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糖化胶原蛋白刺激牙龈肌成纤维细胞的分化。

Glycated Collagen Stimulates Differentiation of Gingival Myofibroblasts.

机构信息

Department of Dentistry, Faculty of Medicine, Pontifical Catholic University of Chile (Pontificia Universidad Católica de Chile), Santiago, Chile.

Physics Department, University of Santiago, Santiago, Chile.

出版信息

J Periodontol. 2017 Sep;88(9):926-935. doi: 10.1902/jop.2017.160730. Epub 2017 May 18.

Abstract

BACKGROUND

Glucose-derived metabolites may alter the structure and biologic properties of important proteins in periodontium, such as collagens. As a consequence, it is possible that collagen-binding cells may change their phenotypic traits. Although the glucose-derived product methylglyoxal (MGO) has been detected in periodontal lesions, the precise effect of collagen glycation on gingival connective tissue biology is not fully understood. The present study evaluates whether collagen glycation by MGO may affect phenotypic properties and remodeling capacity of human gingival fibroblasts (HGFs).

METHODS

Primary cultures of HGFs were grown on Type I collagen matrices previously treated with MGO. Cell cultures were tested for cell viability, apoptosis, α-smooth muscle actin (SMA), fibronectin (FN) production, and collagen remodeling. Mechanical properties and morphology of MGO-treated collagen gels were evaluated using rheometry and atomic force microscopy. Statistical analysis was performed by Kruskal-Wallis and Mann-Whitney U tests.

RESULTS

MGO-treated collagen did not affect cell viability or apoptosis. In addition, MGO did not induce significant changes in morphology or mechanical properties of the collagen matrix. However, MGO-treated collagen stimulated an increase in the myofibroblast marker α-SMA, production and assembly of FN, and contraction of collagen matrices. Moreover, use of a triple-helical peptide that reconstitutes the collagen-binding domain for integrins GFOGER reverted the assembly of FN induced by MGO-treated collagen.

CONCLUSIONS

The present study shows that collagen glycation by MGO stimulates differentiation of myofibroblasts and production and assembly of FN. These responses may alter the homeostatic balance and wound-healing response of gingival connective tissues affected by diabetes mellitus or aging.

摘要

背景

葡萄糖衍生代谢物可能会改变牙周组织中重要蛋白质(如胶原蛋白)的结构和生物学特性。因此,胶原结合细胞可能会改变其表型特征。尽管已经在牙周病损中检测到葡萄糖衍生产物甲基乙二醛(MGO),但胶原蛋白糖化对牙龈结缔组织生物学的确切影响尚未完全阐明。本研究评估了 MGO 对胶原蛋白的糖化是否可能影响人牙龈成纤维细胞(HGF)的表型特性和重塑能力。

方法

将原代培养的 HGF 接种在预先用 MGO 处理的 I 型胶原基质上。对细胞培养物进行细胞活力、细胞凋亡、α-平滑肌肌动蛋白(α-SMA)、纤维连接蛋白(FN)产生和胶原重塑的检测。使用流变仪和原子力显微镜评估 MGO 处理的胶原凝胶的机械性能和形态。通过 Kruskal-Wallis 和 Mann-Whitney U 检验进行统计分析。

结果

MGO 处理的胶原蛋白不影响细胞活力或细胞凋亡。此外,MGO 对胶原基质的形态或机械性能没有引起明显变化。然而,MGO 处理的胶原蛋白刺激肌成纤维细胞标志物 α-SMA 的增加、FN 的产生和组装以及胶原基质的收缩。此外,使用重新构建整合素 GFOGER 胶原结合域的三螺旋肽可逆转 MGO 处理的胶原蛋白诱导的 FN 组装。

结论

本研究表明,MGO 对胶原蛋白的糖化刺激了肌成纤维细胞的分化以及 FN 的产生和组装。这些反应可能会改变受糖尿病或衰老影响的牙龈结缔组织的动态平衡和愈合反应。

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