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J Vis Exp. 2013 May 27(75):e50477. doi: 10.3791/50477.
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The formation of actin waves during regeneration after axonal lesion is enhanced by BDNF.BDNF 增强轴突损伤后再生过程中肌动蛋白波的形成。
Sci Rep. 2011;1:183. doi: 10.1038/srep00183. Epub 2011 Dec 6.
2
Long-range and long-term interferometric tracking by static and dynamic force-clamp optical tweezers.
Opt Express. 2011 Nov 7;19(23):22364-76. doi: 10.1364/OE.19.022364.
3
Optical delivery of liposome encapsulated chemical stimuli to neuronal cells.脂质体包裹的化学刺激物的光学传递到神经元细胞。
J Biomed Opt. 2011 Sep;16(9):095001. doi: 10.1117/1.3616133.
4
Combined optical tweezers and laser dissector for controlled ablation of functional connections in neural networks.联合光学镊子和激光解剖器用于神经网络中功能连接的控制消融。
J Biomed Opt. 2011 May;16(5):051306. doi: 10.1117/1.3560268.
5
The role of stretching in slow axonal transport.拉伸在缓慢轴突运输中的作用。
Biophys J. 2011 Jan 19;100(2):351-60. doi: 10.1016/j.bpj.2010.12.3695.
6
Surgery with molecular fluorescence imaging using activatable cell-penetrating peptides decreases residual cancer and improves survival.使用可激活细胞穿透肽的分子荧光成像引导手术可减少残留肿瘤并改善生存。
Proc Natl Acad Sci U S A. 2010 Mar 2;107(9):4317-22. doi: 10.1073/pnas.0910261107. Epub 2010 Feb 16.
7
Axon extension occurs independently of centrosomal microtubule nucleation.轴突延伸独立于中心体微管成核。
Science. 2010 Feb 5;327(5966):704-7. doi: 10.1126/science.1182179. Epub 2010 Jan 7.
8
Cell stimulation with optically manipulated microsources.利用光学操控的微源进行细胞刺激。
Nat Methods. 2009 Dec;6(12):905-9. doi: 10.1038/nmeth.1400. Epub 2009 Nov 15.
9
A physical model of axonal elongation: force, viscosity, and adhesions govern the mode of outgrowth.轴突伸长的物理模型:力、粘度和粘附作用决定生长模式。
Biophys J. 2008 Apr 1;94(7):2610-20. doi: 10.1529/biophysj.107.117424. Epub 2008 Jan 4.
10
Filopodia act as phagocytic tentacles and pull with discrete steps and a load-dependent velocity.丝状伪足起到吞噬触手的作用,并以离散的步骤和负载依赖的速度进行拉动。
Proc Natl Acad Sci U S A. 2007 Jul 10;104(28):11633-8. doi: 10.1073/pnas.0702449104. Epub 2007 Jul 9.

在皮牛顿和毫秒分辨率下测量激光诱导轴突损伤过程中的张力释放,以评估轴突与底物的粘附力。

Measurement of tension release during laser induced axon lesion to evaluate axonal adhesion to the substrate at piconewton and millisecond resolution.

作者信息

Vassalli Massimo, Basso Michele, Difato Francesco

机构信息

Institute of Biophysics, National Research Council of Italy.

出版信息

J Vis Exp. 2013 May 27(75):e50477. doi: 10.3791/50477.

DOI:10.3791/50477
PMID:23748878
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3720120/
Abstract

The formation of functional connections in a developing neuronal network is influenced by extrinsic cues. The neurite growth of developing neurons is subject to chemical and mechanical signals, and the mechanisms by which it senses and responds to mechanical signals are poorly understood. Elucidating the role of forces in cell maturation will enable the design of scaffolds that can promote cell adhesion and cytoskeletal coupling to the substrate, and therefore improve the capacity of different neuronal types to regenerate after injury. Here, we describe a method to apply simultaneous force spectroscopy measurements during laser induced cell lesion. We measure tension release in the partially lesioned axon by simultaneous interferometric tracking of an optically trapped probe adhered to the membrane of the axon. Our experimental protocol detects the tension release with piconewton sensitivity, and the dynamic of the tension release at millisecond time resolution. Therefore, it offers a high-resolution method to study how the mechanical coupling between cells and substrates can be modulated by pharmacological treatment and/or by distinct mechanical properties of the substrate.

摘要

发育中的神经网络中功能连接的形成受外在线索影响。发育中神经元的轴突生长受化学和机械信号支配,但其感知和响应机械信号的机制尚不清楚。阐明力在细胞成熟中的作用将有助于设计能促进细胞黏附以及细胞骨架与底物耦合的支架,从而提高不同神经元类型损伤后再生的能力。在此,我们描述一种在激光诱导细胞损伤过程中同步进行力谱测量的方法。我们通过对附着在轴突膜上的光学捕获探针进行同步干涉测量来检测部分损伤轴突中的张力释放。我们的实验方案能以皮牛顿灵敏度检测张力释放,并以毫秒时间分辨率检测张力释放的动态过程。因此,它提供了一种高分辨率方法,用于研究细胞与底物之间的机械耦合如何通过药物处理和/或底物的不同机械特性进行调节。