (Figures 1(a)–1(d)). Approximately uniform expansion and contraction of the culture surface was applied by opening or closing the iris-like device. During mechanical stimulation, a continuous culture surface stretching and contraction was applied. Oscillatory stimulation occurred about a mean surface area of 20 cm2 with amplitude of 10% (±2 cm2) at a frequency of 0.01 Hz. Unstimulated control cultures were maintained on HESR culture dishes mounted in the iris-like device and held to a fixed surface area of 20 cm2.
2.4. Experimental Protocols
As an initial control, the osteogenic potential of C2C12 cells was tested under nonmechanically stimulated conditions during culture on tissue culture plastic in osteogenic medium (growth medium supplemented with 200 ng/mL BMP-2 (Invitrogen, Burlington, ON)). 200 000 cells were seeded per well in a 6-well plate. After a 24-hour attachment period, cells were harvested from one well as a time zero control. Other wells were then induced with osteogenic medium for 6, 24, and 48 hours after which cells were collected for gene expression and histological analyses (as will be shown).
Four different experimental protocols (A, B, C, and D) were designed to investigate the combined effects of BMP-2 induction and mechanical stimulation. In experiment A, cells were induced with BMP-2 for 48 hours while mechanical stimulation was only applied for the latter 24 hours. These were compared to controls under BMP-2 induction for 48 hours in the absence of any mechanical stimulation (Figure 3(a)). In experiment B, BMP-2 induction and mechanical stimulation were applied simultaneously for 48 hours and compared to controls where BMP-2 induction occurred in the absence of any mechanical stimulation (Figure 4(a)). Protocols A and B were designed to investigate how mechanical stimulation could modulate the time course of BMP-2 induction. In experiment C, cells were primed with BMP-2 for 24 hours after which medium was replaced with fresh growth medium and mechanical stimulation was applied for the next 24 hours. These were compared to controls primed with BMP-2 for 24 hours after which medium was replaced with growth medium but no mechanical stimulation was applied (Figure 5(a)). Experiment D was similar to experiment C except that the control culture involved BMP-2 induction for 48 hours without any mechanical stimulation (Figure 6(a)). Protocols C and D addressed the question of whether mechanical stimulation could replace BMP-2 induction.
2.5. Reverse Transcription and Quantitative Real-Time PCR
Total RNA was isolated using TRIzol Reagent (Invitrogen) following the manufacturer’s protocol. Reverse transcription was performed using 500 ng of total RNA in 20 μL volume per reaction using the qScript cDNA synthesis kit following the manufacturer’s instructions (Quanta Biosciences, Gaithersburg, MD). cDNA was diluted 1 : 10 and 1 μL of each cDNA sample was loaded per reaction (in duplicate) using PerfeCTa SYBR Green FastMix (Quanta Biosciences). Standard quantitative real-time PCR protocols were performed using HPRT for normalization as previously described . PCR primers for the transcription factors Runx2 and osterix (Osx) and for alkaline phosphatase (Alpl), Osteopontin, collagen type I (Col1a1), bone Gla protein, iso-bone sialoprotein (Ibsp), osteoprotegerin (OPG), and HPRT  were generated exactly as described elsewhere .
2.6. Western Blotting
C2C12 cells were lysed in lysis buffer (20 mM Tris (pH 7.4), 150 mM NaCl, 1 mM EDTA, 0.5% Triton X-100, and 1 mM β-glycerophosphate supplemented with complete EDTA-free protease inhibitor cocktail). 10 μg of total protein was run on a 10% SDS-PAGE gel and transferred to nitrocellulose membranes. Membranes were blocked in 5% BSA for 2 hours. For ERK1/2 analysis, blots were probed with antibodies against p42/p44 (1 : 2000, Cell Signalling), phospho-p42/p44 (1 : 1000, Cell Signalling), phospho-p38 (1 : 1000, Cell Signalling), and phospho-JNK (1 : 1000, Cell Signalling) followed by anti-rabbit horseradish peroxidase-conjugated secondary antibody (1 : 10000, Cell Signalling). For Wnt signaling, blots were probed with antibodies against β-catenin (1 : 1000, Abcam) and -tubulin (1 : 1000, Abcam, Cambridge, MA), followed by incubation with anti-mouse horseradish peroxidase-conjugated secondary antibody (1 : 5000, Cell Signalling). Washed membranes were developed using Super Signal West Pico Substrate (Thermo Scientific, Rockford, IL) and BioMax MR film (Eastman Kodak).
C2C12 cells were washed with deionized water and fixed with 4% paraformaldehyde (Alfa Aesar, Ward Hill, MA) for 2 min. Formaldehyde was then removed by washing with PBS and ALP assay was immediately performed according to the manufacturer’s instructions (Alkaline Phosphatase Detection Kit, Millipore). Images were captured using a Zeiss Axiovert 40C microscope equipped with a Canon Powershot A640 digital camera attached to a Zeiss MC80DX 1.0x tube adapter.
