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Manipulating freely diffusing single 20-nm particles in an Anti-Brownian Electrokinetic Trap (ABELtrap)

机译:在抗布朗电动陷阱(ABELtrap)中操纵自由扩散的20 nm单个粒子

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Conformational changes of individual fluorescently labeled proteins can be followed in solution using a confocal microscope. Two fluorophores attached to selected domains of the protein report fluctuating conformations. Based on Forster resonance energy transfer (FRET) between these fluorophores on a single protein, sequential distance changes between the dyes provide the real time trajectories of protein conformations. However, observation times are limited for freely diffusing biomolecules by Brownian motion through the confocal detection volume. A. E. Cohen and W. E. Moemer have invented and built microfluidic devices with 4 electrodes for an Anti-Brownian Electrokinetic Trap (ABELtrap). Here we present an ABELtrap based on a laser focus pattern generated by a pair of acousto-optical beam deflectors and controlled by a programmable FPGA chip. Fluorescent 20-nm beads in solution were used to mimic freely diffusing large proteins like solubilized F_0F_1-ATP synthase. The ABELtrap could hold these nanobeads for about 10 seconds at the given position. Thereby, observation times of a single particle were increased by a factor of 1000.
机译:可以使用共聚焦显微镜在溶液中追踪单个荧光标记蛋白的构象变化。附着在蛋白质选定结构域上的两个荧光团报告了波动的构象。基于单个蛋白质上这些荧光团之间的Forster共振能量转移(FRET),染料之间的顺序距离变化可提供蛋白质构象的实时轨迹。然而,通过布朗运动穿过共聚焦检测体积来自由扩散生物分子的观察时间受到限制。 A. E. Cohen和W. E. Moemer发明并制造了带有4个电极的微流体装置,用于抗布朗电动势阱(ABELtrap)。在这里,我们介绍一个基于激光聚焦图案的ABELtrap,该聚焦图案由一对声光光束偏转器产生,并由可编程FPGA芯片控制。溶液中的20 nm荧光珠用于模拟自由扩散的大蛋白,例如溶解的F_0F_1-ATP合酶。 ABELtrap可以将这些纳米珠在给定位置保持约10秒。因此,单个粒子的观察时间增加了1000倍。

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