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去除细胞外钙离子后,细胞间黏附连接中膜-微丝相互作用的变化。

Changes in membrane-microfilament interaction in intercellular adherens junctions upon removal of extracellular Ca2+ ions.

作者信息

Volberg T, Geiger B, Kartenbeck J, Franke W W

出版信息

J Cell Biol. 1986 May;102(5):1832-42. doi: 10.1083/jcb.102.5.1832.

Abstract

EGTA-induced depletion of Ca2+ ions from the culture medium of Madin-Darby bovine kidney epithelial cells results in rapid splitting of adherens-type junctions and the detachment of the vinculin- and actin-containing filament bundle from the cytoplasmic faces of the plasma membrane of the zonula adhaerens. This process was monitored by phase-contrast microscopy, combined with electron microscopy and immunofluorescent localization of the two proteins. It is shown that shortly after extracellular free Ca2+ concentration is lowered to the micromolar range, the actin-containing, junction-associated belt of microfilaments, together with the vinculin-rich junctional plaque material, is irreversibly detached as one structural unit from the plasma membrane, contracts, and is displaced towards the perinuclear cytoplasm where it gradually disintegrates. Other actin- and vinculin-containing structures present in the same cells, notably the focal contacts at the substratum, are not similarly affected by the Ca2+ depletion and retain both the adhesion to the external surface and the association with the plaque and microfilament components. Electron microscopic examination has shown that the membrane domain of the zonulae adhaerentes, unlike that of desmosomes, is not endocytosed after Ca2+ removal and that the displaced actin- and vinculin-containing plaque and filament belt are not associated with a particular membrane. It is further shown that upon restoration of normal Ca2+ levels in the culture medium, new intercellular contacts are established gradually by accretion of both vinculin and actin into new belt-like plaque- and microfilament-containing structures.

摘要

乙二醇双(2-氨基乙基醚)四乙酸(EGTA)诱导从Madin-Darby牛肾上皮细胞培养基中耗尽钙离子,导致黏附连接快速分裂,含纽蛋白和肌动蛋白的丝束从小带黏附处质膜的胞质面脱离。通过相差显微镜、结合电子显微镜以及这两种蛋白质的免疫荧光定位对该过程进行监测。结果显示,在细胞外游离钙离子浓度降低到微摩尔范围后不久,含肌动蛋白的、与连接相关的微丝带,连同富含纽蛋白的连接斑物质,作为一个结构单元从质膜上不可逆地脱离,收缩并向核周细胞质移位,在那里逐渐解体。同一细胞中存在的其他含肌动蛋白和纽蛋白的结构,特别是与基质的黏着斑,不受钙离子耗尽的类似影响,保持对外表面的黏附以及与斑和微丝成分的关联。电子显微镜检查表明,与桥粒不同,小带黏附处的膜结构域在钙离子去除后不会被内吞,并且移位的含肌动蛋白和纽蛋白的斑和丝带不与特定膜相关联。进一步表明,在培养基中恢复正常钙离子水平后,通过将纽蛋白和肌动蛋白积累到新的含斑和微丝的带状结构中,逐渐建立新的细胞间接触。

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