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大鼠牙齿发育、稳态维持及再生过程中连接蛋白26、32和43的组合表达模式。

Combinatorial expression patterns of the connexins 26, 32, and 43 during development, homeostasis, and regeneration of rat teeth.

作者信息

Fried K, Mitsiadis T A, Guerrier A, Haegerstrand A, Meister B

机构信息

Department of Neuroscience, Karolinska Institutet, Stockholm, Sweden.

出版信息

Int J Dev Biol. 1996 Oct;40(5):985-95.

PMID:8946246
Abstract

Gap junctions permit the exchange of regulatory molecules between cells and play important roles during organogenesis. The expression pattern of the gap junction proteins connexin 26, 32, and 43 was studied by immunohistochemistry in the developing, adult, and injured rat teeth. Connexins 32 and 43, but not the connexin 26, were detected during the late stages of embryonic tooth development (bell stage). Expression of connexin 32 was predominant in epithelial cells, whereas connexin 43 was more widely distributed and found in both epithelial and mesenchymal cells. During cytodifferentiation (early postnatal stages), both connexin 32 and 43 were expressed in the epithelial-derived ameloblasts, synthesizing and secreting the enamel matrix proteins. In mesenchyme, connexin 32 was observed only in differentiating odontoblasts, while connexin 43 was expressed in both differentiating and functional odontoblasts, which secrete the dentin matrix. In adult rat teeth, connexin 26 and 43 were expressed in the odontoblastic layer at low and high levels, respectively, while connexin 32 was absent from odontoblasts. Electron microscopy showed that connexin 43 was distributed exclusively at sites of contacts between odontoblasts. However, double immunostaining combined with confocal microscopy suggested an occasional overlap between odontoblasts and calcitonin gene-related peptide-positive nerve fibers. Denervation experiments showed that the expression of connexins in dental pulp was independent of innervation, whereas in injured teeth connexin 43 was upregulated in pulpal fibroblasts. Finally, cultured dental epithelial cells expressed both connexin 32 and 43, and connexin 43 was detected in cultured pulp fibroblasts in vitro, thus mimicking the in vivo distribution pattern of connexins. These results demonstrate that connexins are involved in tooth development and suggest that a given connexin may have distinct roles during odontogenesis and tooth homeostasis.

摘要

缝隙连接允许细胞间调节分子的交换,并在器官发生过程中发挥重要作用。采用免疫组织化学方法,研究了缝隙连接蛋白连接蛋白26、32和43在发育中的、成年的和损伤的大鼠牙齿中的表达模式。在胚胎牙齿发育后期(钟状期)检测到连接蛋白32和43,但未检测到连接蛋白26。连接蛋白32在上皮细胞中表达占主导,而连接蛋白43分布更广泛,在上皮细胞和间充质细胞中均有发现。在细胞分化过程中(出生后早期阶段),连接蛋白32和43均在上皮来源的成釉细胞中表达,成釉细胞合成并分泌釉质基质蛋白。在间充质中,仅在分化中的成牙本质细胞中观察到连接蛋白32,而连接蛋白43在分化中的和成功能性的成牙本质细胞中均有表达,成牙本质细胞分泌牙本质基质。在成年大鼠牙齿中,连接蛋白26和43分别在成牙本质细胞层低水平和高水平表达,而成牙本质细胞中没有连接蛋白32。电子显微镜显示,连接蛋白43仅分布在成牙本质细胞之间的接触部位。然而,双重免疫染色结合共聚焦显微镜检查表明,成牙本质细胞与降钙素基因相关肽阳性神经纤维偶尔会有重叠。去神经支配实验表明,牙髓中连接蛋白的表达与神经支配无关,而在损伤的牙齿中,连接蛋白43在牙髓成纤维细胞中上调。最后,培养的牙上皮细胞表达连接蛋白32和43,并且在体外培养的牙髓成纤维细胞中检测到连接蛋白43,从而模拟了连接蛋白在体内的分布模式。这些结果表明连接蛋白参与牙齿发育,并提示特定的连接蛋白在牙发生和牙齿内环境稳定过程中可能具有不同的作用。

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