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Force dependency of biochemical reactions measured by single molecule force-clamp spectroscopy

机译:通过单分子力夹谱法测量生化反应的力依赖性

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摘要

Here we describe a protocol for using force-clamp spectroscopy to precisely quantify the effect of force on biochemical reactions. A calibrated force is used to control the exposure of reactive sites in a single polyprotein substrate composed of repeated domains. The use of polyproteins allows the identification of successful single-molecule recordings from unambiguous mechanical unfolding fingerprints. Biochemical reactions are then measured directly by detecting the length changes of the substrate held at a constant force. We present the layout of a force-clamp spectrometer along with protocols to design and conduct experiments. These experiments measure reaction kinetics as a function of applied force. We show sample data of the force dependency of two different reactions, protein unfolding and disulfide reduction. These data, which can be acquired in just a few days, reveal mechanistic details of the reactions that currently cannot be resolved by any other technique.
机译:在这里,我们描述了一种使用力钳光谱法精确量化力对生化反应的影响的协议。校准力用于控制由重复域组成的单个多蛋白底物中反应位点的暴露。使用多蛋白可以从明确的机械展开指纹中鉴定出成功的单分子记录。然后通过检测保持恒定力的底物的长度变化直接测量生化反应。我们介绍了力夹式光谱仪的布局以及设计和进行实验的协议。这些实验测量反应动力学与施加力的关系。我们显示了两个不同的反应,蛋白质展开和二硫化物还原的力依赖性的样本数据。这些可以在短短几天内获得的数据揭示了目前其他任何技术都无法解决的反应机理细节。

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