2.8. Statistical Analysis
All experiments were performed at least three times. Statistical significance of differences between mechanically stimulated cultures and unstimulated controls was evaluated using two-tailed unequal variance -tests ().
3.1. Osteogenic Differentiation of C2C12 Cells in the Presence of BMP-2 Is Time Sensitive
C2C12 cells cultured in osteogenic medium for 6, 24, and 48 hours specifically began differentiating towards an osteoblast-like phenotype. qPCR analysis indicated significant changes in Runx2, Osx, Alp, Col1a1, Osteopontin, and bone Gla protein after 48 hours of induction with BMP-2 (Figure 2). While most genes were downregulated compared to time zero controls after 6 hours, there were trends for increases in all of them with time. Strong alkaline phosphatase activity was clearly visible (purple stain) after 48 hours in BMP-2-treated samples versus untreated C2C12 cells (Figure 2 inset).
3.2. Low-Frequency Stimulation Enhances Osteogenesis in C2C12 Cells after BMP-2 Priming
Experiment A included 24 hours of priming with BMP-2 followed by 24 hours of superimposed mechanical stimulation (Figure 3(a)). This protocol had no obvious effect on gross morphology (Figure 3(b)). As indicated by qPCR (Figure 3(c)), low-frequency mechanical stimulation significantly upregulated expression of Runx2, Osx, Alp and Col1a1 with respect to BMP-2-induced controls at 48 hours. Upregulation of osteopontin also approached significance (). Mechanical stimulation caused trends for upregulation of bone Gla protein and OPG versus controls but these were not statistically significant (Figure 3(c)).
3.3. Low-Frequency Stimulation without BMP-2 Priming Does Not Enhance Osteogenesis
In experiment B, BMP-2 induction and low-frequency mechanical stimulation were applied simultaneously for 48 hours (Figure 4(a)). qPCR analysis demonstrated no significant changes in osteogenic gene expression compared to nonmechanically stimulated controls at 48 hours (Figure 4(b)), although Runx2 appeared slightly upregulated (). No changes in cell morphology were observed (not shown).
3.4. Low-Frequency Stimulation Is Sufficient to Modulate Osteogenesis after BMP-2 Priming
In experiment C, cells were primed for 24 hours with BMP-2, after which low-frequency mechanical stimulation was applied for 24 hours in the absence of BMP-2 and compared to controls without BMP-2 (Figure 5(a)). qPCR results indicated significant upregulation of Col1a1 and strong trends for upregulation of Osx and Alp which approached significance ( and 0.08) versus nonmechanically stimulated controls (Figure 5(b)). In contrast, osteopontin was significantly downregulated versus controls.
3.5. BMP-2-Induced Osteogenesis Masks the Effects of Low-Frequency Mechanical Stimulation
In experiment D, mechanically stimulated cells from experiment C were compared to controls in which BMP-2 was present for 48 hours (Figure 6(a)). Less osteogenic differentiation was observed in cells exposed to low-frequency mechanical stimulation versus those induced with BMP-2 alone for 48 hours (Figure 6(b)). These effects were particularly significant for Runx2, Osx and Alp.
3.6. Low-Frequency Mechanical Stimulation Alters MAPK and Wnt Signaling in C2C12 Cells
In experiment A, Western blot analysis of protein lysates at 48 hours showed that priming with BMP-2 followed by superposition of low-frequency mechanical stimulation downregulated ERK and p38 activity (Figure 7). In experiment B, Western blot analysis revealed that concomitant application of low-frequency mechanical stimulation and BMP-2 without priming caused an increase in ERK activity. For experiment C, no changes were observed in MAPK activity between cells primed with BMP-2 and then mechanically stimulated without BMP-2 versus nonmechanically stimulated controls which were primed and then cultured without BMP-2. In experiment D, when mechanical stimulation after priming was compared to 48 hours of BMP-2-induced controls, an increase in ERK activity was observed with no detectable change in p38 activity (not shown). JNK activity was below detection for all experiments (not shown). When analyzing Wnt signalling, no detectable changes in β-catenin were observed under most experimental conditions, with the exception of a slight increase in experiment D (Figure 7).
Previous studies have shown that BMP-2 induces osteogenesis through upregulation of the key transcription factors Runx2  and Osx (Osterix) [23, 24]. The present results confirm these findings and moreover demonstrate that low-frequency mechanical stimulation can enhance osteogenic differentiation of C2C12 cells in the presence of BMP-2. BMP-2 alone induces expression of bone marker genes such as alkaline phosphatase (Alp), Osteopontin, and collagen type I , and we have clearly shown here that concomitant low-frequency mechanical stimulation has a synergistic effect on C2C12 osteogenic differentiation depending on the timing of these costimuli. These findings are consistent with those of previous studies involving significantly different mechanical conditions, notably higher oscillatory stimulation frequencies [26–28]. These previous studies employed frequencies between 0.1 and 1 Hz to show that mechanical stimulation can inhibit or induce stem cell differentiation to desired lineages [29–33]. The present results show that this upregulation in bone marker genes can also occur at frequencies as low as 0.01 Hz, which are much lower than fundamental frequencies of locomotion. This indicates that enhancement in osteogenic differentiation of C2C12 cells by oscillatory mechanical stimulation can occur for a wider range of frequencies than previously believed, similar to previous findings for inhibition of adipogenic differentiation .
