9 research outputs found
Number of MG 63 cells on day 1, 3 and 7 (A, C, E), their spreading area (D) and their growth dynamics (B) on a standard polystyrene cell culture dish (PS), undoped NCD films (B_0) and NCD films doped with 133, 1000 and 6700 ppm of boron (B_133, B_1000 and B_6700, respectively).
<p>Mean ± S.E.M. from 3 experiments; each included 32 microphotographs (day 1 and 3) and 18 measurements in a hemocytometer (day 7) per experimental group). ANOVA, Student-Newman-Keuls method. Statistical significance: I, II, III, IV, V: <i>p</i>≤0.05 compared to the group labelled with the same Roman number.</p
Surface morphology of NCD samples without boron doping (A), with boron 133 ppm (B), 1000 ppm (C) and 6700 ppm (D).
<p>Field emission scanning electron microscope (e_Line, Raith). Scale bar is 200 nm.</p
Neutron depth profiling of boron over doped NCD samples.
<p>Neutron depth profiling of boron over doped NCD samples.</p
Raman spectra of undoped and boron-doped NCD samples.
<p>Raman spectra of undoped and boron-doped NCD samples.</p
The cell population doubling time of MG 63 cells between days 1 and 3 (DT<sub>1–3</sub>), days 3 and 7 (DT<sub>3–7</sub>) and days 1 and 7 (DT<sub>1–7</sub>) after seeding on polystyrene culture dishes (PS) and NCD films doped with 0, 133, 1000 or 6700 ppm of boron.
<p>Mean ± S.E.M. from 3 experiments (in total, 9 measurements for each experimental group and time interval). ANOVA, Student-Newman-Keuls Method. Statistical significance: <b><sup>I, II, V</sup></b>: <i>p</i>≤0.05 compared to polystyrene, undoped NCD and NCD doped with 6700 ppm of B, respectively.</p
Immunofluorescence staining of talin in MG 63 cells on day 3 after seeding on microscopic glass coverslips (A), undoped NCD (B), NCD films doped with boron in concentrations of 133 ppm (C) 1000 ppm (D) and 6700 ppm (E).
<p>The cell nuclei are counterstained with propidium iodide. Olympus IX 51 epifluorescence microscope, DP 70 digital camera, obj. 100×, bar = 10 µm.</p
Dependence of the surface parameters of the NCD samples on the boron doping level.
<p>*Values adjusted to the surface potential of gold.</p><p>For the NDP measurements, the accuracy can achieve 5% (which is the precision of the boron atoms in the etalon). However, the precision of the NDP technique also depends on other parameters, e.g. the stability of the neutron beam intensity, identical geometry of the etalon and the measured sample, etc. Realistically, the NDP data can be routinely measured with accuracy of 10% in our case.</p><p>For roughness, potential, phase and contact angle, the data is presented as Mean ± S.D. (Standard Deviation). In the case of roughness and AFM phase, each <i>rms</i> value was determined from 65 536 data points on each sample type. The mean and S.D. of <i>rms</i> values were calculated from 5 such measurements across the sample. In the case of surface potential, the mean and S.D. values were calculated from 65 536 measurements across each sample. The contact angle was calculated from fitting the curve of the water droplet, and the mean and S.D. values were calculated from 16 measurements for each sample type.</p><p>Statistical Analysis: ANOVA, Student-Newman-Keuls Method. Statistical significance: <sup>I, II, III, IV</sup>: <i>p</i>≤0.05 compared to the group labelled with the same Roman number.</p><p>For the room temperature electrical resistivity measurements, the accuracy is better than 1%.</p
Microscopic images of surface potential variations as detected by Kelvin force microscopy (left column), and surface topography as detected by atomic force microscopy (right column) on NCD samples without boron doping (A) and with nominal boron doping of 133 ppm (B), 1000 ppm (C), and 6700 ppm (D).
<p>The AFM oscillation amplitude was 100 nm, the setpoint was 50%. The KFM lift height was 30 nm. The detection frequency was 75 kHz.</p
Concentration of β<sub>1</sub>-integrin adhesion receptors, integrin-associated focal adhesion proteins talin and vinculin, markers of osteogenic cell differentiation osteocalcin, alkaline phosphatase, collagen I and osteopontin, and immunoglobuline adhesion molecule ICAM-1, a marker of cell immune activation, in MG 63 cells on day 7 after seeding on polystyrene culture dishes (PS) and NCD films doped with 0, 133, 1000 or 6700 ppm of boron.
<p>Measured by ELISA per mg of protein. The absorbances are given as a percentage of the control values obtained on PS. Mean ± S.E.M. from 3 experiments (each included 12–16 measurements for each experimental group). ANOVA, Student-Newman-Keuls Method. Statistical significance: <sup>I, II, III, IV</sup>: <i>p</i>≤0.05 compared to the group labelled with the same Roman number.</p