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荧光磷脂酰丝氨酸插入红细胞质膜。被自体巨噬细胞识别。

Insertion of fluorescent phosphatidylserine into the plasma membrane of red blood cells. Recognition by autologous macrophages.

作者信息

Tanaka Y, Schroit A J

出版信息

J Biol Chem. 1983 Sep 25;258(18):11335-43.

PMID:6885820
Abstract

The interaction of macrophages with red blood cells (RBC) displaying phosphatidylserine (PS) in their surface membranes was investigated after the transfer of an exogenously supplied fluorescent lipid analog to the RBC. Nonfluorescent (quenched) lipid vesicles were formed by ultrasonication from 1-acyl-2-[(N-4-nitro-benzo-2-oxa-1,3 diazole)aminocaproyl]phosphatidyl-serine (NBD-PS) or 1-acyl-2[(N-4-nitrobenzo-2-oxa-1,3 diazole)aminocaproyl]phosphatidylcholine (NBD-PC). The interaction of these vesicles with RBC was monitored as a function of vesicle concentration by assessment of the degree to which cell-associated lipid fluorescence was dequenched after vesicle treatment. When vesicle concentrations of less than 100 ng/ml were used, lipid fluorescence was largely dequenched, indicating that lipid transfer was the predominant mechanism of both NBD-PS and NBD-PC uptake; however, when vesicle concentrations were increased to greater than 100 ng/ml, a concentration-dependent increase in the fraction of quenched cell-associated lipid was observed, indicating that another mechanism, possibly vesicle-cell adhesion, also occurred. Using NBD-PS at concentrations at which dilution of all the phospholipid analog in the recipient cell membrane could be unequivocally confirmed, we observed that the uptake of NBD-PS-treated RBC by macrophages was increased 5-fold over that of controls, whereas the uptake of RBC containing an equivalent amount of exogenously supplied NBD-PC was unaltered. Furthermore, preincubation of macrophage monolayers with vesicles containing PS resulted in a approximately 60% inhibition in the uptake of NBD-PS-treated RBC, whereas no inhibition in the uptake of control, opsonized, or NBD-PC-treated RBC was observed. These findings suggest that PS in the outer leaflet of RBC might serve as a signal for triggering their recognition by macrophages.

摘要

在将外源性供应的荧光脂质类似物转移至红细胞后,研究了巨噬细胞与表面膜上显示磷脂酰丝氨酸(PS)的红细胞(RBC)之间的相互作用。通过超声处理由1-酰基-2-[(N-4-硝基苯并-2-恶唑-1,3-二氮杂环戊二烯)氨基己酰基]磷脂酰丝氨酸(NBD-PS)或1-酰基-2-[(N-4-硝基苯并-2-恶唑-1,3-二氮杂环戊二烯)氨基己酰基]磷脂酰胆碱(NBD-PC)形成非荧光(淬灭)脂质囊泡。通过评估囊泡处理后细胞相关脂质荧光的去淬灭程度,监测这些囊泡与红细胞的相互作用随囊泡浓度的变化。当使用浓度低于100 ng/ml的囊泡时,脂质荧光大部分去淬灭,表明脂质转移是NBD-PS和NBD-PC摄取的主要机制;然而,当囊泡浓度增加到大于100 ng/ml时,观察到淬灭的细胞相关脂质比例呈浓度依赖性增加,表明还发生了另一种机制,可能是囊泡-细胞粘附。使用能明确确认受体细胞膜中所有磷脂类似物均被稀释的浓度的NBD-PS,我们观察到巨噬细胞对经NBD-PS处理的红细胞的摄取比对照组增加了5倍,而含有等量外源性供应的NBD-PC的红细胞的摄取未改变。此外,用含PS的囊泡对巨噬细胞单层进行预孵育,导致经NBD-PS处理的红细胞的摄取受到约60%的抑制,而未观察到对对照、调理或经NBD-PC处理的红细胞摄取的抑制。这些发现表明,红细胞外叶中的PS可能作为触发巨噬细胞识别它们的信号。

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