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Single-molecule photon stamping FRET spectroscopy study of enzymatic conformational dynamics

机译:单分子光子冲压酶构象动力学的FRET光谱研究

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摘要

The fluorescence resonant energy transfer (FRET) from a donor to an acceptor via transition dipole–dipole interactions decreases the donor's fluorescent lifetime. The donor's fluorescent lifetime decreases as the FRET efficiency increases, following the equation: EFRET = 1 − τDA/τD, where τD and τDA are the donor fluorescence lifetime without FRET and with FRET. Accordingly, the FRET time trajectories associated with single-molecule conformational dynamics can be recorded by measuring the donor's lifetime fluctuations. In this article, we report our work on the use of a Cy3/Cy5-labeled enzyme, HPPK to demonstrate probing single-molecule conformational dynamics in an enzymatic reaction by measuring single-molecule FRET donor lifetime time trajectories. Compared with single-molecule fluorescence intensity-based FRET measurements, single-molecule lifetime-based FRET measurements are independent of fluorescence intensity. The latter has an advantage in terms of eliminating the analysis background noise from the acceptor fluorescence detection leak through noise, excitation light intensity noise, or light scattering noise due to local environmental factors, for example, in a AFM-tip correlated single-molecule FRET measurements. Furthermore, lifetime-based FRET also supports simultaneous single-molecule fluorescence anisotropy.
机译:通过过渡偶极-偶极相互作用,从供体到受体的荧光共振能量转移(FRET)会缩短供体的荧光寿命。随FRET效率的增加,供体的荧光寿命降低,其公式如下:EFRET = 1-τDA/τD,其中τD和τDA是无FRET和有FRET时的供体荧光寿命。因此,可以通过测量供体的寿命波动来记录与单分子构象动力学相关的FRET时间轨迹。在本文中,我们报告了我们使用Cy3 / Cy5标记的酶HPPK的工作,以通过测量单分子FRET供体的寿命时间轨迹来证明酶反应中的单分子构象动力学。与基于单分子荧光强度的FRET测量相比,基于单分子寿命的FRET测量与荧光强度无关。后者的优势在于消除了由于噪声,激发光强度噪声或由于局部环境因素引起的光散射噪声(例如在AFM尖端相关的单分子FRET中)引起的受体荧光检测泄漏的分析背景噪声测量。此外,基于寿命的FRET还支持同时的单分子荧光各向异性。

著录项

  • 期刊名称 other
  • 作者

    Yufan He; Maolin Lu; H. Peter Lu;

  • 作者单位
  • 年(卷),期 -1(15),3
  • 年度 -1
  • 页码 1039/c2cp42944f
  • 总页数 13
  • 原文格式 PDF
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