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使用n-(9-蒽氧基)脂肪酸荧光探针检测感染伯氏疟原虫的小鼠红细胞膜微粘度的变化。

Changes in the membrane microviscosity of mouse red blood cells infected with Plasmodium berghei detected using n-(9-anthroyloxy) fatty acid fluorescent probes.

作者信息

Howard R J, Sawyer W H

出版信息

Parasitology. 1980 Apr;80(2):331-42. doi: 10.1017/s0031182000000792.

Abstract

A set of n-(9-anthroyloxy) fatty acids (n = 2, 6, 9, 12, 16) have been used as fluorescent probes to examine the lipid environment at different depths in the outer membrane of normal mouse erythrocytes and red blood cells from Plasmodium berghei-infected blood. Fluorescent polarization experiments with normal mouse erythrocytes have demonstrated a typical gradient in microviscosity from the surface to the centre of the bilayer as a consequence of the motional properties of the C-atoms of the phospholipid acyl chains. The fluorescent probes rotate faster in the membrane of purified pluriparasitized cells (greater than 90% purity) than with the remaining fraction of red blood cells from infected blood (20--40% immature, infected red cells, and uninfected red cells), or normal mouse erythrocytes. This increase in fluidity with heavily infected cells occurs predominantly at the centre of the lipid bilayer, rather than at the membrane surface. A comparison of the polarization values of intact and lysed infected cells indicates that the fluorescent fatty acids preferentially label the plasma membrane rather than the internal membranes of infected cells. The results suggest that P. berghei infection causes a change in the composition and/or organization of the outer membrane of pluriparasitized cells which produces a decrease in membrane microviscosity.

摘要

一组n -(9 - 蒽氧基)脂肪酸(n = 2、6、9、12、16)已被用作荧光探针,以检测正常小鼠红细胞以及感染伯氏疟原虫血液中的红细胞外膜不同深度处的脂质环境。对正常小鼠红细胞进行的荧光偏振实验表明,由于磷脂酰链中碳原子的运动特性,双层膜从表面到中心的微粘度呈现出典型的梯度变化。荧光探针在纯化的多寄生虫感染细胞(纯度大于90%)的膜中的旋转速度比感染血液中剩余部分的红细胞(20 - 40%为未成熟、感染的红细胞以及未感染的红细胞)或正常小鼠红细胞中的旋转速度更快。重度感染细胞的这种流动性增加主要发生在脂质双层的中心,而非膜表面。对完整和裂解的感染细胞的偏振值进行比较表明,荧光脂肪酸优先标记感染细胞的质膜而非内膜。结果表明,伯氏疟原虫感染会导致多寄生虫感染细胞外膜的组成和/或组织结构发生变化,从而使膜微粘度降低。

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