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使用全内反射荧光光谱法对质膜相关光敏剂进行选择性检测:原卟啉IX光漂白与光动力疗效之间的相关性

Selective examination of plasma membrane-associated photosensitizers using total internal reflection fluorescence spectroscopy: correlation between photobleaching and photodynamic efficacy of protoporphyrin IX.

作者信息

Strauss W S, Sailer R, Gschwend M H, Emmert H, Steiner R, Schneckenburger H

机构信息

Institut für Lasertechnologien in der Medizin und Messtechnik, Universität Ulm, Germany.

出版信息

Photochem Photobiol. 1998 Mar;67(3):363-9.

PMID:9523537
Abstract

Fluorescence spectra, fluorescence decay kinetics, photobleaching kinetics and photodynamic efficacy of protoporphyrin IX (PP) were investigated in endothelial cells in vitro after different incubation times. Fluorescence spectra and photobleaching kinetics were determined during total internal reflection (TIR) illumination or epi-illumination. Because penetration depth of the excitation light during TIR illumination was limited to about 100 nm, plasma membrane-associated PP was almost selectively examined. Spectra obtained by TIR fluorescence spectroscopy (FS) showed a very low background, whereas spectra obtained by epi-illumination exhibited considerable background by autofluorescence and scattered light. For photobleaching kinetics during TIR illumination after 1 h or 24 h incubation, a biexponential fluorescence decrease was observed with a rapidly and a slowly bleaching portion. After 1 h incubation, the rapidly bleaching portion was the predominant fraction, whereas after 24 h incubation comparable relative amounts of the rapidly and slowly bleaching portion were determined. The rapidly and slowly bleaching portion were assigned to PP monomers and aggregated species in close vicinity to the plasma membrane. Fluorescence decay measurements after epi-illumination support the decrease of PP monomers within the whole cell with increasing incubation time. In contrast to TIR illumination, photobleaching of PP during epi-illumination was characterized by slow monoexponential fluorescence decrease after 1 h or 24 h incubation. Photodynamic efficacy of PP using epi-illumination was found to depend strongly on incubation time. Considerable cell inactivation was determined for short incubation times (1 h or 3 h), whereas photodynamic efficacy was diminished for longer incubation times. Reduced photodynamic efficacy after long incubation times was assigned to the lower amount of photodynamically active monomers determined close to the plasma membrane as well as within the whole cell. In conclusion, TIRFS measurements are suggested to be an appropriate tool for the examination of the plasma membrane-associated photosensitizer fraction in living cells.

摘要

在体外对内皮细胞进行不同孵育时间后,研究了原卟啉IX(PP)的荧光光谱、荧光衰减动力学、光漂白动力学和光动力效应。在全内反射(TIR)照明或落射照明期间测定荧光光谱和光漂白动力学。由于TIR照明期间激发光的穿透深度限制在约100nm,因此几乎选择性地检测了与质膜相关的PP。通过TIR荧光光谱(FS)获得的光谱显示背景非常低,而通过落射照明获得的光谱由于自发荧光和散射光而呈现相当大的背景。对于孵育1小时或24小时后TIR照明期间的光漂白动力学,观察到双指数荧光下降,有快速和缓慢漂白部分。孵育1小时后,快速漂白部分是主要部分,而孵育24小时后,确定了快速和缓慢漂白部分的相对量相当。快速和缓慢漂白部分分别归因于质膜附近的PP单体和聚集物。落射照明后的荧光衰减测量支持随着孵育时间增加全细胞内PP单体的减少。与TIR照明相反,落射照明期间PP的光漂白特征是孵育1小时或24小时后单指数荧光缓慢下降。发现使用落射照明时PP的光动力效应强烈依赖于孵育时间。短孵育时间(1小时或3小时)时确定有相当程度的细胞失活,而较长孵育时间时光动力效应减弱。长时间孵育后光动力效应降低归因于在质膜附近以及全细胞内确定的光动力活性单体数量减少。总之,建议TIRFS测量是检查活细胞中与质膜相关的光敏剂部分的合适工具。

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