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两类紧密连接可通过ZO-1亚型显示出来。

Two classes of tight junctions are revealed by ZO-1 isoforms.

作者信息

Balda M S, Anderson J M

机构信息

Department of Internal Medicine, Yale University School of Medicine, New Haven, Connecticut 06510.

出版信息

Am J Physiol. 1993 Apr;264(4 Pt 1):C918-24. doi: 10.1152/ajpcell.1993.264.4.C918.

DOI:10.1152/ajpcell.1993.264.4.C918
PMID:7682777
Abstract

The tight junction forms the intercellular barrier separating tissue compartments. The characteristics of this barrier are remarkably diverse among different epithelia and endothelia and are not explained by our limited knowledge of its molecular composition. Two isoforms of the 220-kDa tight junction protein ZO-1 result from alternative RNA splicing and differ by an internal 80-amino acid domain, termed alpha (E. Willott, M. S. Balda, M. Heintzman, B. Jameson, and J. M. Anderson. Am. J. Physiol. 262 (Cell Physiol. 31): C1119-C1124, 1992). Using antibodies specific for each isoform and double-labeled immunofluorescence microscopy, we observed that the ZO-1 alpha- isoform is restricted to junctions of endothelial cells and highly specialized epithelial cells of both seminiferous tubules (Sertoli cells) and renal glomeruli (podocytes); in contrast, the ZO-1 alpha+ isoform is expressed in cells of all other epithelia examined. Both immunoblotting and ribonuclease protection analysis confirmed this pattern of expression. This distribution does not correlate with differences in junctional resistance or ultrastructural complexity. Instead, we observe a correlation with junctional plasticity; ZO-1 alpha- is expressed in structurally dynamic junctions, whereas ZO-1 alpha+ is expressed in those which are less dynamic. This is the first molecular distinction among tight junctions and reveals a fundamental dichotomy with implications for how the paracellular barriers of endothelia and epithelia are regulated.

摘要

紧密连接形成分隔组织区室的细胞间屏障。这种屏障的特性在不同的上皮细胞和内皮细胞之间存在显著差异,而我们对其分子组成的有限了解并不能解释这些差异。220 kDa紧密连接蛋白ZO-1的两种同工型是由可变RNA剪接产生的,它们的区别在于一个内部的80个氨基酸结构域,称为α(E. Willott、M. S. Balda、M. Heintzman、B. Jameson和J. M. Anderson。《美国生理学杂志》262卷(细胞生理学31):C1119 - C1124,1992年)。使用针对每种同工型的特异性抗体和双标记免疫荧光显微镜,我们观察到ZO-1α-同工型仅限于内皮细胞以及生精小管(支持细胞)和肾小球(足细胞)的高度特化上皮细胞的连接;相反,ZO-1α+同工型在所有其他检查的上皮细胞中表达。免疫印迹和核糖核酸酶保护分析均证实了这种表达模式。这种分布与连接电阻或超微结构复杂性的差异无关。相反,我们观察到它与连接可塑性相关;ZO-1α-在结构动态的连接中表达,则ZO-1α+在动态性较低的连接中表达。这是紧密连接之间的首次分子区分,并揭示了一种基本的二分法,对内皮细胞和上皮细胞的细胞旁屏障的调节方式具有重要意义。

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