Laboratory for Bone and Implant Sciences (LBIS), The Jane and Jerry Weintraub Center for Reconstructive Biotechnology, Division of Advanced Prosthodontics, Biomaterials and Hospital Dentistry, UCLA School of Dentistry, 10833 Le Conte Avenue, Los Angeles, CA 90095-1668, USA.
Biomaterials. 2010 Mar;31(7):1546-57. doi: 10.1016/j.biomaterials.2009.11.018. Epub 2009 Dec 5.
In this study, we tested the potential of UV-photofunctionalized titanium surfaces to overcome compromised bone-titanium integration in a gap healing model. Titanium in rod and disk forms was acid etched and then stored for 4 weeks under dark ambient conditions. Titanium rods with and without UV pretreatment were placed into a rat femur with (contact healing) or without (gap healing) contact with the innate cortical bone. The titanium implants were subjected to a biomechanical push-in test, micro-CT bone morphometry, and surface elemental analysis after 2 weeks of healing. The strength of bone-titanium integration in the gap healing model was one-third of that in the contact healing model. However, UV-treated implants in the gap healing condition produced a strength of bone-titanium integration equivalent to that of untreated implants in the contact healing condition. Bone volume around UV-treated implants was 2- to 3-fold greater than that around the untreated implants in the gap healing model. A bone generation profile drawn along the long axis of the implant exhibited greater contrast between the untreated and UV-treated surfaces in the cortical area than in the bone marrow area. The bone tissue formed on UV-treated implants showed a higher Ca/P ratio than that formed on untreated titanium. The rate of cell proliferation, alkaline phosphatase activity, and calcium deposition in femoral periosteal cells and in bone marrow-derived osteoblasts were greater in cultures on UV-treated titanium disks than in cultures on untreated disks. The UV-enhanced function in periosteal cells was more pronounced when they were co-cultured with bone marrow-derived osteoblasts, indicating a synergistic effect of UV-treated titanium with biological signals from bone marrow-derived osteoblasts. Within the limitation of the model used in this study, UV-photofunctionalized titanium surfaces may overcome the challenging condition of bone-titanium integration without cortical bone support. UV treatment of implants induced marked improvements in the behavior of bone formation and quantity and quality of bone tissue around the implants. These effects may be related to the promoted function of both periosteum- and bone marrow-derived osteogenic cells at the local level around UV-treated titanium surfaces.
在这项研究中,我们测试了经紫外线光功能化的钛表面在间隙愈合模型中克服受损的骨-钛整合的潜力。棒状和盘状钛经过酸蚀处理,然后在黑暗的环境条件下储存 4 周。带有和不带有紫外线预处理的钛棒被放置在大鼠股骨中,与固有皮质骨接触(接触愈合)或不接触(间隙愈合)。在愈合 2 周后,钛植入物接受生物力学推压试验、微 CT 骨形态计量学和表面元素分析。在间隙愈合模型中,骨-钛整合的强度是接触愈合模型的三分之一。然而,在间隙愈合条件下经紫外线处理的植入物产生的骨-钛整合强度与接触愈合条件下未经处理的植入物相当。在间隙愈合模型中,骨体积围绕紫外线处理的植入物比未处理的植入物大 2-3 倍。沿着植入物长轴绘制的骨生成轮廓显示,在皮质区域,未经处理和紫外线处理表面之间的对比度大于骨髓区域。在紫外线处理的植入物上形成的骨组织的 Ca/P 比值高于未经处理的钛上形成的 Ca/P 比值。股骨骨膜细胞和骨髓源性成骨细胞在紫外线处理的钛盘上的细胞增殖率、碱性磷酸酶活性和钙沉积率高于在未经处理的钛盘上的培养。当与骨髓源性成骨细胞共培养时,骨膜细胞的 UV 增强功能更为明显,表明紫外线处理的钛与骨髓源性成骨细胞的生物信号具有协同作用。在本研究中使用的模型的限制范围内,经紫外线光功能化的钛表面可能在没有皮质骨支持的情况下克服骨-钛整合的挑战性条件。植入物的紫外线处理显著改善了植入物周围骨形成的行为以及骨组织的数量和质量。这些影响可能与局部周围紫外线处理的钛表面处骨膜和骨髓源性成骨细胞的功能促进有关。
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