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高速扫描探针显微镜观察活成纤维细胞前缘层的动力学。

Dynamics of leading lamellae of living fibroblasts visualized by high-speed scanning probe microscopy.

机构信息

Division of Biological Sciences, Graduate School of Science, Hokkaido University, Kita-ku, Sapporo, Japan.

出版信息

Histochem Cell Biol. 2010 Jan;133(1):59-67. doi: 10.1007/s00418-009-0644-7. Epub 2009 Oct 9.

Abstract

In this study, we aimed at improving the temporal resolution of scanning probe microscopy (SPM) for observing living cells by introducing soft cantilevers, low feedback-gain operations, and cantilever deflection imaging. We achieved visualization of the mechanical architecture in leading lamellae of living fibroblasts at a temporal resolution of around 10 s, which is higher than that of conventional contact-mode SPM. Time-lapse SPM could be used to monitor not only cytoskeletal dynamics but also the dynamics of numerous microgranules. Statistical analysis of microgranular motion revealed that the microgranules have superdiffusive behaviors and significant directional order of motion. We also found that the direction of their motion is correlated with the direction of growing actin stress fibers. The combination of SPM with fluorescence microscopy showed that vinculin, a component of cell-substratum adhesion sites, localizes at the microgranules. Our experimental data provides a new insight into the intracellular mechanical architecture and its structural dynamics, suggesting that high-speed live-cell SPM has great potential for investigating the structural origin of cellular dynamics.

摘要

在这项研究中,我们旨在通过引入软悬臂梁、低反馈增益操作和悬臂梁挠度成像来提高扫描探针显微镜(SPM)观察活细胞的时间分辨率。我们实现了对活成纤维细胞前导褶层中机械结构的可视化,时间分辨率约为 10 秒,高于传统的接触模式 SPM。时移 SPM 不仅可以用于监测细胞骨架动力学,还可以用于监测大量微颗粒的动力学。对微颗粒运动的统计分析表明,微颗粒具有超扩散行为和显著的运动方向有序性。我们还发现,它们的运动方向与生长的肌动蛋白应力纤维的方向相关。SPM 与荧光显微镜的结合表明,细胞-基质黏附位点的组成部分 vinculin 定位于微颗粒上。我们的实验数据为细胞内机械结构及其结构动力学提供了新的见解,表明高速活细胞 SPM 具有很大的潜力,可以用于研究细胞动力学的结构起源。

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