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在单层囊泡中重建的 Claudin-4 足以形成分隔膜蛋白的紧密界面。

Claudin-4 reconstituted in unilamellar vesicles is sufficient to form tight interfaces that partition membrane proteins.

机构信息

Department of Bioengineering and Biophysics Program, University of California, Berkeley, CA 94720, USA.

Department of Internal Medicine & Center for Investigation of Membrane Excitability Disease, Washington University Medical School, St. Louis, MO 63110, USA.

出版信息

J Cell Sci. 2018 Oct 31;132(4):jcs221556. doi: 10.1242/jcs.221556.

Abstract

Tight junctions have been hypothesized to act as molecular fences in the plasma membrane of epithelial cells, helping to form differentiated apical and basolateral domains. While this fence function is believed to arise from the interaction of four-pass transmembrane claudins, the complexity of tight junctions has made direct evidence of their role as a putative diffusion barrier difficult to obtain. Here, we address this challenge by reconstituting claudin-4 into giant unilamellar vesicles using microfluidic jetting. We find that reconstituted claudin-4 alone can form adhesive membrane interfaces without the accessory proteins that are present By controlling the molecular composition of the inner and outer leaflets of jetted vesicle membranes, we show that claudin-4-mediated interfaces can drive partitioning of extracellular membrane proteins with ectodomains as small as 5 nm but not of inner or outer leaflet lipids. Our findings indicate that homotypic interactions of claudins and their small size can contribute to the polarization of epithelial cells.

摘要

紧密连接被假设为上皮细胞质膜中的分子围栏,有助于形成分化的顶侧和基底外侧区域。虽然这种围栏功能被认为是由四跨膜闭合蛋白的相互作用产生的,但紧密连接的复杂性使得直接获得它们作为假定扩散屏障的作用的证据变得困难。在这里,我们通过使用微流喷射将紧密连接蛋白-4重构成巨大的单层囊泡来解决这一挑战。我们发现,单独的重组紧密连接蛋白-4可以在没有辅助蛋白的情况下形成粘性的膜界面,而这些辅助蛋白存在于 通过控制喷射囊泡膜的内、外叶的分子组成,我们表明,紧密连接蛋白-4介导的界面可以驱动外域小至 5nm 的细胞外膜蛋白的分区,但不能驱动内或外叶层脂质的分区。我们的发现表明,紧密连接蛋白的同源相互作用及其小尺寸可以有助于上皮细胞的极化。

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