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将诱导多能干细胞与端粒酶逆转录酶永生化的角质形成细胞和成纤维细胞一起整合到重建的人牙龈中,可增强牙龈上皮的表型。

Incorporation of iPSCs together with TERT-immortalized keratinocytes and fibroblasts into reconstructed human gingiva enhances phenotype of gingival epithelium.

作者信息

Brueske Lisa-Lee, Roffel Sanne, Beekhuis-Hoekstra Stephanie, de Vries Helga E, Gibbs Susan

机构信息

Department of Oral Cell Biology, Academic Centre for Dentistry Amsterdam (ACTA), University of Amsterdam and Vrije Universiteit Amsterdam, Amsterdam, The Netherlands.

Department of Molecular Cell Biology and Immunology, Amsterdam UMC Location Vrije Universiteit Amsterdam, Amsterdam, The Netherlands.

出版信息

PLoS One. 2025 Jul 21;20(7):e0327728. doi: 10.1371/journal.pone.0327728. eCollection 2025.

Abstract

The oral mucosa plays an important role in maintaining oral and systemic health by protecting the body from harmful environmental stimuli and pathogens. Current reconstructed human gingiva models (RhG) serve as valuable testing platforms for safety and efficacy testing of dental materials, however they lack important phenotypic characteristics typical of the gingival epithelium. We aimed to determine whether incorporating induced pluripotent stem cells (iPSCs) into the hydrogel of a cell-line RhG (reconstructed epithelium on fibroblast-populated-hydrogel) would improve its phenotype. Immortalized human gingival fibroblasts were resuspended with and without iPSCs in collagen-fibrin hydrogels and gingival keratinocytes were seeded on top of the hydrogels to construct RhGs. RhGs were cultured at air-liquid interface for 1, 2, 4 and 6 weeks and extensively characterized by immunohistochemistry. In situ hybridization for X and Y chromosomes was conducted to identify female iPSCs and male fibroblasts in the RhGs. iPSC-RhGs showed increased epithelial thickening, rete ridge formation, increased cell proliferation and normalized expression of differentiation markers (keratins, involucrin, loricrin, SKALP/elafin) compared to standard RhGs, resulting in an epithelial phenotype very similar to the native gingiva. An increase in apoptotic cells was detected in iPSC-RhGs after 1 week air-exposed culture, and no iPSCs were detected in the hydrogels after 2 weeks air-exposed culture. The increase in apoptotic iPSCs after 1 week air-exposed culture correlated with an increase in keratinocyte proliferation responsible for the superior phenotype observed at 2 weeks.

摘要

口腔黏膜通过保护身体免受有害环境刺激和病原体侵害,在维持口腔和全身健康方面发挥着重要作用。目前的重建人牙龈模型(RhG)可作为牙科材料安全性和有效性测试的重要平台,然而它们缺乏牙龈上皮典型的重要表型特征。我们旨在确定将诱导多能干细胞(iPSC)整合到细胞系RhG(成纤维细胞填充水凝胶上的重建上皮)的水凝胶中是否会改善其表型。将永生化人牙龈成纤维细胞在含有和不含有iPSC的情况下重悬于胶原-纤维蛋白水凝胶中,并将牙龈角质形成细胞接种在水凝胶顶部以构建RhG。将RhG在气液界面培养1、2、4和6周,并通过免疫组织化学进行广泛表征。进行X和Y染色体的原位杂交以鉴定RhG中的女性iPSC和男性成纤维细胞。与标准RhG相比,iPSC-RhG显示上皮增厚增加、 rete嵴形成、细胞增殖增加以及分化标志物(角蛋白、内披蛋白、兜甲蛋白、SKALP/弹性蛋白酶)表达正常化,从而产生与天然牙龈非常相似的上皮表型。在暴露于空气的培养1周后,在iPSC-RhG中检测到凋亡细胞增加,在暴露于空气的培养2周后,在水凝胶中未检测到iPSC。暴露于空气的培养1周后凋亡iPSC的增加与角质形成细胞增殖的增加相关,这导致在2周时观察到优异的表型。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f332/12279103/ed14b4b3542c/pone.0327728.g001.jpg

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