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用宏观显微镜对大量支撑脂质双层进行成像。

Imaging large arrays of supported lipid bilayers with a macroscope.

机构信息

Department of Chemistry, Texas A&M University, College Station, Texas 77843, USA.

出版信息

Biointerphases. 2007 Jun;2(2):57-63. doi: 10.1116/1.2732312.

DOI:10.1116/1.2732312
PMID:20408637
Abstract

Herein, the authors present fluorescence resonance energy transfer (FRET) and two-dimensional protein saturation data acquired from spatially addressed arrays of solid supported lipid bilayers (SLBs). The SLB arrays were imaged with an epifluorescencetotal internal reflection macroscope. The macroscope allowed 1x imaging and had a relatively high numerical aperture (0.4). Such powerful light gathering and large field of view capabilities make it possible to simultaneously image dozens of addressed SLBs. Three experiments have been performed. First, a 9x7 array of supported lipid bilayer was fabricated and imaged in which each bilayer element was individually addressed. Second, a FRET assay was developed between Texas Red-DHPE (1,2-dihexadecanoyl-sn-glycero-3-phosphoethanolamine) and NBD-PE (1,2-dipalmitoyl-sn-glycero-3-phosphoethanolamine-n-(7-nitro-2-1,3-benzoxadiazol-4-yl)). The concentration of dye could be varied at each address and the value of the Forster radius (7.3+/-0.6 nm) was easily abstracted. Third, a ligandreceptor recognition assay was designed to show the two-dimensional number density of proteins which can be bound at saturation. It was found for the streptavidinbiotin pair that the protein saturated at the interface above 3 mol % biotin concentration. This corresponded to a two-dimensional footprint of 40 nm(2) for the streptavidin molecule. These results clearly open the door to using individually addressed bilayers for obtaining large amounts of biophysical data at the supported bilayeraqueous interface. Such abilities will be crucial to obtaining sufficient data for determining the interfacial mechanisms for a variety of membraneprotein interactions.

摘要

本文介绍了从空间寻址的固体支撑脂双层(SLB)阵列获得的荧光共振能量转移(FRET)和二维蛋白质饱和数据。SLB 阵列使用明场荧光全内反射显微镜进行成像。该显微镜允许 1x 成像,并且具有相对较高的数值孔径(0.4)。如此强大的聚光能力和大视野使同时对数十个寻址的 SLB 进行成像成为可能。进行了三个实验。首先,制造并成像了 9x7 个支持脂双层的阵列,其中每个双层元件都可以单独寻址。其次,开发了 Texas Red-DHPE(1,2-二硬脂酰-sn-甘油-3-磷酸乙醇胺)和 NBD-PE(1,2-二棕榈酰-sn-甘油-3-磷酸乙醇胺-n-(7-硝基-2-1,3-苯并恶唑-4-基))之间的 FRET 测定法。可以在每个地址处改变染料的浓度,并且很容易提取出Förster 半径(7.3+/-0.6nm)的值。第三,设计了配体-受体识别测定法,以显示可以在饱和时结合在二维界面上的蛋白质的二维数密度。对于链霉亲和素-生物素对,发现蛋白质在界面上的浓度超过 3 mol%生物素浓度时达到饱和。这对应于链霉亲和素分子的二维足迹为 40nm(2)。这些结果清楚地为使用单独寻址的双层在支持双层-水界面获得大量生物物理数据开辟了道路。这些能力对于获得足够的数据以确定各种膜蛋白相互作用的界面机制将至关重要。

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