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The Role of ZO-2 in Modulating JAM-A and γ-Actin Junctional Recruitment, Apical Membrane and Tight Junction Tension, and Cell Response to Substrate Stiffness and Topography

by Hernández-Guzmán, Christian , Vázquez-Victorio, Genaro , Wadurkar, Anand Sunil , Alarcón, Lourdes , Méndez-Méndez, Juan Vicente , González-Mariscal, Lorenza , Pinto-Dueñas, Diana Cristina , Chanona-Pérez, José Jorge , Martín-Tapia, Dolores , Marsch, Patrick Matthew , Nangia, Shikha

in Actins - metabolism / Analysis / Atomic force microscopy / Extracellular matrix / Kinases / Muscle proteins / Phosphoproteins - metabolism / Proteins / Sensors / Tight Junctions - metabolism / Topography / Zonula Occludens-1 Protein - metabolism

2024

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The Role of ZO-2 in Modulating JAM-A and γ-Actin Junctional Recruitment, Apical Membrane and Tight Junction Tension, and Cell Response to Substrate Stiffness and Topography

2024

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The Role of ZO-2 in Modulating JAM-A and γ-Actin Junctional Recruitment, Apical Membrane and Tight Junction Tension, and Cell Response to Substrate Stiffness and Topography

2024

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Journal Article

The Role of ZO-2 in Modulating JAM-A and γ-Actin Junctional Recruitment, Apical Membrane and Tight Junction Tension, and Cell Response to Substrate Stiffness and Topography

Hernández-Guzmán, Christian,

Vázquez-Victorio, Genaro,

Wadurkar, Anand Sunil,

Alarcón, Lourdes,

Méndez-Méndez, Juan Vicente,

González-Mariscal, Lorenza,

Pinto-Dueñas, Diana Cristina,

Chanona-Pérez, José Jorge,

Martín-Tapia, Dolores,

Marsch, Patrick Matthew,

Nangia, Shikha

2024

Overview

This work analyzes the role of the tight junction (TJ) protein ZO-2 on mechanosensation. We found that the lack of ZO-2 reduced apical membrane rigidity measured with atomic force microscopy, inhibited the association of γ-actin and JAM-A to the cell border, and instead facilitated p114RhoGEF and afadin accumulation at the junction, leading to an enhanced mechanical tension at the TJ measured by FRET, with a ZO-1 tension probe, and increased tricellular TJ tension. Simultaneously, adherens junction tension measured with an E-cadherin probe was unaltered. The stability of JAM-A and ZO-2 binding was assessed by a collaborative in silico study. The absence of ZO-2 also impacted the cell response to the substrate, as monolayers plated in 20 kPa hydrogels developed holes not seen in parental cultures and displayed a retarded elongation and formation of cell aggregates. The absence of ZO-2 was sufficient to induce YAP and Snail nuclear accumulation in cells cultured over glass, but when ZO-2 KD cells were plated in nanostructured ridge arrays, they displayed an increased abundance of nuclear Snail and conspicuous internalization of claudin-4. These results indicate that the absence of ZO-2 also impairs the response of cells to substrate stiffness and exacerbates transformation triggered by substrate topography.

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Publisher

MDPI AG,MDPI

Subject

Actins - metabolism

/ Analysis

/ Atomic force microscopy

/ Extracellular matrix

/ Kinases

/ Muscle proteins

/ Phosphoproteins - metabolism