The bioactive glass 45S5 was crystallized to 8-100 vol % of crystals by thermal treatments from 550-680Β°C. The microstructure of the glass-ceramics had a very uniform crystal size, ranging from 8 to 20 pm. Fourier-transform infrared (!?TIR) spectroscopy was used to determine the rate of hydroxycarbo
Effect of bioactive glass crystallization on the conformation and bioactivity of adsorbed proteins
β Scribed by Laura A. Buchanan; Ahmed El-Ghannam
- Publisher
- John Wiley and Sons
- Year
- 2009
- Tongue
- English
- Weight
- 917 KB
- Volume
- 9999A
- Category
- Article
- ISSN
- 1549-3296
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β¦ Synopsis
Abstract
Protein adsorption onto the surface of a biomaterial mediates cell adhesion and enhances tissueβimplant integration. In a previous study, we demonstrated that crystallization of bioactive glass (BG) significantly increased the negative zeta potential and decreased serum protein adsorption onto the material surface. In this study, the conformation of protein adsorbed onto the surface of amorphous bioactive glass (ABG) and crystallized bioactive glass (CBG) was analyzed and correlated to bone marrow mesenchymal stem cell adhesion and spreading. ABG and CBG were immersed in three different protein solutions containing 10% fetal bovine serum, bovine serum albumin (BSA), and fibronectin (FN) for 4 h at 37Β°C. Grazing angle Fourier transform infrared spectroscopy (GAβFTIR) demonstrated that the ratio of (amide I)/(amide II) functional groups of all proteins adsorbed onto ABG was greater than that for proteins adsorbed onto CBG. The Gaussian curve fitting analysis suggests that the significant expression of amide I, rich in charged and flexible unordered secondary structure of adsorbed FN, stimulated bone cell adhesion and spreading on the surface of ABG. CBG enforces protein conformation that exposes amide II, rich in neutral and stable Ξ²βsheet structure and Ξ±βhelix, which limited cell adhesion and spreading. Although ABG adsorbed significantly higher quantity of BSA than FN, GAβFTIR analyses showed that the ratio of amide I/amide II was significantly higher for adsorbed FN. Therefore, the intensity of amide I or amide II bands cannot be taken as a measure of the quantity of adsorbed protein. Β© 2009 Wiley Periodicals, Inc. J Biomed Mater Res, 2010
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