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High-speed atomic force microscopy imaging of live mammalian cells

机译:哺乳动物活细胞的高速原子力显微镜成像

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Direct imaging of morphological dynamics of live mammalian cells with nanometer resolution under physiological conditions is highly expected, but yet challenging. High-speed atomic force microscopy (HS-AFM) is a unique technique for capturing biomolecules at work under near physiological conditions. However, application of HS-AFM for imaging of live mammalian cells was hard to be accomplished because of collision between a huge mammalian cell and a cantilever during AFM scanning. Here, we review our recent improvements of HS-AFM for imaging of activities of live mammalian cells without significant damage to the cell. The improvement of an extremely long (~3?μm) AFM tip attached to a cantilever enables us to reduce severe damage to soft mammalian cells. In addition, a combination of HS-AFM with simple fluorescence microscopy allows us to quickly locate the cell in the AFM scanning area. After these improvements, we demonstrate that developed HS-AFM for live mammalian cells is possible to image morphogenesis of filopodia, membrane ruffles, pits open-close formations, and endocytosis in COS-7, HeLa cells as well as hippocampal neurons.
机译:在生理条件下以纳米分辨率直接对活的哺乳动物细胞的形态动力学进行直接成像是令人期待的,但仍具有挑战性。高速原子力显微镜(HS-AFM)是一种独特的技术,可用于在接近生理条件下捕获工作中的生物分子。但是,由于在AFM扫描过程中巨大的哺乳动物细胞和悬臂之间发生了碰撞,因此很难将HS-AFM应用于活体哺乳动物细胞的成像。在这里,我们回顾了我们最近对HS-AFM的改进,用于对活的哺乳动物细胞的活动进行成像,而对细胞没有明显的破坏。连接到悬臂的超长(〜3?μm)AFM尖端的改进使我们能够减少对哺乳动物软细胞的严重破坏。此外,HS-AFM与简单的荧光显微镜相结合,使我们能够在AFM扫描区域中快速定位细胞。经过这些改进后,我们证明为哺乳动物活细胞开发的HS-AFM可能会在COS-7,HeLa细胞以及海马神经元中对丝状伪足,膜褶皱,凹坑开闭形成和内吞作用的图像进行成像。

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