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Antibodies to high molecular weight polypeptides of desmosomes: specific localization of a class of junctional proteins in cells and tissue.桥粒高分子量多肽抗体:一类连接蛋白在细胞和组织中的特异性定位
Differentiation. 1981;20(3):217-41. doi: 10.1111/j.1432-0436.1981.tb01178.x.
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Stratification and terminal differentiation of cultured epidermal cells.培养的表皮细胞的分层与终末分化。
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Different modes of internalization of proteins associated with adhaerens junctions and desmosomes: experimental separation of lateral contacts induces endocytosis of desmosomal plaque material.与黏着连接和桥粒相关的蛋白质的不同内化模式:侧向接触的实验性分离诱导桥粒斑物质的内吞作用。
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Desmoplakins of epithelial and myocardial desmosomes are immunologically and biochemically related.上皮和心肌桥粒中的桥粒斑蛋白在免疫学和生物化学上相关。
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钙诱导培养的人角质形成细胞中桥粒成分的重组。

Calcium-induced reorganization of desmosomal components in cultured human keratinocytes.

作者信息

Watt F M, Mattey D L, Garrod D R

出版信息

J Cell Biol. 1984 Dec;99(6):2211-5. doi: 10.1083/jcb.99.6.2211.

DOI:10.1083/jcb.99.6.2211
PMID:6209289
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2113584/
Abstract

We used antibodies raised against individual desmosomal components to study calcium-induced desmosome formation in human keratinocytes. When keratinocytes are forced to grow as a monolayer by reducing the level of calcium ions in the culture medium, there is little contact between adjacent cells. Raising the level of calcium ions rapidly induces desmosome formation, and stratification occurs within 24 h. We found that before addition of calcium the 115,000- and 100,000-mol-wt core glycoproteins were distributed over the entire cell surface, whereas the plaque proteins (205,000 and 230,000 mol wt), the 82,000- and 86,000-mol-wt proteins, and the 150,000-mol-wt glycoprotein were located throughout the cytoplasm. 15 min after increasing the calcium ion concentration, all of these molecules appeared at the cell margins. The intensity of peripheral staining increased over the next 2 h and during this time the distribution of keratin filaments changed from predominantly perinuclear to extend throughout the cytoplasm. Keratinocytes could be dissociated with EDTA for up to 2 h after exposure to calcium. After 3 h of exposure to calcium the cells were no longer susceptible to EDTA dissociation and staining for desmosomal plaque antigens persisted in regions of intercellular contact. Desmosomal staining in stratified cultures became greatly reduced within 24 h of lowering the calcium ion concentration again. We have preliminary evidence that stratification occurs by breakdown of desmosomes at lateral surfaces and reformation at surfaces of contact between basal and suprabasal cells, rather than by rearrangement of existing desmosomes. Involucrin-positive cells in the monolayer appeared to contain more 205,000- and 230,000-mol-wt proteins free in the cytoplasm than involucrin-negative cells.

摘要

我们使用针对单个桥粒成分产生的抗体,来研究钙离子诱导人角质形成细胞中桥粒形成的过程。当通过降低培养基中钙离子水平迫使角质形成细胞单层生长时,相邻细胞间几乎没有接触。提高钙离子水平会迅速诱导桥粒形成,并且在24小时内会发生分层。我们发现,在添加钙离子之前,115,000和100,000道尔顿的核心糖蛋白分布在整个细胞表面,而斑块蛋白(205,000和230,000道尔顿)、82,000和86,000道尔顿的蛋白以及150,000道尔顿的糖蛋白则分布在整个细胞质中。增加钙离子浓度15分钟后,所有这些分子都出现在细胞边缘。在接下来的2小时内,周边染色强度增加,在此期间,角蛋白丝的分布从主要位于核周变为延伸至整个细胞质。角质形成细胞在接触钙离子后长达2小时可用EDTA解离。接触钙离子3小时后,细胞不再易受EDTA解离影响,并且桥粒斑块抗原染色在细胞间接触区域持续存在。再次降低钙离子浓度24小时内,分层培养物中的桥粒染色大大减少。我们有初步证据表明,分层是通过侧面桥粒的分解以及基底细胞和基底上层细胞接触表面的重新形成而发生的,而不是通过现有桥粒的重新排列。单层中含兜甲蛋白阳性的细胞似乎比含兜甲蛋白阴性的细胞在细胞质中含有更多游离的205,000和230,000道尔顿的蛋白。