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纳米拓扑结构通过胞质液体复合物增强紧密连接蛋白的动态重塑。

Nanotopography Enhances Dynamic Remodeling of Tight Junction Proteins through Cytosolic Liquid Complexes.

作者信息

Huang Xiao, Shi Xiaoyu, Hansen Mollie Eva, Setiady Initha, Nemeth Cameron L, Celli Anna, Huang Bo, Mauro Theodora, Koval Michael, Desai Tejal A

机构信息

Department of Bioengineering and Therapeutic Sciences, University of California, San Francisco, San Francisco, California 94158, United States.

Department of Pharmaceutical Chemistry, University of California, San Francisco, San Francisco, California 94158, United States.

出版信息

ACS Nano. 2020 Oct 27;14(10):13192-13202. doi: 10.1021/acsnano.0c04866. Epub 2020 Sep 24.

Abstract

Nanotopographic materials provide special biophysical stimuli that can regulate epithelial tight junctions and their barrier function. Through the use of total internal reflection fluorescence microscopy of live cells, we demonstrated that contact of synthetic surfaces with defined nanotopography at the apical surface of epithelial monolayers increased paracellular permeability of macromolecules. To monitor changes in tight junction morphology in live cells, we fluorescently tagged the scaffold protein zonula occludens-1 (ZO-1) through CRISPR/Cas9-based gene editing to enable live cell tracking of ZO-1 expressed at physiologic levels. Contact between cells and nanostructured surfaces destabilized junction-associated ZO-1 and promoted its arrangement into highly dynamic liquid cytosolic complexes with a 1-5 μm diameter. Junction-associated ZO-1 rapidly remodeled, and we observed the direct transformation of cytosolic complexes into junction-like structures. Claudin-family tight junction transmembrane proteins and F-actin also were associated with these ZO-1 containing cytosolic complexes. These data suggest that these cytosolic structures are important intermediates formed in response to nanotopographic cues that facilitate rapid tight junction remodeling in order to regulate paracellular permeability.

摘要

纳米拓扑材料提供特殊的生物物理刺激,可调节上皮紧密连接及其屏障功能。通过对活细胞进行全内反射荧光显微镜观察,我们证明,具有特定纳米拓扑结构的合成表面与上皮单层细胞顶端表面接触,会增加大分子的细胞旁通透性。为了监测活细胞中紧密连接形态的变化,我们通过基于CRISPR/Cas9的基因编辑对支架蛋白闭合小带蛋白1(ZO-1)进行荧光标记,以便对生理水平表达的ZO-1进行活细胞追踪。细胞与纳米结构表面之间的接触使与连接相关的ZO-1不稳定,并促使其排列成直径为1-5μm的高度动态的液态胞质复合物。与连接相关的ZO-1迅速重塑,并且我们观察到胞质复合物直接转变为连接样结构。闭合蛋白家族紧密连接跨膜蛋白和F-肌动蛋白也与这些含有ZO-1的胞质复合物相关。这些数据表明,这些胞质结构是响应纳米拓扑线索而形成的重要中间体,有助于快速的紧密连接重塑,从而调节细胞旁通透性。

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