Inhibition of Rac and ROCK Signalling Influence Osteoblast Adhesion, Differentiation and Mineralization on Titanium Topographies

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Abstract

Reducing the time required for initial integration of bone-contacting implants with host tissues would be of great clinical significance. Changes in osteoblast adhesion formation and reorganization of the F-actin cytoskeleton in response to altered topography are known to be upstream of osteoblast differentiation, and these processes are regulated by the Rho GTPases. Rac and RhoA (through Rho Kinase (ROCK)). Using pharmacological inhibitors, we tested how inhibition of Rac and ROCK influenced osteoblast adhesion, differentiation and mineralization on PT (Pre-treated) and SLA (sandblasted large grit, acid etched) topographies. Inhibition of ROCK, but not Rac, significantly reduced adhesion number and size on PT, with adhesion size consistent with focal complexes. After 1 day, ROCK, but not Rac inhibition increased osteocalcin mRNA levels on SLA and PT, with levels further increasing at 7 days post seeding. ROCK inhibition also significantly increased bone sialoprotein expression at 7 days, but not BMP-2 levels. Rac inhibition significantly reduced BMP-2 mRNA levels. ROCK inhibition increased nuclear translocation of Runx2 independent of surface roughness. Mineralization of osteoblast cultures was greater on SLA than on PT, but was increased by ROCK inhibition and attenuated by Rac inhibition on both topographies. In conclusion, inhibition of ROCK signalling significantly increases osteoblast differentiation and biomineralization in a topographic dependent manner, and its pharmacological inhibition could represent a new therapeutic to speed bone formation around implanted metals and in regenerative medicine applications. © 2013 Prowse et al.

Figures

  • Figure 1. Characterization of the surfaces used in the study. (a) SEM micrographs of pre-treated (PT) and SLA surfaces. In (b) surface roughness parameters of the three-dimensional surface topography of PT and SLA quantitatively measured using confocal microscopy. For detailed description, see materials and methods. (c) AFM micrographs of the PT surface. doi:10.1371/journal.pone.0058898.g001
  • Figure 2. Influence of NCS23766 and Y27632 on the activity of Rac1 and ROCK on tissue culture plastic. Studies were run for 1 week and 3 days to quantify the temporal suppression of the inhibitors. NCS23766 significantly reduced Rac1 activity and Y27632 inhibited the activity of ROCK. Alizarin red staining of wells demonstrated increased mineralization in the presence of ROCK inhibitors. Treatments were analyzed via one-way ANOVA with a Bonferroni post-test (* denotes significance of p,0.05 between treatments). doi:10.1371/journal.pone.0058898.g002
  • Figure 3. Immunofluorescent detection of adhesions and F-actin organization in osteoblasts cultured on PT and SLA surfaces with and without Rac and ROCK inhibition at 24 h. Osteoblasts form stressfibres on PT, but not SLA. ROCK inhibition disrupts stressfibre formation in osteoblasts on both PT surfaces. Cells were stained for vinculin (green), F-actin (red), and nuclei (blue). doi:10.1371/journal.pone.0058898.g003
  • Figure 4. Influence of topography, Rac and ROCK inhibition on (a) adhesion number and (b) adhesion size. Graphs represent mean 6 SEM of 3 independent experiments completed in triplicate. Treatments were analyzed via two-way ANOVA with a Bonferroni posttest (# denotes significance of p,0.05 between PT and SLA, * denotes significance of p,0.05 between treatments within a surface type). doi:10.1371/journal.pone.0058898.g004
  • Figure 5. Influence of topography, Rac1 and ROCK inhibition on expression of (a) BMP-2, (b) osteocalcin and (c) bone sialoprotein in osteoblasts at 24 h post seeding. ALP mRNA levels were significantly increased on PT by both inhibitors, but only ROCK had an effect on SLA. No significant differences were observed in BMP-2 or BSP levels under any treatment, but ROCK inhibition significantly increased osteocalcin levels on both PT and SLA. Graphs represent mean 6 SEM of 3 independent experiments completed with 4 replicates per experiment. Treatments were analyzed via two-way ANOVA with a Bonferroni post-test (# denotes significance of p,0.05 between PT and SLA, * denotes significance of p,0.05 between treatments within a surface type). doi:10.1371/journal.pone.0058898.g005
  • Figure 6. Influence of topography, Rac1 and ROCK inhibition on expression of (a) BMP-2, (b) osteocalcin and (c) bone sialoprotein in osteoblasts at 7 days post seeding. ROCK inhibition significantly increased osteocalcin and BSP mRNA levels on both PT and SLA compared to control surfaces. Graphs represent mean 6 SEM of 3 independent experiments completed with 4 replicates per experiment. Treatments were analyzed via two-way ANOVA with a Bonferroni post-test (# denotes significance of p,0.05 between PT and SLA, * denotes significance of p,0.05 between treatments within a surface type). doi:10.1371/journal.pone.0058898.g006
  • Figure 7. Rac1 and ROCK inhibition influence localization of the osteogenic transcription factor, Runx2. (a) At 1 week, cells were labeled with specific antibodies to Runx2, and (b) quantification of nuclear translocation. Rac1-inhibition reduced nuclear localization of Runx2 on both PT and SLA compared to controls although it was still found in the cytoplasm. ROCK inhibition increased nuclear localization of Runx2 on both PT and SLA compared to controls and it was also found in the cytoplasm. Treatments were analyzed via two-way ANOVA with a Bonferroni post-test (# denotes significance of p,0.05 between PT and SLA, * denotes significance of p,0.05 between treatments within a surface type). doi:10.1371/journal.pone.0058898.g007
  • Figure 8. Topography, Rac1 and ROCK inhibition synergistically affect osteoblast biomineralization. (a) Quantification of the intensity of tetracycline labelling and (b) number of nodules demonstrated that ROCK inhibition significantly increased mineral deposition by osteoblasts on both PT and SLA. Images are representative of triplicates from three experiments. Treatments were analyzed via two-way ANOVA with a Bonferroni post-test (# denotes significance of p,0.05 between PT and SLA, *denotes significance of p,0.05 between treatments within a surface type). doi:10.1371/journal.pone.0058898.g008

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Prowse, P. D. H., Elliott, C. G., Hutter, J., & Hamilton, D. W. (2013). Inhibition of Rac and ROCK Signalling Influence Osteoblast Adhesion, Differentiation and Mineralization on Titanium Topographies. PLoS ONE, 8(3). https://doi.org/10.1371/journal.pone.0058898

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