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用于无干扰监测膜融合和膜间脂质转移的跨膜脂质

Membrane-spanning lipids for an uncompromised monitoring of membrane fusion and intermembrane lipid transfer.

作者信息

Schwarzmann Günter, Breiden Bernadette, Sandhoff Konrad

机构信息

Life & Medical Sciences (LIMES) Institute, Membrane Biology & Lipid Biochemistry Unit, Kekulé-Institut für Organische Chemie und Biochemie, Universität Bonn, D-53121 Bonn, Germany.

出版信息

J Lipid Res. 2015 Oct;56(10):1861-79. doi: 10.1194/jlr.M056929. Epub 2015 Aug 11.

Abstract

A Förster resonance energy transfer-based fusion and transfer assay was developed to study, in model membranes, protein-mediated membrane fusion and intermembrane lipid transfer of fluorescent sphingolipid analogs. For this assay, it became necessary to apply labeled reporter molecules that are resistant to spontaneous as well as protein-mediated intermembrane transfer. The novelty of this assay is the use of nonextractable fluorescent membrane-spanning bipolar lipids. Starting from the tetraether lipid caldarchaeol, we synthesized fluorescent analogs with fluorophores at both polar ends. In addition, we synthesized radioactive glycosylated caldarchaeols. These labeled lipids were shown to stretch through bilayer membranes rather than to loop within a single lipid layer of liposomes. More important, the membrane-spanning lipids (MSLs) in contrast to phosphoglycerides proved to be nonextractable by proteins. We could show that the GM2 activator protein (GM2AP) is promiscuous with respect to glycero- and sphingolipid transfer. Saposin (Sap) B also transferred sphingolipids albeit with kinetics different from GM2AP. In addition, we could unambiguously show that the recombinant activator protein Sap C x His6 induced membrane fusion rather than intermembrane lipid transfer. These findings showed that these novel MSLs, in contrast with fluorescent phosphoglycerolipids, are well suited for an uncompromised monitoring of membrane fusion and intermembrane lipid transfer.

摘要

我们开发了一种基于Förster共振能量转移的融合与转移分析方法,用于在模型膜中研究蛋白质介导的荧光鞘脂类似物的膜融合和膜间脂质转移。对于该分析方法,有必要应用对自发的以及蛋白质介导的膜间转移具有抗性的标记报告分子。该分析方法的新颖之处在于使用了不可提取的荧光跨膜双极脂质。从四醚脂质嗜热栖热菌醇出发,我们合成了在两个极性末端都带有荧光团的荧光类似物。此外,我们还合成了放射性糖基化嗜热栖热菌醇。这些标记脂质被证明能伸展穿过双层膜,而不是在脂质体的单个脂质层内成环。更重要的是,与磷酸甘油酯相比,跨膜脂质(MSL)被证明不能被蛋白质提取。我们可以证明,GM2激活蛋白(GM2AP)在甘油脂质和鞘脂转移方面具有混杂性。鞘磷脂激活蛋白(Sap)B也能转移鞘脂,尽管其动力学与GM2AP不同。此外,我们可以明确表明,重组激活蛋白Sap C x His6诱导的是膜融合而不是膜间脂质转移。这些发现表明,与荧光磷酸甘油脂质相比,这些新型MSL非常适合对膜融合和膜间脂质转移进行无干扰监测。

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