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用于超灵敏生化研究的电子自旋共振扫描探针光谱学。

Electron spin resonance scanning probe spectroscopy for ultrasensitive biochemical studies.

作者信息

Campbell Jason P, Ryan Jason T, Shrestha Pragya R, Liu Zhanglong, Vaz Canute, Kim Ji-Hong, Georgiou Vasileia, Cheung Kin P

机构信息

†National Institute of Standards and Technology, 100 Bureau Drive, MS 8120, Gaithersburg, Maryland 20899, United States.

§Department of Electrical and Computer Engineering, George Mason University, 4400 University Drive, Fairfax, Virginia 22030, United States.

出版信息

Anal Chem. 2015;87(9):4910-6. doi: 10.1021/acs.analchem.5b00487. Epub 2015 Apr 22.

DOI:10.1021/acs.analchem.5b00487
PMID:25867553
Abstract

Electron spin resonance (ESR) spectroscopy's affinity for detecting paramagnetic free radicals, or spins, has been increasingly employed to examine a large variety of biochemical interactions. Such paramagnetic species are broadly found in nature and can be intrinsic (defects in solid-state materials systems, electron/hole pairs, stable radicals in proteins) or, more often, purposefully introduced into the material of interest (doping/attachment of paramagnetic spin labels to biomolecules of interest). Using ESR to trace the reactionary path of paramagnetic spins or spin-active proxy molecules provides detailed information about the reaction's transient species and the label's local environment. For many biochemical systems, like those involving membrane proteins, synthesizing the necessary quantity of spin-labeled biomolecules (typically 50 pmol to 100 pmol) is quite challenging and often limits the possible biochemical reactions available for investigation. Quite simply, ESR is too insensitive. Here, we demonstrate an innovative approach that greatly enhances ESR's sensitivity (>20000× improvement) by developing a near-field, nonresonant, X-band ESR spectrometric method. Sensitivity improvement is confirmed via measurement of 140 amol of the most common nitroxide spin label in a ≈593 fL liquid cell at ambient temperature and pressure. This experimental approach eliminates many of the typical ESR sample restrictions imposed by conventional resonator-based ESR detection and renders the technique feasible for spatially resolved measurements on a wider variety of biochemical samples. Thus, our approach broadens the pool of possible biochemical and structural biology studies, as well as greatly enhances the analytical power of existing ESR applications.

摘要

电子自旋共振(ESR)光谱对检测顺磁性自由基或自旋的亲和力,已越来越多地用于研究各种生化相互作用。这类顺磁性物质在自然界广泛存在,可以是固有的(固态材料系统中的缺陷、电子/空穴对、蛋白质中的稳定自由基),或者更常见的是,有意引入到感兴趣的材料中(将顺磁性自旋标记物掺杂/附着到感兴趣的生物分子上)。利用ESR追踪顺磁性自旋或自旋活性替代分子的反应路径,可提供有关反应瞬态物种和标记物局部环境的详细信息。对于许多生化系统,如涉及膜蛋白的系统,合成所需数量的自旋标记生物分子(通常为50皮摩尔至100皮摩尔)极具挑战性,且常常限制了可供研究的可能生化反应。简而言之,ESR灵敏度太低。在此,我们展示了一种创新方法,通过开发一种近场、非共振、X波段ESR光谱测定方法,极大地提高了ESR的灵敏度(提高了>20000倍)。通过在环境温度和压力下,在一个约593飞升液体池中测量140阿托摩尔最常见的氮氧化物自旋标记物,证实了灵敏度的提高。这种实验方法消除了传统基于谐振器的ESR检测所施加的许多典型ESR样品限制,并使该技术可用于对更广泛的生化样品进行空间分辨测量。因此,我们的方法拓宽了可能的生化和结构生物学研究范围,并极大地增强了现有ESR应用的分析能力。

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