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二维荧光寿命相关光谱扫描:从微秒到亚秒级 DNA 霍利迪连接点的构象动力学。

Scanning Two-Dimensional Fluorescence Lifetime Correlation Spectroscopy: Conformational Dynamics of DNA Holliday Junction from Microsecond to Subsecond.

机构信息

Molecular Spectroscopy Laboratory, RIKEN, 2-1 Hirosawa, Wako 351-0198, Japan.

Cellular Informatics Laboratory, RIKEN, 2-1 Hirosawa, Wako 351-0198, Japan.

出版信息

J Phys Chem Lett. 2022 Feb 10;13(5):1249-1257. doi: 10.1021/acs.jpclett.1c03787. Epub 2022 Jan 28.

Abstract

Single-molecule Förster resonance energy transfer (smFRET) is widely utilized to investigate the structural heterogeneity and dynamics of biomolecules. However, it has been difficult to simultaneously achieve a wide observation time window, a high structure resolution, and a high time resolution with the current smFRET methods. Herein, we introduce a new method utilizing two-dimensional fluorescence lifetime correlation spectroscopy (2D FLCS) and surface immobilization techniques. This method, scanning 2D FLCS, enables us to examine the structural heterogeneity and dynamics of immobilized biomolecules on a time scale from microsecond to subsecond by slowly scanning the sample stage at the rate of ∼1 μm/s. Application to the DNA Holliday junction (HJ) complex under various [Mg] conditions demonstrates that scanning 2D FLCS enables tracking reaction kinetics from 25 μs to 30 ms with a time resolution as high as 1 μs. Furthermore, the high structure resolution of scanning 2D FLCS allows us to unveil the ensemble nature of each isomer state and the heterogeneity of the dynamics of the HJ.

摘要

单分子Förster 共振能量转移 (smFRET) 被广泛用于研究生物分子的结构异质性和动力学。然而,当前的 smFRET 方法很难同时实现宽观测时间窗口、高结构分辨率和高时间分辨率。在此,我们介绍了一种利用二维荧光寿命相关光谱 (2D FLCS) 和表面固定化技术的新方法。这种方法,即扫描 2D FLCS,通过以约 1 μm/s 的速度缓慢扫描样品台,使我们能够在从微秒到亚秒的时间尺度上检查固定化生物分子的结构异质性和动力学。将其应用于各种 [Mg] 条件下的 DNA 霍利迪交叉 (HJ) 复合物,证明扫描 2D FLCS 能够以高达 1 μs 的时间分辨率跟踪从 25 μs 到 30 ms 的反应动力学。此外,扫描 2D FLCS 的高结构分辨率使我们能够揭示每个异构体状态的整体性质和 HJ 动力学的异质性。

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