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蛋白质、膜和核酸动态特性的荧光光谱研究。

Fluorescence spectroscopic investigations of the dynamic properties of proteins, membranes and nucleic acids.

作者信息

Lakowicz J R

出版信息

J Biochem Biophys Methods. 1980 Jan-Feb;2(1):91-119. doi: 10.1016/0165-022x(80)90077-9.

Abstract

Fluorescence spectroscopy can reveal the dynamic properties of proteins, membranes and nucleic acids on the nanosecond timescale. Dynamic processes which can affect the fluorescence spectral characteristics of biopolymer-bound fluorophores include dipolar relaxation around excited state dipoles, rotational diffusion of fluorophores, and permeation of bipolymers of fluorescence quenchers. The occurrence of these processes is revealed by the time-dependence of the Stokes's shifts, the time dependence of fluorescence anisotropies and the quenching of fluorescence, respectively. We will describe each of these processes in detail using examples of data obtained for membrane-bound fluorophores. In addition, we will review the fluorescence spectral evidence for nanosecond structural fluctuations in proteins and nucleic acids. In total, fluorescence spectroscopy indicates that both proteins and membranes fluctuate rapidly on the nanosecond and subnanosecond timescale. In contrast, base pairs in double-helical DNA appear to be immobile on this timescale.

摘要

荧光光谱能够在纳秒时间尺度上揭示蛋白质、膜和核酸的动态特性。能够影响与生物聚合物结合的荧光团的荧光光谱特征的动态过程包括激发态偶极子周围的偶极弛豫、荧光团的旋转扩散以及荧光猝灭剂的双聚物渗透。这些过程的发生分别通过斯托克斯位移的时间依赖性、荧光各向异性的时间依赖性以及荧光猝灭来揭示。我们将使用膜结合荧光团获得的数据示例详细描述这些过程中的每一个。此外,我们将回顾蛋白质和核酸中纳秒级结构波动的荧光光谱证据。总体而言,荧光光谱表明蛋白质和膜在纳秒和亚纳秒时间尺度上都会快速波动。相比之下,双螺旋DNA中的碱基对在这个时间尺度上似乎是固定不动的。

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