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KMID : 1023820150070060496
The Journal of Advanced Prosthodontics
2015 Volume.7 No. 6 p.496 ~ p.505
Effect of microgrooves and fibronectin conjugation on the osteoblast marker gene expression and differentiation
Park Su-Jung

Lee Sung-Bok
Ahn Su-Jin
Im Byung-Jin
Lee Do-Yun
Jee Yu-Jin
Yoon Joon-Ho
Taixing Cui
Lee Sang-Cheon
Lee Suk-Won
Abstract
PURPOSE : To determine the effect of fibronectin (FN)-conjugated, microgrooved titanium (Ti) on osteoblast differentiation and gene expression in human bone marrow-derived mesenchymal stem cells (MSCs).

MATERIALS AND METHODS : Photolithography was used to fabricate the microgrooved Ti, and amine functionalization (silanization) was used to immobilize fibronectin on the titanium surfaces. Osteoblast differentiation and osteoblast marker gene expression were analyzed by means of alkaline phosphatase activity assay, extracellular calcium deposition assay, and quantitative real-time PCR.

RESULTS : The conjugation of fibronectin on Ti significantly increased osteoblast differentiation in MSCs compared with non-conjugated Ti substrates. On the extracellular calcium deposition assays of MSCs at 21 days, an approximately two-fold increase in calcium concentration was observed on the etched 60-¥ìm-wide/10-¥ìm-deep microgrooved surface with fibronectin (E60/10FN) compared with the same surface without fibronectin (E60/10), and a more than four-fold increase in calcium concentration was observed on E60/10FN compared with the non-etched control (NE0) and etched control (E0) surfaces. Through a series of analyses to determine the expression of osteoblast marker genes, a significant increase in all the marker genes except type I collagen ¥á1 mRNA was seen with E60/10FN more than with any of the other groups, as compared with NE0.

CONCLUSION : The FN-conjugated, microgrooved Ti substrate can provide an effective surface to promote osteoblast differentiation and osteoblast marker gene expression in MSCs.
KEYWORD
The FN-conjugated, microgrooved Ti substrate can provide an effective surface to promote osteoblast differentiation and osteoblast marker gene expression in MSCs.
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