Cellular ageing of oral fibroblasts differentially modulates extracellular matrix organization

纤维连接蛋白 细胞外基质 纤维蛋白 老化 成纤维细胞 衰老 细胞生物学 人口 伤口愈合 弹性蛋白 化学 病理 生物 分子生物学 免疫学 体外 生物化学 医学 遗传学 环境卫生
作者
Srividya Atkuru,Giridharan Muniraj,Thankiah Sudhaharan,Keng‐Hwee Chiam,Graham Wright,Gopu Sriram
出处
期刊:Journal of Periodontal Research [Wiley]
卷期号:56 (1): 108-120 被引量:17
标识
DOI:10.1111/jre.12799
摘要

Abstract Background and Objectives Ageing is associated with an impaired cellular function that can affect tissue architecture and wound healing in gingival and periodontal tissues. However, the impact of oral fibroblast ageing on the structural organization of the extracellular matrix (ECM) proteins is poorly understood. Hence, in this study, we investigated the impact of cellular ageing of oral fibroblasts on the production and structural organization of collagen and other ECM proteins. Methods Oral fibroblasts were serially subcultured, and replicative cellular senescence was assessed using population doubling time, Ki67 counts and expression of P21 WAFI . The production and structural organization of ECM proteins were assessed at early (young‐oFB) and late (aged‐oFB) passages. The thickness and pattern of collagen produced by live cultures of young‐ and aged‐oFB were assessed using a label‐free and non‐invasive second harmonic generation (SHG)‐based multiphoton imaging. Expression of other ECM proteins (fibronectin, fibrillin, collagen‐IV and laminins) was evaluated using immunocytochemistry and confocal microscopy‐based depth profile analysis. Results Aged‐oFB displayed a higher population doubling time, lower Ki67+ cells and higher expression of P21 WAFI indicative of slower proliferation rate and senescence phenotype. SHG imaging demonstrated that young‐oFB produced a thick, interwoven network of collagen fibres, while the aged‐oFB produced thin and linearly organized collagen fibres. Similarly, analysis of immunostained cultures showed that young‐oFB produced a rich, interwoven mesh of fibronectin, fibrillin and collagen‐IV fibres. In contrast, the aged‐oFB produced linearly organized fibronectin, fibrillin and collagen‐IV fibres. Lastly, there was no observable difference in production and organization of laminins among the young‐ and aged‐oFB. Conclusion Our results suggest that oral fibroblast ageing impairs ECM production and more importantly the organization of ECM fibres, which could potentially impair wound healing in the elderly.

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