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口腔角质细胞对镍基牙科铸造合金的体外反应。

Oral keratinocyte responses to nickel-based dental casting alloys in vitro.

机构信息

School of Metallurgy and Materials, University of Birmingham, Edgbaston, Birmingham, B15 2TT, UK.

出版信息

J Biomater Appl. 2010 Sep;25(3):251-67. doi: 10.1177/0885328209349870. Epub 2009 Dec 11.

Abstract

Adverse reactions of oral mucosa to nickel-based dental casting alloys are probably due to corrosion metal ion release. We exposed H400 oral keratinocytes to two Ni-based dental alloys (Matchmate and Dsign10) as well as NiCl( 2) (1-40 microg/mL Ni(2+)). Alloy derived Ni(2+) media concentrations were determined. Direct culture on both alloys resulted in inhibited growth with a greater effect observed for Dsign10 (higher ion release). Indirect exposure of cells to conditioned media from Dsign10 negatively affected cell numbers (approximately 64% of control by 6 days) and morphology while Matchmate-derived media did not. Exposure to increasing NiCl(2) negatively affected cell growth and morphology, and the Granulocyte-macrophage colony-stimulating factor (GM-CSF) transcript was significantly up-regulated in cells following direct and indirect exposure to Dsign10. NiCl(2) exposure up-regulated all cytokine transcripts at 1 day. At day 6, IL-1beta and IL-8 transcripts were suppressed while GM-CSF and IL-11 increased with Ni(2+) dose. Accumulation of Ni(2+) ions from alloys in oral tissues may affect keratinocyte viability and chronic inflammation.

摘要

口腔黏膜对镍基牙科铸造合金的不良反应可能是由于腐蚀金属离子释放所致。我们将 H400 口腔角质细胞暴露于两种镍基牙科合金(Matchmate 和 Dsign10)以及 NiCl(2)(1-40μg/mL Ni(2+))中。测定了合金衍生的 Ni(2+)介质浓度。两种合金直接培养均导致细胞生长受到抑制,而 Dsign10 的抑制作用更为明显(离子释放量更高)。间接暴露于 Dsign10 条件培养基会对细胞数量产生负面影响(6 天内约为对照的 64%)并改变细胞形态,而 Matchmate 衍生的培养基则没有。随着 NiCl(2)浓度的增加,细胞生长和形态受到负面影响,并且在直接和间接暴露于 Dsign10 后,细胞中的粒细胞-巨噬细胞集落刺激因子(GM-CSF)转录本显著上调。NiCl(2)暴露在第 1 天会上调所有细胞因子的转录本。在第 6 天,IL-1beta 和 IL-8 转录本受到抑制,而 GM-CSF 和 IL-11 随着 Ni(2+)剂量的增加而增加。合金中镍离子在口腔组织中的积累可能会影响角质细胞的活力和慢性炎症。

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