首页> 美国卫生研究院文献>The Journal of Biophysical and Biochemical Cytology >Tight junction structure and ZO-1 content are identical in two strains of Madin-Darby canine kidney cells which differ in transepithelial resistance
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Tight junction structure and ZO-1 content are identical in two strains of Madin-Darby canine kidney cells which differ in transepithelial resistance

机译:两种Madin-Darby犬肾细胞的紧密连接结构和ZO-1含量相同但跨上皮抵抗力不同

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摘要

The relationship of tight junction permeability to junction structure and composition was examined using two strains of Madin-Darby canine kidney (MDCK) cells (I and II) which differ greater than 30-fold in transepithelial resistance. This parameter is largely determined by paracellular, and hence junctional, permeability under most conditions. When these two strains of cells were grown on permeable filter supports, they formed monolayers with equivalent linear amounts of junction/area of monolayer. Ultrastructural analysis of these monolayers by thin section EM revealed no differences in overall cellular morphology or in tight junction organization. Morphometric analysis of freeze-fractured preparations indicated that the tight junctions of these two cell strains were similar in both number and density of junctional fibrils. Prediction of transepithelial resistance for the two strains from this freeze-fracture data and a published structure-function formulation (Claude, P. 1978, J. Memb. Biol. 39:219- 232) yielded values (I = 26.5 omega/cm2, II = 35.7 omega/cm2) that were significantly lower than those observed (I = 2,500-5,000 omega/cm2, II = 50-70 omega/cm2). Consistent with these structural studies, a comparison of the distribution and cellular content of ZO-1, a polypeptide localized exclusively to the tight junction, revealed no significant differences in either the localization of ZO-1 or the amount of ZO-1 per micron of junction (I = 1,415 +/- 101 molecules/micron, II = 1,514 +/- 215 molecules/micron).
机译:使用两株Madin-Darby犬肾(MDCK)细胞(I和II)检查了紧密连接通透性与连接结构和组成的关系,它们的跨上皮阻力相差30倍以上。在大多数情况下,该参数很大程度上取决于细胞旁的通透性,因此取决于连接的通透性。当这两个细胞株在可渗透滤膜支架上生长时,它们形成具有相等线性量的单层连接/区域的单层。通过薄层电磁波对这些单分子层的超微结构分析表明,总体细胞形态或紧密连接组织无差异。冷冻断裂制剂的形态分析表明,这两个细胞株的紧密连接在连接原纤维的数量和密度上相似。根据此冻裂数据和已发布的结构功能公式(Claude,P. 1978,J. Memb。Biol。39:219-232)预测这两个菌株的跨上皮抵抗力,得出的值(I = 26.5Ω/ cm2, II = 35.7Ω/ cm2),明显低于观察到的值(I = 2,500-5,000Ω/ cm2,II = 50-70Ω/ cm2)。与这些结构研究一致,ZO-1(仅位于紧密连接处的多肽)的分布和细胞含量的比较表明,ZO-1的定位或每微米颗粒的ZO-1的量均无显着差异。连接(I = 1,415 +/- 101分子/微米,II = 1,514 +/- 215分子/微米)。

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