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Application of atomic force microscopy for studying intracellular signalization in neurons

机译:原子力显微镜在神经元细胞内信号转导研究中的应用

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The first attempt is made at applying the method of atomic force microscopy (AFM) for determining the molecular mechanisms of intracellular signalization with the participation of Na+, K+-ATPhase playing an important role of a signal transductor (amplifier). The AFM method combined with the organotypic cultivation makes it possible to obtain quantitative information on the Young moduli of living neurons and cells subjected to the action of very low concentrations of ouabain. This substance is known to trigger in this case the intracellular signalization processes by transferring a molecular signal to the genome of a cell. The cell response is manifested in a sharp intensification of protein synthesis accompanied by a rearrangement of the cytoskeleton and activation of enzyme signal pathways in a cytosol. AFM measurements of the images of the cell surface relief are performed using the PeakForce quantitative nanomechanical properties mapping PeakForce QNM mode. The Young moduli of control neurons and of sensory neurons under the action of ouabain are measured simultaneously. It is found that the activation of the signal-transducing function of Na+, K+-ATPhase triggers intracellular signal cascades, which increase the cell stiffness. The application of the AFM method in further studies of the mechanisms of intracellular molecular processes appears as promising. Its combination with inhibitory analysis will clarify the role of individual molecules (e.g., a number of ferments) in regulation of growth and development of living organisms.
机译:首次尝试应用原子力显微镜(AFM)方法来确定细胞内信号传导的分子机制,其中Na +,K + -ATPhase参与了信号转导(放大器)的重要作用。原子力显微镜方法与器官典型培养相结合,可以获取关于在极低浓度的哇巴因作用下的活神经元和细胞的杨氏模量的定量信息。在这种情况下,已知该物质通过将分子信号转移至细胞基因组来触发细胞内信号转导过程。细胞反应表现为蛋白质合成的急剧增强,伴随着细胞骨架的重新排列和胞浆中酶信号途径的激活。使用PeakForce定量纳米力学特性映射PeakForce QNM模式进行细胞表面起伏图像的AFM测量。同时测量在哇巴因作用下的控制神经元和感觉神经元的杨氏模量。发现Na +,K + -ATP酶的信号转导功能的激活触发细胞内信号级联,这增加了细胞的硬度。原子力显微镜方法在细胞内分子过程机理的进一步研究中的应用似乎很有希望。它与抑制性分析的结合将阐明单个分子(例如许多发酵液)在调节活生物体生长和发育中的作用。

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