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亲脂性荧光探针三甲氨基二苯基己三烯的内化过程遵循细胞中质膜的内吞作用和再循环过程。

Internalization of the lipophilic fluorescent probe trimethylamino-diphenylhexatriene follows the endocytosis and recycling of the plasma membrane in cells.

作者信息

Illinger D, Poindron P, Fonteneau P, Modollel M, Kuhry J G

机构信息

Laboratorie de Biophysique, Unité Associée 491 au Céntre National de la Recherche Scientifique, Université Louis Pasteur Strasbourg, Faculté de Pharmacie, Illkirch, France.

出版信息

Biochim Biophys Acta. 1990 Nov 30;1030(1):73-81. doi: 10.1016/0005-2736(90)90240-o.

Abstract

The lipophilic fluorescent probe trimethylamino-diphenylhexatriene (TMA-DPH) has been shown previously to behave as a marker of plasma membrane in living cell systems, and it has therefore been widely used in membrane fluidity studies via fluorescence anisotropy measurements. However, progressive internalization of this probe in cells could lead to unsuitable interferences, when long incubations times were required. The mechanism of this internalization had not yet been elucidated. We present here fluorescence-intensity kinetic results and fluorescence micrographic data on L929 cells and on mouse bone-marrow macrophages, which allow us to identify the mechanism as fluid-phase pinocytosis: the probe remains associated with the plasma membrane throughout its internalization-recycling flow and it is finally concentrated in lysosomes. The study was facilitated by the partition equilibrium property of TMA-DPH between plasma membranes and the external aqueous medium, which allowed to immediately distinguish the internalized fraction of the probe from the peripheral labelling, by simply washing cells. This conclusion is confirmed by the features of the influence of temperature on TMA-DPH internalization.

摘要

亲脂性荧光探针三甲基氨基 - 二苯基己三烯(TMA - DPH)此前已被证明在活细胞系统中可作为质膜的标志物,因此它已通过荧光各向异性测量广泛应用于膜流动性研究。然而,当需要较长孵育时间时,该探针在细胞内的逐渐内化可能会导致不适当的干扰。这种内化的机制尚未阐明。我们在此展示了关于L929细胞和小鼠骨髓巨噬细胞的荧光强度动力学结果及荧光显微图像数据,这使我们能够将该机制确定为液相胞饮作用:探针在其内化 - 再循环过程中始终与质膜相关联,最终集中在溶酶体中。TMA - DPH在质膜和外部水相介质之间的分配平衡特性有助于该研究,通过简单洗涤细胞,就能立即将内化的探针部分与周边标记区分开来。温度对TMA - DPH内化影响的特征证实了这一结论。

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