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Porous titanium and Ti-35Nb alloy: effects on gene expression of osteoblastic cells derived from human alveolar bone

机译:多孔钛和Ti-35Nb合金:对源自人牙槽骨的成骨细胞基因表达的影响

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Tests on titanium alloys that possess low elastic modulus, corrosion resistance and minimal potential toxicity are ongoing. This study aimed to evaluate the behavior of human osteoblastic cells cultured on dense and porous Titanium (Ti) samples comparing to dense and porous Ti-35 Niobium (Ti-35Nb) samples, using gene expression analysis. Scanning electronic microscopy confirmed surface porosity and pore interconnectivity and X-ray diffraction showed titanium beta-phase stabilization in Ti-35Nb alloy. There were no differences in expression of transforming growth factor-beta, integrin-beta 1, alkaline phosphatase, osteopontin, macrophage colony stimulating factor, prostaglandin E synthase, and apolipoprotein E regarding the type of alloy, porosity and experimental period. The experimental period was a significant factor for the markers: bone sialoprotein II and interleukin 6, with expression increasing over time. Porosity diminished Runt-related transcription factor-2 (Runx-2) expression. Cells adhering to the Ti-35Nb alloy showed statistically similar expression to those adhering to commercially pure Ti grade II, for all the markers tested. In conclusion, the molecular mechanisms of interaction between human osteoblasts and the Ti-35Nb alloy follow the principal routes of osseointegration of commercially pure Ti grade II. Porosity impaired the route of transcription factor Runx-2.
机译:具有低弹性模量,耐腐蚀性和最小潜在毒性的钛合金的测试正在进行中。这项研究旨在通过基因表达分析来评估在致密和多孔的钛(Ti)样品上培养的人成骨细胞与致密和多孔的Ti-35铌(Ti-35Nb)样品相比的行为。扫描电子显微镜证实表面孔隙率和孔互连性,X射线衍射显示Ti-35Nb合金中的钛β相稳定。关于合金的类型,孔隙率和实验时间,转化生长因子-β,整联蛋白-β1,碱性磷酸酶,骨桥蛋白,巨噬细胞集落刺激因子,前列腺素E合酶和载脂蛋白E的表达没有差异。实验时期是标志物的重要因素:骨唾液蛋白II和白介素6,表达随时间增加。孔隙率降低了Runt相关转录因子2(Runx-2)的表达。对于所有测试的标志物,粘附在Ti-35Nb合金上的细胞在统计学上均与粘附在商业纯钛II级上的细胞相似。总之,人类成骨细胞与Ti-35Nb合金之间相互作用的分子机制遵循商业纯II级Ti骨整合的主要途径。孔隙度削弱了转录因子Runx-2的途径。

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