It is known that BMP-2 can induce osteogenic differentiation of stem cells [34–36]. Moreover, exposure to BMP-2 is necessary for initiation of osteogenic differentiation of C2C12 cells . Our pilot studies established that low-frequency mechanical stimulation in the absence of BMP-2 exposure did not significantly drive osteogenic differentiation of C2C12 cells by itself (data not shown). Therefore all experiments performed in the present study involved a 24–48-hour exposure to BMP-2 as a “priming” step to provide an environment within which mechanical effects on osteogenesis could be investigated. Interestingly, when mechanical stimulation was started at the same time as BMP-2 induction such that no priming period with BMP-2 alone occurred, no significant changes in osteogenic gene expression were observed (Figure 4). In contrast, synergistic effects on osteogenesis were observed when concomitant BMP-2 and mechanical stimuli were applied following priming by BMP-2 alone (Figure 3). Specifically, the early osteogenic markers Runx2, Osx, and Alp  and the late osteogenic marker Col1a1  were significantly upregulated versus nonmechanically stimulated controls. However, no significant changes in the other osteogenic markers Gla, Ibsp, or OPG were observed. Evidently, osteogenic effects of low-frequency mechanical stimulation on C2C12 cells can be critically dependent upon previous exposure to growth factor stimulation, and the timing and sequence of superimposed BMP-2 and mechanical stimuli can sensitively influence osteogenesis.
After initiation of osteogenesis with BMP-2 priming, our latter experiments tested if mechanical stimulation in the absence of BMP-2 could further modulate osteogenesis or match the efficacy of continued BMP-2 exposure. Following 24 hours of BMP-2 priming, low-frequency mechanical stimulation significantly upregulated expression of Osx, Alp, and Col1a1 versus controls where BMP-2 exposure stopped after priming (Figure 5). Conversely, osteopontin was slightly downregulated, but overall the effects of mechanical stimulation alone following BMP-2 priming indicated enhancement of osteogenesis. However, low-frequency mechanical stimulation after priming in the absence of BMP-2 could not match the efficacy of continued BMP-2 exposure in non-mechanically stimulated controls (Figure 6). Specifically, significantly diminished expression of Runx2, Osx, and Alp was observed in mechanically stimulated cells in competition with BMP-2-stimulated controls, though Col1a1 and osteopontin were expressed at similar levels in both conditions. Therefore, it appears that low-frequency mechanical stimulation can enhance osteogenesis of C2C12 cells when BMP-2 concentration decreases; however, this enhancement is not as potent as continued high concentrations of BMP-2 [19, 26].
Recent studies utilizing high-frequency mechanical stimulation have indicated a role for mitogen-activated protein (MAP) kinase signaling in stem cell differentiation . Other in vitro studies also implied that β-catenin is required downstream of BMP-2 for osteoblast mineralization . The extracellular-related kinase (ERK) and p38 kinase pathways are strong candidates for this activity since previous work has shown that mechanical stimulation induces a rapid and transient change in both kinase activities in C2C12 and osteoblast-like cells [41–43]. Also, the Wnt signalling pathway is involved in the response of bone-like cells to mechanical loading  and is also active during osteogenic differentiation of C2C12 cells [45–47]. Consistent with these findings, our Western blot data suggest that low-frequency mechanical stimulation following BMP-2 priming may act primarily through ERK and β-catenin (Wnt) signalling. However, we were unable to detect differences in p38 and JNK activities under our experimental conditions. Further studies are required to elucidate the differences between modes of mechanical stimulation in terms of the specific intercellular signaling pathways activated during osteogenic differentiation.
Perhaps the most obvious context within which varying growth factor concentrations and low-frequency mechanical stimulation act in concert on stem cells is during development [48, 49]. It is perhaps unwarranted to extrapolate the findings of this in vitro study to more complex processes; however the present results suggest a model for interpretation of how these stimuli can contribute in a coordinated fashion during development. For example, during limb bud development, transient growth factor concentration gradients initiate stem cell differentiation and establish basic morphology , while subsequent low-frequency movement and growth may refine these patterns by modulating cytokine, growth factor, and ECM protein production, thus ultimately promoting terminal differentiation and structure . These insights may enable future application of present findings for improved control of stem cell differentiation in cell-based therapies.
Conflict of Interests
One of the authors (T. M. Quinn) is a shareholder in the company Cytomec GmbH, which makes the iris-like devices for cell culture on high extension surfaces used in this study. There is no further conflict of interests.
This paper was supported by the Canada Research Chairs and NSERC Discovery Grants Program.
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