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Coupling integrin dynamics to cellular adhesion behaviors

机译:整合素动力学与细胞粘附行为的耦合

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Visualizing fluorescent proteins is essential for understanding cellular function. While advances in microscopy can now resolve individual molecules, determining whether the labeled molecules report native behaviors and how the measured behaviors can be coupled to cellular outputs remains challenging. Here, we used integrin alpha-beta heterodimers – which connect extracellular matrix (ECM) and the cytoskeleton – to quantify the mobility and conformation of labeled integrins. We found that while unlabeled and labeled integrins all localized to adhesions and support anchorage-dependent cell function, integrin mobility decreased when the beta rather than the alpha subunit was labeled. In contrast to unlabeled and alpha labeled subunits, beta labeled subunits changed cellular behavior; decreasing protrusive activity and increasing adhesion size and the extent of cell spreading. Labeling the beta subunit changed the integrin conformation, extending the molecule and exposing an epitope that is revealed by activation with Mn2+treatment. Our findings indicate labeling induced changes in dynamic integrin behavior alter molecular conformation as well as cellular adhesion-dependent function to demonstrate a coupling between molecular inputs and distinct cellular outputs.This article has an associated First Person interview with the first author of the paper.
机译:可视化荧光蛋白对于理解细胞功能至关重要。虽然显微镜技术的进步现在可以分辨单个分子,但是确定标记分子是否报告天然行为以及如何将测得的行为与细胞输出结合仍然具有挑战性。在这里,我们使用了整合素α-β异二聚体-连接细胞外基质(ECM)和细胞骨架-定量标记的整合素的迁移率和构象。我们发现,虽然未标记和标记的整联蛋白均定位于粘连并支持锚定依赖性细胞功能,但当标记β而不是α亚基时,整联蛋白的迁移率下降。与未标记和亚标记的亚基相比,β标记的亚基改变了细胞的行为。减少突出活动,增加粘附大小和细胞扩散程度。标记β亚基改变了整联蛋白构象,扩展了分子并暴露了通过Mn2 +处理激活所揭示的表位。我们的发现表明标记诱导的动态整联蛋白行为的变化改变了分子构象以及细胞粘附依赖性功能,以证明分子输入与不同细胞输出之间的耦合。本文与第一作者相关的第一人称访谈。

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