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体外腭融合过程中内侧边缘上皮细胞的命运:通过DiI标记和共聚焦显微镜进行的分析

The fate of medial edge epithelial cells during palatal fusion in vitro: an analysis by DiI labelling and confocal microscopy.

作者信息

Carette M J, Ferguson M W

机构信息

Department of Cell and Structural Biology, University of Manchester, UK.

出版信息

Development. 1992 Feb;114(2):379-88. doi: 10.1242/dev.114.2.379.

Abstract

Fusion of bilateral shelves, to form the definitive mammalian secondary palate, is critically dependent on removal of the medial edge cells that constitute the midline epithelial seam. Conflicting views suggest that programmed apoptotic death or epithelial-mesenchymal transformation of these cells is predominantly involved. Due in part to the potentially ambiguous interpretation of static images and the notable absence of fate mapping studies, the process by which this is achieved has, however, remained mechanistically equivocal. Using an in vitro mouse model, we have selectively labelled palatal epithelia with DiI and examined the fate of medial edge epithelial (MEE) cells during palatal fusion by localisation using a combination of conventional histology and confocal laser scanning microscopy (CLSM). In dynamic studies using CLSM, we have made repetitive observations of the same palatal cultures in time-course investigations. Our results concurred with the established morphological criteria of seam degeneration; however, they provided no evidence of MEE cell death or transformation. Instead we report that MEE cells migrate nasally and orally out of the seam and are recruited into, and constitute, epithelial triangles on both the oral and nasal aspects of the palate. Subsequently these cells become incorporated into the oral and nasal epithelia on the surface of the palate. We hypothesize an alternative method of seam degeneration in vivo which largely conserves the MEE population by recruiting it into the nasal and oral epithelia.

摘要

双侧腭突融合形成最终的哺乳动物次生腭,关键取决于构成中线上皮缝的内侧边缘细胞的清除。相互矛盾的观点表明,这些细胞的程序性凋亡死亡或上皮-间充质转化起主要作用。然而,部分由于静态图像的解释可能存在歧义,且明显缺乏细胞命运图谱研究,实现这一过程的机制仍不明确。利用体外小鼠模型,我们用碘化丙啶选择性标记腭上皮,通过结合传统组织学和共聚焦激光扫描显微镜(CLSM)定位,研究腭融合过程中内侧边缘上皮(MEE)细胞的命运。在使用CLSM的动态研究中,我们在时间进程研究中对相同的腭培养物进行了重复观察。我们的结果与已确立的缝退化形态学标准一致;然而,它们没有提供MEE细胞死亡或转化的证据。相反,我们报告MEE细胞从缝中向鼻腔和口腔迁移,并被招募到腭的口腔和鼻腔两侧的上皮三角形中并构成其一部分。随后,这些细胞被纳入腭表面的口腔和鼻腔上皮。我们假设一种体内缝退化的替代方法,该方法通过将MEE细胞招募到鼻腔和口腔上皮中,在很大程度上保留了MEE细胞群体。

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