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掺入巨型单层囊泡中的膜蛋白的分布、侧向流动性及功能

Distribution, lateral mobility and function of membrane proteins incorporated into giant unilamellar vesicles.

作者信息

Doeven Mark K, Folgering Joost H A, Krasnikov Victor, Geertsma Eric R, van den Bogaart Geert, Poolman Bert

机构信息

Department of Biochemistry, Groningen Biomolecular Sciences and Biotechnology Institute and Materials Science Centre, University of Groningen, Nijenborgh 4, 9747 AG Groningen, The Netherlands.

出版信息

Biophys J. 2005 Feb;88(2):1134-42. doi: 10.1529/biophysj.104.053413. Epub 2004 Dec 1.

Abstract

GUVs have been widely used for studies on lipid mobility, membrane dynamics and lipid domain (raft) formation, using single molecule techniques like fluorescence correlation spectroscopy. Reports on membrane protein dynamics in these types of model membranes are by far less advanced due to the difficulty of incorporating proteins into GUVs in a functional state. We have used sucrose to prevent four distinct membrane protein(s) (complexes) from inactivating during the dehydration step of the GUV-formation process. The amount of sucrose was optimized such that the proteins retained 100% biological activity, and many proteo-GUVs were obtained. Although GUVs could be formed by hydration of lipid mixtures composed of neutral and anionic lipids, an alternate current electric field was required for GUV formation from neutral lipids. Distribution, lateral mobility, and function of an ATP-binding cassette transport system, an ion-linked transporter, and a mechanosensitive channel in GUVs were determined by confocal imaging, fluorescence correlation spectroscopy, patch-clamp measurements, and biochemical techniques. In addition, we show that sucrose slows down the lateral mobility of fluorescent lipid analogs, possibly due to hydrogen-bonding with the lipid headgroups, leading to larger complexes with reduced mobility.

摘要

巨型单层囊泡(GUVs)已被广泛用于脂质流动性、膜动力学和脂质结构域(筏)形成的研究,采用了诸如荧光相关光谱等单分子技术。由于难以将处于功能状态的蛋白质整合到GUVs中,关于这些类型模型膜中膜蛋白动力学的报道目前还很有限。我们使用蔗糖来防止四种不同的膜蛋白(复合物)在GUV形成过程的脱水步骤中失活。蔗糖的用量经过优化,使得蛋白质保留100%的生物活性,并获得了许多蛋白质-GUVs。虽然GUVs可以通过由中性和阴离子脂质组成的脂质混合物水合形成,但从中性脂质形成GUVs需要交变电场。通过共聚焦成像、荧光相关光谱、膜片钳测量和生化技术确定了GUVs中ATP结合盒转运系统、离子连接转运体和机械敏感通道的分布、横向流动性和功能。此外,我们表明蔗糖会减缓荧光脂质类似物的横向流动性,这可能是由于与脂质头部基团形成氢键,导致形成更大的复合物且流动性降低。

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