Department of Oral Biological and Medical Sciences, Faculty of Dentistry, University of British Columbia, Vancouver, B.C., Canada.
Cells Tissues Organs. 2011;193(1-2):53-63. doi: 10.1159/000320178. Epub 2010 Nov 3.
The medial epithelial seam (MES) between the palatal shelves degrades during palatal fusion to achieve the confluence of palatal mesenchyme. Cellular mechanisms underlying the degradation of MES have been proposed, such as apoptosis, epithelial-mesenchymal transition (EMT) and migration of medial edge epithelia (MEE). Extracellular matrix components have been shown to play an important role in EMT in many model systems. Periostin (also known as osteoblast-specific factor-2) is a secreted mesenchymal extracellular matrix component that affects the ability of cells to migrate and/or facilitates EMT during both embryonic development and pathologic conditions. In this study, we evaluated the spatiotemporal expression patterns of periostin during mouse palatal fusion by in situ hybridization and immunofluorescence. Periostin mRNA and protein were present in the palatal mesenchyme, the protein being distributed in a fine fibrillar network and in the basement membrane, but absent from the epithelium. During MES degradation, the protein was strongly expressed in the basement membrane underlying the MES and in some select MEE. Confocal microscopic analysis using an EMT marker, twist1, and an epithelial marker, cytokeratin 14, provided evidence that select MEE were undergoing EMT in association with periostin. Moreover, the major extracellular matrix molecules in basement membrane, laminin and collagen type IV were degraded earlier than periostin. The result is that select MEE establish interactions with periostin in the mesenchymal extracellular matrix, and these new cell-matrix interactions may regulate MEE transdifferentiation during palatal fusion.
中隔上皮缝(MES)在腭融合过程中降解,以实现腭间充质的融合。已经提出了 MES 降解的细胞机制,例如细胞凋亡、上皮-间充质转化(EMT)和中隔缘上皮(MEE)的迁移。已经表明细胞外基质成分在许多模型系统中的 EMT 中发挥重要作用。骨膜蛋白(也称为成骨细胞特异性因子-2)是一种分泌的间充质细胞外基质成分,它影响细胞迁移的能力和/或在胚胎发育和病理条件下促进 EMT。在这项研究中,我们通过原位杂交和免疫荧光评估了骨膜蛋白在小鼠腭融合过程中的时空表达模式。骨膜蛋白 mRNA 和蛋白存在于腭间充质中,蛋白分布在细纤维网络和基膜中,但不存在于上皮中。在 MES 降解过程中,蛋白在 MES 下方的基膜中强烈表达,并在一些选定的 MEE 中表达。使用 EMT 标志物 twist1 和上皮标志物角蛋白 14 进行共聚焦显微镜分析,提供了证据表明,一些选定的 MEE 正在发生 EMT,与骨膜蛋白有关。此外,基膜中的主要细胞外基质分子层粘连蛋白和 IV 型胶原比骨膜蛋白更早降解。结果是,选定的 MEE 在间质细胞外基质中与骨膜蛋白建立相互作用,这些新的细胞-基质相互作用可能调节腭融合过程中 MEE 的转分化。