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The role of mechanotransduction versus hypoxia during simulated orthodontic compressive strain—an in vitro study of human periodontal ligament fibroblasts

机译:机械转导与缺氧在模拟正畸压缩应变中的作用-人牙周膜成纤维细胞的体外研究

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摘要

During orthodontic tooth movement (OTM) mechanical forces trigger pseudo-inflammatory, osteoclastogenic and remodelling processes in the periodontal ligament (PDL) that are mediated by PDL fibroblasts via the expression of various signalling molecules. Thus far, it is unknown whether these processes are mainly induced by mechanical cellular deformation (mechanotransduction) or by concomitant hypoxic conditions via the compression of periodontal blood vessels. Human primary PDL fibroblasts were randomly seeded in conventional six-well cell culture plates with O2-impermeable polystyrene membranes and in special plates with gas-permeable membranes (Lumox®, Sarstedt), enabling the experimental separation of mechanotransducive and hypoxic effects that occur concomitantly during OTM. To simulate physiological orthodontic compressive forces, PDL fibroblasts were stimulated mechanically at 2 g·cm−2 for 48 h after 24 h of pre-incubation. We quantified the cell viability by MTT assay, gene expression by quantitative real-time polymerase chain reaction (RT-qPCR) and protein expression by western blot/enzyme-linked immunosorbent assays (ELISA). In addition, PDL-fibroblast-mediated osteoclastogenesis (TRAP+ cells) was measured in a 72-h coculture with RAW264.7 cells. The expression of HIF-1α, COX-2, PGE2, VEGF, COL1A2, collagen and ALPL, and the RANKL/OPG ratios at the mRNA/protein levels during PDL-fibroblast-mediated osteoclastogenesis were significantly elevated by mechanical loading irrespective of the oxygen supply, whereas hypoxic conditions had no significant additional effects. The cellular–molecular mediation of OTM by PDL fibroblasts via the expression of various signalling molecules is expected to be predominantly controlled by the application of force (mechanotransduction), whereas hypoxic effects seem to play only a minor role. In the context of OTM, the hypoxic marker HIF-1α does not appear to be primarily stabilized by a reduced O2 supply but is rather stabilised mechanically.
机译:在正畸牙齿移动(OTM)期间,机械力会触发牙周膜(PDL)中的假炎症,破骨细胞和重塑过程,这些过程由PDL成纤维细胞通过各种信号分子的表达介导。迄今为止,尚不清楚这些过程是主要由机械细胞变形(机械转导)引起,还是由牙周血管压缩引起的低氧状态引起。将人类原发性PDL成纤维细胞随机接种在具有O2不可渗透的聚苯乙烯膜的常规六孔细胞培养板和具有透气膜的特殊板(Lumox®,Sarstedt)中,从而能够在实验过程中同时分离机械传导和低氧作用OTM。为了模拟生理学上的正畸压力,预培养24小时后,以2 g·cm -2 机械刺激PDL成纤维细胞48 h。我们通过MTT法定量细胞活力,通过定量实时聚合酶链反应(RT-qPCR)定量基因表达,并通过western blot /酶联免疫吸附法(ELISA)定量蛋白质表达。另外,在与RAW264.7细胞共培养72小时的过程中,测量了PDL-成纤维细胞介导的破骨细胞生成(TRAP + 细胞)。机械负荷下,无论氧气如何,在PDL成纤维细胞介导的破骨细胞形成过程中,HIF-1α,COX-2,PGE2,VEGF,COL1A2,胶原蛋白和ALPL的表达以及mRNA /蛋白水平上的RANKL / OPG比均显着升高供氧不足,而低氧条件没有明显的其他影响。预计PDL成纤维细胞通过各种信号分子的表达对OTM的细胞分子介导主要受力(机械转导)的控制,而低氧作用似乎只起很小的作用。在OTM的背景下,缺氧标记物HIF-1α似乎并未因减少的O2供给而基本稳定,而是通过机械方式稳定了。

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