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Elongated Growth of Octacalcium Phosphate Crystals in Recombinant Amelogenin Gels under Controlled Ionic Flow
M. Iijima*,1,
Y. Moriwaki1,
H.B. Wen2,3,
A.G. Fincham2 and
J. Moradian-Oldak2
1 Asahi University School of Dentistry, Dental Materials and Technology, 1851-1 Hozumi, Hozumi-cho, Motosu-gun, Gifu 501-0296, Japan;
2 University of Southern California, School of Dentistry, Center for Craniofacial Molecular Biology, Los Angeles, CA, USA; anad
3 present address, DePuy, a Johnson & Johnson company, PO Box 988, 700 Orthopaedic Drive, Warsaw, IN 46581-0988, USA;

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Figure 1. Direct visualization of amelogenin nanospheres (10-20 nm in diameter) in 10% rM179 amelogenin gel by a Tapping mode AFM in air. The gel was formed in 10 mM phosphate buffer at pH 6.5, with conditions resembling those of OCP crystallization, and fixed at 37°C (see MATERIALS & METHODS).
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Figure 2. SEM images of crystals grown (a) without protein, in (b) 10% rM179, (c) 10%r M166, (d) 10% polyacrylamide gel, (e) 0.5% agarose gel, and (f) 10% albumin. Note that OCP crystals in a, d, e, and f show typical ribbon-like morphology, while the cylindrical and prismatic fibers grew only in amelogenin gels, regardless of the existence of the hydrophilic C-terminal of amelogenin.
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Figure 3. Effects of 10% gels of bovine amelogenins, rM166, rM179, polyacrylamide, and 10% albumin and gelatin on the morphology of OCP crystal, which are represented by (a) the length-to-width ratio (L/W) and (b) the width-to-thickness ratio (W/T) of crystals. Aspect ratios and their standard deviations (SD) were calculated based on the mean values and SD values of each dimension in the Table . Error bars represent SD values. (c) Schema ofOCP crystal, showing length, width, thickness, crystal faces, and crystallographic axes.
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Journal of Dental Research, Vol. 81, No. 1,
69-73 (2002)
DOI: 10.1177/154405910208100115

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