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一种用于长达一周的蛋白质动力学研究的 HaloTag 锚定标尺。

A HaloTag Anchored Ruler for Week-Long Studies of Protein Dynamics.

机构信息

Department of Biological Sciences, Columbia University , 1212 Amsterdam Avenue, New York, New York 10027, United States.

出版信息

J Am Chem Soc. 2016 Aug 24;138(33):10546-53. doi: 10.1021/jacs.6b05429. Epub 2016 Aug 9.

DOI:10.1021/jacs.6b05429
PMID:27409974
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5510598/
Abstract

Under physiological conditions, protein oxidation and misfolding occur with very low probability and on long times scales. Single-molecule techniques provide the ability to distinguish between properly folded and damaged proteins that are otherwise masked in ensemble measurements. However, at physiological conditions these rare events occur with a time constant of several hours, inaccessible to current single-molecule approaches. Here we present a magnetic-tweezers-based technique that allows, for the first time, the study of folding of single proteins during week-long experiments. This technique combines HaloTag anchoring, sub-micrometer positioning of magnets, and an active correction of the focal drift. Using this technique and protein L as a molecular template, we generate a magnet law by correlating the distance between the magnet and the measuring paramagnetic bead with unfolding/folding steps. We demonstrate that, using this magnet law, we can accurately measure the dynamics of proteins over a wide range of forces, with minimal dispersion from bead to bead. We also show that the force calibration remains invariant over week-long experiments applied to the same single proteins. The approach demonstrated in this Article opens new, exciting ways to examine proteins on the "human" time scale and establishes magnetic tweezers as a valuable technique to study low-probability events that occur during protein folding under force.

摘要

在生理条件下,蛋白质氧化和错误折叠发生的概率非常低,且需要很长时间。单分子技术提供了一种区分正确折叠和受损蛋白质的能力,而这些在整体测量中是被掩盖的。然而,在生理条件下,这些罕见事件的时间常数为几个小时,目前的单分子方法无法达到。在这里,我们提出了一种基于磁镊的技术,该技术首次允许在长达一周的实验中研究单个蛋白质的折叠。该技术结合了 HaloTag 固定、亚微米级磁铁定位和对焦点漂移的主动校正。使用该技术和蛋白质 L 作为分子模板,我们通过关联磁铁和测量顺磁珠之间的距离与展开/折叠步骤生成了一个磁律。我们证明,使用这个磁律,我们可以在很宽的力范围内准确地测量蛋白质的动力学,并且从一个珠子到另一个珠子的分散性最小。我们还表明,在应用于相同单个蛋白质的长达一周的实验中,力校准保持不变。本文中展示的方法为在“人类”时间尺度上研究蛋白质开辟了新的、令人兴奋的途径,并确立了磁镊作为研究在力作用下发生的低概率蛋白质折叠事件的有价值技术。

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本文引用的文献

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Work Done by Titin Protein Folding Assists Muscle Contraction.肌联蛋白蛋白质折叠所做的功有助于肌肉收缩。
Cell Rep. 2016 Feb 16;14(6):1339-1347. doi: 10.1016/j.celrep.2016.01.025. Epub 2016 Feb 4.
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The elastic free energy of a tandem modular protein under force.受力作用下串联模块化蛋白质的弹性自由能。
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