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细胞黏附分子埃-钙黏蛋白的一些结构和功能方面

Some structural and functional aspects of the cell adhesion molecule uvomorulin.

作者信息

Vestweber D, Kemler R

出版信息

Cell Differ. 1984 Dec;15(2-4):269-73. doi: 10.1016/0045-6039(84)90084-8.

Abstract

The cell adhesion molecule uvomorulin (UM) was analysed by comparing antisera produced against the whole molecule (gp123) with antisera made against fragments of UM. Of the proteins recognized by different anti-UM antisera (molecular weights of 123, 102, 92 and 84 kDa), the 102 kDa molecule is not derived from gp123. The 102 kDa molecule is not glycosylated and is also different from gp123 by peptide map analysis. However, rabbit antisera raised against the purified 102 kDa protein interfered with the aggregation of embryonal carcinoma (EC) cells. Also, a monoclonal antibody selected to interfere with EC cell aggregation recognized the 102 kDa molecule as well as gp123. Thus, the functional site of cell adhesion seems not to be mediated by sugar residues. Experimental evidence is provided suggesting that UM is not only involved in the compaction of preimplantation embryos but seems to be an ubiquitous cell adhesion molecule regulating epithelial cell adhesion mechanisms.

摘要

通过比较针对整个分子(gp123)产生的抗血清与针对uvomorulin(UM)片段产生的抗血清,对细胞粘附分子uvomorulin(UM)进行了分析。在不同抗UM抗血清识别的蛋白质(分子量分别为123、102、92和84 kDa)中,102 kDa的分子并非来自gp123。102 kDa的分子未被糖基化,并且通过肽图分析也与gp123不同。然而,针对纯化的102 kDa蛋白产生的兔抗血清会干扰胚胎癌细胞(EC)的聚集。此外,选择用于干扰EC细胞聚集的单克隆抗体也识别102 kDa的分子以及gp123。因此,细胞粘附的功能位点似乎不是由糖残基介导的。提供的实验证据表明,UM不仅参与着床前胚胎的紧密化,而且似乎是一种调节上皮细胞粘附机制的普遍存在的细胞粘附分子。

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