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通过相位调制荧光光谱法分析激发态过程。

Analysis of excited-state processes by phase-modulation fluorescence spectroscopy.

作者信息

Lakowicz J R, Balter A

出版信息

Biophys Chem. 1982 Oct;16(2):117-32. doi: 10.1016/0301-4622(82)85013-8.

Abstract

Fluorescence phase shift and demodulation methods were used in the analysis of excited-state reactions and to investigate solvent relaxation around fluorophores in viscous solvents. The chosen samples illustrate the results expected for fluorophores bound to biological macromolecules. These moderately simple samples served to test the theoretical predictions described in the preceding paper (J.R. Lakowicz and A.B. Balter, Biophys. Chem. 16 (1982) 99.) and to illustrate the characteristic features of phase-modulation data expected from samples which display time-dependent spectral shifts. The excited-state protonation of acridine and exciplex formation between anthracene and diethylaniline provided examples of one-step reactions in which the lifetimes of the initially excited and the reacted species were independent of emission wavelength. Using these samples we demonstrated the following: (1) Wavelength-dependent phase shift and demodulation values can be used to prove the occurrence of an excited-state process. Proof is obtained by observation of phase angles (ø) larger than 90 degrees or by measurement of ratios of m/cos ø greater than 1, where m is the modulation of the emission relative to that of the excitation. (2) For a two-state process the individual emission spectra of each state can be calculated from the wavelength-dependent phase and modulation data. (3) The phase difference or demodulation factor between the initially excited and the reacted states reveals directly the fluorescence lifetime of the product of the reaction. (4) Phase-sensitive detection of fluorescence can be used to prove that the lifetimes of both the initially excited and the reacted states are independent of emission wavelength. (5) If steady-state spectra of the individual species are known, then phase-sensitive emission spectra can be used to measure the lifetimes of the individual components irrespective of the extent of spectral overlap. (6) Spectral regions of constant lifetime can be identified by the ratios of phase-sensitive emission spectra. In addition, we examined 6-propionyl-2-dimethylaminonaphthalene (PRODAN) and N-acetyl-L-tryptophanamide (NATA) in viscous solvents where the solvent relaxation times were comparable to the fluorescence lifetimes. Using PRODAN in n-butanol we used m/cos ø measurements, relative to the blue edge of the emission, to demonstrate that solvent relaxation requires more than a single step. For NATA in propylene glycol we used phase-sensitive detection of fluorescence to directly record the emission spectra of the initially excited and the solvent relaxed states. These measurements can be easily extended to fluorophores which are bound to proteins and membranes and are likely to be useful in studies of the dynamic properties of biopolymers.

摘要

荧光相移和解调方法用于激发态反应分析以及研究粘性溶剂中荧光团周围的溶剂弛豫。所选样品展示了与生物大分子结合的荧光团预期的结果。这些相对简单的样品用于检验前文(J.R. Lakowicz和A.B. Balter,《生物物理化学》16 (1982) 99)中描述的理论预测,并说明显示时间相关光谱位移的样品预期的相位调制数据的特征。吖啶的激发态质子化以及蒽与二乙苯胺之间激基复合物的形成提供了一步反应的例子,其中初始激发态和反应态的寿命与发射波长无关。使用这些样品我们证明了以下几点:(1) 波长相关的相移和解调值可用于证明激发态过程的发生。通过观察大于90度的相角 (ø) 或测量m/cos ø比值大于1来获得证明,其中m是发射相对于激发的调制。(2) 对于双态过程,每个态的单独发射光谱可根据波长相关的相位和调制数据计算得出。(3) 初始激发态和反应态之间的相位差或解调因子直接揭示反应产物的荧光寿命。(4) 荧光的相敏检测可用于证明初始激发态和反应态的寿命均与发射波长无关。(5) 如果已知各个物种的稳态光谱,那么相敏发射光谱可用于测量各个组分的寿命,而与光谱重叠程度无关。(6) 恒定寿命的光谱区域可通过相敏发射光谱的比值来识别。此外,我们在粘性溶剂中研究了6-丙酰基-2-二甲基氨基萘 (PRODAN) 和N-乙酰-L-色氨酸酰胺 (NATA),其中溶剂弛豫时间与荧光寿命相当。在正丁醇中使用PRODAN,我们通过相对于发射蓝边的m/cos ø测量,证明溶剂弛豫需要不止一步。对于丙二醇中的NATA,我们使用荧光的相敏检测直接记录初始激发态和溶剂弛豫态的发射光谱。这些测量可轻松扩展到与蛋白质和膜结合的荧光团,并且可能在生物聚合物动态性质的研究中有用。

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