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Mapping nanomechanical properties of live cells using multi-harmonic atomic force microscopy

机译:使用多谐波原子力显微镜绘制活细胞的纳米力学特性图

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The nanomechanical properties of living cells, such as their surface elastic response and adhesion, have important roles in cellular processes such as morphogenesis~1, mechano-transduction~2, focal adhesion~3, motility~(4,5), metastasis~6 and drug delivery~(7-10). Techniques based on quasi-static atomic force microscopy techniques~(11-17) can map these properties, but they lack the spatial and temporal resolution that is needed to observe many of the relevant details. Here, we present a dynamic atomic force microscopy ~(18-28) method to map quantitatively the nanomechanical properties of live cells with a throughput (measured in pixels/minute) that is ~10-1,000 times higher than that achieved with quasi-static atomic force microscopy techniques. The local properties of a cell are derived from the 0th, 1st and 2nd harmonic components of the Fourier spectrum of the AFM cantilevers interacting with the cell surface. Local stiffness, stiffness gradient and the viscoelastic dissipation of live Escherichia coli bacteria, rat fibroblasts and human red blood cells were all mapped in buffer solutions. Our method is compatible with commercial atomic force microscopes and could be used to analyse mechanical changes in tumours, cells and biofilm formation with sub-10 nm detail.
机译:活细胞的纳米力学性能,例如其表面弹性反应和粘附,在细胞形成过程中起重要作用,例如形态发生〜1,机械转导〜2,局灶性粘附〜3,运动性〜(4,5),转移〜6和药物输送〜(7-10)。基于准静态原子力显微镜技术〜(11-17)的技术可以映射这些属性,但它们缺乏观察许多相关细节所需的时空分辨率。在这里,我们提出了一种动态原子力显微镜〜(18-28)方法来定量绘制活细胞的纳米力学性能,其吞吐量(以像素/分钟为单位)比准静态的吞吐量高约10-1,000倍。原子力显微镜技术。单元格的局部特性是从AFM悬臂与单元格表面相互作用的傅立叶光谱的第0,第1和第2谐波分量中得出的。活大肠杆菌,大鼠成纤维细胞和人红细胞的局部刚度,刚度梯度和粘弹性消散都绘制在缓冲溶液中。我们的方法与商业原子力显微镜兼容,可用于分析低于10 nm细节的肿瘤,细胞和生物膜形成中的机械变化。

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