[巴戟天多糖对炎症微环境中牙周韧带成纤维细胞 FN 和 FN-EDA 的影响]。

Q4 Medicine

上海口腔医学 Pub Date : 2024-04-01

Zan Zhang, Jing-Yi Dai, Hong-Xuan Cai, Wei-Xing Si, Jing-Wen Yang, Ya-Guang Tian

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引用次数: 0

摘要

目的：探讨巴戟天多糖（MOP）对炎性牙周韧带成纤维细胞中纤维粘连蛋白（FN）和含额外结构域A的纤维粘连蛋白（FN-EDA）表达的影响：将 36 只大鼠随机分为对照组（12 只）和模型组（24 只）。模型组采用正畸钢丝结扎法建立牙周炎。三周后，每组选取 6 只大鼠，经 Micro-CT 确认后完成建模。模型组的其余大鼠被随机分为牙周炎组、正常生理盐水（NS）组和 MOP 组。MOP组在大鼠左侧上颌第一磨牙腭侧注射MOP（200 mg/kg，3 d，50 μL，4周）。NS 组注射相同剂量的 NS，牙周炎组不进行任何治疗。取大鼠左上颌组织，用 H-E 染色法观察牙周组织的病理变化。免疫组化法检测 FN 和 FN-EDA 的表达。体外培养牙周韧带成纤维细胞，用 CCK-8 检测 MOP 对细胞活性的影响。第四代细胞分为对照组、炎症组（10 毫克/毫升脂多糖）和实验组（12.5 微克/毫升 MOP、12.5 微克/毫升 MOP+10 毫克/毫升脂多糖）。通过 qRT-PCR 和 Western 印迹检测 FN 和 FN-EDA 的表达。使用 Prism 8.0 软件包对数据进行统计分析：在体内实验中，MOP 组 FN-EDA 的表达明显低于牙周炎组和 NS 组（P＜0.05），炎症细胞浸润减少。但各组 FN 的表达无明显差异。在体外实验中，与对照组相比，炎症组 FN-EDA mRNA 和蛋白的表达明显增加（P＜0.000 1）。MOP能明显降低炎症细胞中FN-EDA的表达，但对FN的表达无明显影响：结论：随着 FN-EDA 在炎性牙周韧带组织和细胞中的表达增加，MOP 可能通过下调 FN-EDA 起到抑制炎症的作用。

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[Effects of Morinda officinalis polysaccharides on FN and FN-EDA of periodontal ligament fibroblasts in inflammatory microenvironment].

Purpose: To investigate the effect of Morinda officinalis polysaccharides(MOP) on the expression of fibronectin(FN) and fibronectin containing extra domain A(FN-EDA) in inflammatory periodontal ligament fibroblasts.

Methods: Thirty six rats were randomly divided into a control group(n=12) and a model group (n=24). The model group used orthodontic wire ligation to establish periodontitis. After three weeks, 6 rats from each group were selected and confirmed by Micro-CT to complete the modeling. The remaining rats in the model group were randomly divided into periodontitis group, normal saline(NS) group, and MOP group. In the MOP group, MOP (200 mg/kg for 3 d, 50 μL for 4 weeks) was injected into the palatal side of the left maxillary first molar of the rats. In the NS group, same volume of NS was injected, and no treatment was performed in the periodontitis group. The left maxillary tissue of rats were taken and the pathological changes of periodontal tissue were observed by H-E staining. The expression of FN and FN-EDA was detected by immunohistochemistry. Periodontal ligament fibroblasts were cultured in vitro, the effect of MOP on cell activity detected by CCK-8. The fourth generation cells were divided into control group, inflammation group (10 mg/mL lipopolysaccharide), and experimental group (12.5 μg/mL MOP, 12.5 μg/mL MOP+10 mg/mL lipopolysaccharide). The expression of FN and FN-EDA was detected by qRT-PCR and Western blot. The data were statistically analyzed using Prism 8.0 software package.

Results: In vivo experiments, the expression of FN-EDA in the MOP group was significantly lower than that in the periodontitis group and NS group(P＜0.05), and the infiltration of inflammatory cells was reduced. However, there was no significant difference in the expression of FN in each group. In vitro experiments, compared with the control group, the expression of FN-EDA mRNA and protein in the inflammation group was significantly increased(P＜0.000 1). MOP significantly reduced the expression of FN-EDA in inflammatory cells, but had no significant effect on FN expression.

Conclusions: With increased expression of FN-EDA in inflammatory periodontal ligament tissues and cells, MOP may play a role in inhibiting inflammation by down-regulating FN-EDA.

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来源期刊

上海口腔医学 Medicine-Medicine (all)

CiteScore

0.30

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0.00%

发文量

5299

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