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部花青540对红细胞膜的光动力作用:脂质和蛋白质成分的结构扰动

Photodynamic action of merocyanine 540 on erythrocyte membranes: structural perturbation of lipid and protein constituents.

作者信息

Feix J B, Bachowski G J, Girotti A W

机构信息

Department of Radiology, Medical College of Wisconsin, Milwaukee 53226.

出版信息

Biochim Biophys Acta. 1991 Sep 2;1075(1):28-35. doi: 10.1016/0304-4165(91)90070-w.

Abstract

erocyanine 540 (MC540) is a membrane-directed photosensitizing dye with antileukemic and antiviral properties. In this study, biophysical and biochemical techniques have been used to examine MC540-sensitized photooxidative damage in the lipid and protein compartments of a test membrane, the human erythrocyte ghost. Irradiation of MC540-sensitized ghosts with white light resulted in oxidative damage to proteins, as manifested by (i) loss of sulfhydryl groups; (ii) intermolecular cross-linking of major polypeptides; and (iii) loss of Mg(2+)-ATPase and Na+,K(+)-ATPase activities. Photooxidation also produced a rapid and progressive increase in general protein motion, as measured by electron paramagnetic resonance spectrometry (EPR) with the sulfhydryl spin label MAL-6. In addition to these effects, ghosts exposed to MC540 and light underwent lipid peroxidation. EPR with two lipophilic spin probes, 5-doxylstearate and 16-doxylstearate, showed that lipid peroxidation is accompanied by a progressive decrease in bilayer fluidity (motional freedom). At a given dye concentration, structural perturbations of proteins were detected at much lower light fluences than those of lipids. When photoreactions were carried out in the presence of ascorbate and iron, there was a strong stimulation of lipid peroxidation (attributed to free radical chain reactions), with a concomitant greater decrease in lipid mobility. Thus, the deleterious effects of photoperoxidation on lipid structure and motional freedom were greatly exacerbated by ascorbate and iron. Membrane damage similar to that described here may play a role in the phototherapeutic activity of MC540.

摘要

部花青540(MC540)是一种具有抗白血病和抗病毒特性的膜导向光敏染料。在本研究中,已使用生物物理和生化技术来检测测试膜(人红细胞血影)的脂质和蛋白质组分中MC540敏化的光氧化损伤。用白光照射MC540敏化的血影导致蛋白质氧化损伤,表现为:(i)巯基损失;(ii)主要多肽的分子间交联;以及(iii)Mg(2 +)-ATP酶和Na +,K(+)-ATP酶活性丧失。光氧化还导致一般蛋白质运动迅速且逐渐增加,这通过使用巯基自旋标记MAL-6的电子顺磁共振光谱法(EPR)来测量。除了这些影响外,暴露于MC540和光的血影还发生脂质过氧化。使用两种亲脂性自旋探针5-硬脂酰氧基氮氧自由基和16-硬脂酰氧基氮氧自由基的EPR表明,脂质过氧化伴随着双层流动性(运动自由度)的逐渐降低。在给定的染料浓度下,检测到蛋白质的结构扰动所需的光通量比脂质的低得多。当在抗坏血酸和铁存在下进行光反应时,脂质过氧化受到强烈刺激(归因于自由基链反应),同时脂质流动性的降低更大。因此,抗坏血酸和铁极大地加剧了光过氧化对脂质结构和运动自由度的有害影响。本文所述的膜损伤可能在MC540的光治疗活性中起作用。

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