Submicron Scale-Structured Hydrophilic Titanium Surfaces Promote Early Osteogenic Gene Response for Cell Adhesion and Cell Differentiation

被引:87
|
作者
Klein, Marcus Oliver [1 ]
Bijelic, Ana [1 ]
Ziebart, Thomas [1 ]
Koch, Felix [1 ]
Kaemmerer, Peer W. [1 ]
Wieland, Marco [2 ]
Konerding, Moritz A. [3 ]
Al-Nawas, Bilal [1 ]
机构
[1] Univ Med Mainz, D-55131 Mainz, Germany
[2] MyoPowers Med Technol SA, Management, Lausanne, Switzerland
[3] Johannes Gutenberg Univ Mainz, Dept Anat, Mainz, Germany
关键词
cell adhesion; cell differentiation; integrins; osteocalcin; osteogenic cell proliferation; runx-2; surface hydrophilicity; titanium surface modifications; OSTEOBLAST DIFFERENTIATION; ALKALINE-PHOSPHATASE; BONE; EXPRESSION; IMPLANTS; MATRIX; PROLIFERATION; ROUGHNESS; PROTEINS; THERAPY;
D O I
10.1111/j.1708-8208.2011.00339.x
中图分类号
R78 [口腔科学];
学科分类号
1003 ;
摘要
Background and Purpose: Titanium (Ti) surface roughness and surface hydrophilicity are key factors to regulate osteogenic cell responses during dental implant healing. In detail, specific integrin-mediated interactions with the extracellular environment trigger relevant osteogenic cell responses like differentiation and matrix synthesis via transcriptions factors. Aim of this study was to monitor surface-dependent osteogenic cell adhesion dynamics, proliferation, and specific osteogenic cell differentiation over a period of 7 days. Materials and Methods: Ti disks were manufactured to present smooth pretreatment (PT) surfaces and rough sandblasted/acid-etched (SLA) surfaces. Further processing to isolate the uncontaminated TiO2 surface from contact with atmosphere provided a highly hydrophilic surface without alteration of the surface topography (modSLA). Tissue culture polystyrene (TCPS) served as control. Human osteogenic cells were cultivated on the respective substrates. After 24 hours, 48 hours, 72 hours, and 7 days, cell morphology on the Ti substrates was visualized by scanning transmission electron microscopy. As a marker of cellular proliferation, cell count was assessed. For the analysis of cell adhesion and differentiation, specific gene expression levels of the integrin subunits 1 and v, runx-2, collagen type I (COL), alkaline phosphatase (AP), and osteocalcin (OC) were obtained by real-time RT-PCR for the respective time points. Data were normalized to internal controls. Results: TCPS and PT surfaces preserved a rather immature, dividing osteogenic phenotype (high proliferation rates, low integrin levels, and low specific osteogenic cell differentiation). SLA and especially modSLA surfaces promoted both cell adhesion as well as the maturation of osteogenic precursors into post-mitotic osteoblasts. In detail, during the first 48 hours, modSLA resulted in lowest cell proliferation rates but exhibited highest levels of the investigated integrins, runx-2, COL, AP, and OC. Conclusion: Our results revealed a strong synergistic effect between submicron-scale roughness and surface hydrophilicity on early osteogenic cell adhesion and maturation.
引用
收藏
页码:166 / 175
页数:10
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