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在转染编码特定桥粒成分的基因后,培养细胞中桥粒的从头形成。

De novo formation of desmosomes in cultured cells upon transfection of genes encoding specific desmosomal components.

作者信息

Koeser Joachim, Troyanovsky Sergey M, Grund Christine, Franke Werner W

机构信息

Division of Cell Biology, German Cancer Research Center, D-69120, Heidelberg, Federal Republic of Germany.

出版信息

Exp Cell Res. 2003 Apr 15;285(1):114-30. doi: 10.1016/s0014-4827(03)00016-8.

Abstract

Desmosomes are cell junctions and cytoskeleton-anchoring structures of epithelia, the myocardium, and dendritic reticulum cells of lymphatic follicles whose major components are known. Using cultured HT-1080 SL-1 fibrosarcoma-derived cells and transfection of cDNAs encoding specific desmosomal components, we have determined a minimum ensemble of proteins sufficient to introduce de novo structures, which, by morphology and functional competence, are indistinguishable from authentic desmosomes. In a more refined analysis, the influence of the desmosomal proteins desmoplakin (Dp), plakoglobin (Pg), and plakophilin 2 (Pp2) on the lateral clustering of the desmosomal transmembrane-glycoprotein desmoglein 2 (Dsg) was examined. We found that for efficient clustering of desmoglein 2 and desmosome structure formation, all three major plaque proteins-desmoplakin, plakoglobin, and plakophilin 2- were necessary. Furthermore, in this cell model, plakophilin 2 was capable of directing desmoplakin to adhaerens junctions (AJ), whereas plakoglobin was crucial for the segregation of desmosomal and AJ components. These results are discussed with respect to the variability in cell junction composition observed in various nonepithelial tissues.

摘要

桥粒是上皮细胞、心肌以及淋巴滤泡树突状网状细胞的细胞连接和细胞骨架锚定结构,其主要成分已知。利用培养的源自HT - 1080 SL - 1纤维肉瘤的细胞以及编码特定桥粒成分的cDNA转染,我们确定了一组足以从头引入结构的最小蛋白质组合,这些结构在形态和功能能力上与真实桥粒无法区分。在更精细的分析中,研究了桥粒蛋白桥粒斑蛋白(Dp)、桥粒芯蛋白(Pg)和桥粒斑菲素蛋白2(Pp2)对桥粒跨膜糖蛋白桥粒芯糖蛋白2(Dsg)侧向聚集的影响。我们发现,为了实现桥粒芯糖蛋白2的有效聚集和桥粒结构形成,所有三种主要的斑块蛋白——桥粒斑蛋白、桥粒芯蛋白和桥粒斑菲素蛋白2——都是必需的。此外,在这个细胞模型中,桥粒斑菲素蛋白2能够将桥粒斑蛋白导向黏附连接(AJ),而桥粒芯蛋白对于桥粒和AJ成分的分离至关重要。针对在各种非上皮组织中观察到的细胞连接组成的变异性对这些结果进行了讨论。

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