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Quantitative evaluation of the impact of artificial cell adhesion via DNA hybridization on E-cadherin-mediated cell adhesion

机译:通过DNA杂交对E-钙黏着蛋白介导的细胞黏附的人工细胞黏附影响的定量评估

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摘要

Programmable cell adhesion with DNA hybridization is a promising approach for fabricating various tissue architectures without sophisticated instrumentation. However, little is known about how this artificial interaction influences the binding of cell adhesion proteins, E-cadherin. In this work, we designed a planar and fluid lipid membrane displaying E-cadherin and/or single-strand DNA with well-defined densities. Visualization of cells on membranes by fluorescence and interference microscopy revealed cell adhesion to be a two-step process: artificial adhesion by DNA hybridization within a few minutes followed by biological adhesion via cadherin-cadherin binding within hours. Furthermore, we discovered that DNA hybridization can substantially facilitate E-cadherin-mediated cell adhesion. The promotive effect is probably due to the enforced binding between E-cadherin molecules in geometrical confinement between two membranes. Our model of cell adhesion can potentially be used to design functional synthetic molecules that can regulate cell adhesion via cell adhesion proteins for tissue engineering.
机译:具有DNA杂交的可编程细胞粘附是一种无需复杂仪器即可制造各种组织结构的有前途的方法。然而,关于这种人工相互作用如何影响细胞粘附蛋白E-钙黏着蛋白的结合,知之甚少。在这项工作中,我们设计了一种平面和液状脂质膜,可显示具有明确定义的密度的E-钙黏着蛋白和/或单链DNA。通过荧光和干涉显微镜对膜上细胞的可视化显示细胞粘附是一个两步过程:在几分钟内通过DNA杂交进行人工粘附,然后在数小时内通过钙粘蛋白-钙粘蛋白结合进行生物粘附。此外,我们发现DNA杂交可以大大促进E-钙粘蛋白介导的细胞粘附。促进作用可能是由于在两个膜之间的几何限制中E-钙粘着蛋白分子之间的强制结合。我们的细胞粘附模型可以潜在地用于设计功能性合成分子,该分子可以通过细胞粘附蛋白调节细胞粘附,从而用于组织工程。

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