NP-12 peptide functionalized nanoparticles counteract the effect of bacterial lipopolysaccharide on cultured osteoblasts

IF 4.6 1区 医学 Q1 DENTISTRY, ORAL SURGERY & MEDICINE Dental Materials Pub Date : 2024-06-12 DOI:10.1016/j.dental.2024.06.017
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Abstract

Objective

To evaluate whether nanoparticles (NPs) functionalized with Tideglusib (TDg, NP-12), and deposited on titanium surfaces, would counteract the effect of bacterial lipopolysaccharide (LPS) on osteoblasts.

Methods

Experimental groups were: (a) Titanium discs (TiD), (b) TiD covered with undoped NPs (Un-NPs) and (c) TiD covered with TDg-doped NPs (TDg-NPs). Human primary osteoblasts were cultured onto these discs, in the presence or absence of bacterial LPS. Cell proliferation was assessed by MTT-assay and differentiation by measuring the alkaline phosphatase activity. Mineral nodule formation was assessed by the alizarin red test. Real-time quantitative polymerase chain reaction was used to study the expression of Runx-2, OSX, ALP, OSC, OPG, RANKL, Col-I, BMP-2, BMP-7, TGF-β1, VEGF, TGF-βR1, TGF-βR2, and TGF-βR3 genes. Osteoblasts morphology was studied by Scanning Electron Microscopy. One-way ANOVA or Kruskal-Wallis and Bonferroni multiple comparisons tests were carried out (p < 0.05).

Results

TDg-NPs enhanced osteoblasts proliferation. Similarly, this group increased ALP production and mineral nodules formation. TDg-NPs on titanium discs resulted in overexpression of the proliferative genes, OSC and OSX, regardless of LPS activity. In the absence of LPS, TDg-NPs up-regulated Runx2, COL-I, ALP, BMP2 and BMP7 genes. OPG/RANKL gene ratios were increased about 2500 and 4,000-fold by TDg-NPs, when LPS was added or not, respectively. In contact with the TDg-NPs osteoblasts demonstrated an elongated spindle-shaped morphology with extracellular matrix production.

Significance

TDg-NPs on titanium discs counteracted the detrimental effect of LPS by preventing the decrease on osteoblasts proliferation and mineralization, and produced an overexpression of proliferative and bone-promoting genes on human primary osteoblasts.

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NP-12肽功能化纳米粒子可抵消细菌脂多糖对培养成骨细胞的影响。
目的评估用 Tideglusib(TDg,NP-12)功能化的纳米颗粒(NPs)沉积在钛表面是否会抵消细菌脂多糖(LPS)对成骨细胞的影响:实验组为(实验组:(a) 钛盘(TiD);(b) 未掺杂 NPs 的钛盘(Un-NPs);(c) 掺杂 TDg 的 NPs 的钛盘(TDg-NPs)。在有或没有细菌 LPS 的情况下,将人类原代成骨细胞培养到这些圆片上。细胞增殖通过 MTT 分析法进行评估,分化通过测量碱性磷酸酶活性进行评估。矿物结节的形成通过茜素红试验进行评估。实时定量聚合酶链反应用于研究 Runx-2、OSX、ALP、OSC、OPG、RANKL、Col-I、BMP-2、BMP-7、TGF-β1、VEGF、TGF-βR1、TGF-βR2 和 TGF-βR3 基因的表达。用扫描电子显微镜研究成骨细胞的形态。进行单因素方差分析或 Kruskal-Wallis 和 Bonferroni 多重比较检验(p 结果:TDg-NPs 增强了成骨细胞的形态:TDg-NPs可促进成骨细胞增殖。同样,该组也增加了 ALP 的产生和矿物质结核的形成。无论 LPS 活性如何,钛盘上的 TDg-NPs 都会导致增殖基因 OSC 和 OSX 的过度表达。在没有 LPS 的情况下,TDg-NPs 会上调 Runx2、COL-I、ALP、BMP2 和 BMP7 基因。在添加或不添加 LPS 的情况下,TDg-NPs 使 OPG/RANKL 基因比率分别增加了约 2500 倍和 4000 倍。与 TDg-NPs 接触的成骨细胞表现出细长的纺锤形形态,并产生细胞外基质:钛盘上的 TDg-NPs 可防止成骨细胞增殖和矿化的减少,从而抵消 LPS 的不利影响,并使人类原发性成骨细胞的增殖基因和促骨基因过度表达。
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来源期刊
Dental Materials
Dental Materials 工程技术-材料科学:生物材料
CiteScore
9.80
自引率
10.00%
发文量
290
审稿时长
67 days
期刊介绍: Dental Materials publishes original research, review articles, and short communications. Academy of Dental Materials members click here to register for free access to Dental Materials online. The principal aim of Dental Materials is to promote rapid communication of scientific information between academia, industry, and the dental practitioner. Original Manuscripts on clinical and laboratory research of basic and applied character which focus on the properties or performance of dental materials or the reaction of host tissues to materials are given priority publication. Other acceptable topics include application technology in clinical dentistry and dental laboratory technology. Comprehensive reviews and editorial commentaries on pertinent subjects will be considered.
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