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可寻址拴系脂质双层阵列的微流体制备以及使用硅烷衍生化纳米玻璃基板的表面等离子体共振进行优化。

Microfluidic fabrication of addressable tethered lipid bilayer arrays and optimization using SPR with silane-derivatized nanoglassy substrates.

作者信息

Taylor Joseph D, Phillips K Scott, Cheng Quan

机构信息

Department of Chemistry, University of California, Riverside, CA 92521, USA.

出版信息

Lab Chip. 2007 Jul;7(7):927-30. doi: 10.1039/b618940g. Epub 2007 May 17.

Abstract

We report the microfluidic fabrication of robust and fluid tethered bilayer arrays within a poly(dimethylsiloxane) (PDMS) chip, and demonstrate its addressability and biosensing by incorporating the GM1 receptor into the bilayer framework for detection of cholera toxin. Rapid optimization of the experimental conditions is achieved by using nanoglassified surfaces in combination with surface plasmon resonance. The ultrathin glassy film on gold mimics glass surfaces employed in microfluidics, allowing real-time monitoring of multiple assembly steps and therefore permitting rapid prototyping of microfluidic arrays. The tethered bilayer array utilizes a covalently immobilized biotinylated protein for generation of well-defined capture zones where a streptavidin link is employed for the immobilization of biotinylated vesicles. Fusion of captured vesicles is accomplished using a concentrated PEG solution, and the lateral diffusion of the tethered bilayer membrane is characterized by fluorescence recovery after photobleaching methods. The tethered membrane arrays demonstrate marked stability and high mobility, which provide an ideal host environment for membrane-associated proteins and open new avenues for high-throughput analysis of these proteins.

摘要

我们报道了在聚二甲基硅氧烷(PDMS)芯片内通过微流控技术制造坚固且流体束缚的双层阵列,并通过将GM1受体整合到双层框架中以检测霍乱毒素来展示其可寻址性和生物传感能力。通过使用纳米分类表面与表面等离子体共振相结合,实现了实验条件的快速优化。金上的超薄玻璃膜模仿了微流控中使用的玻璃表面,允许实时监测多个组装步骤,从而实现微流控阵列的快速原型制作。束缚双层阵列利用共价固定的生物素化蛋白来生成明确的捕获区域,其中使用链霉亲和素来固定生物素化的囊泡。使用浓缩的聚乙二醇溶液完成捕获囊泡的融合,并通过光漂白后荧光恢复方法表征束缚双层膜的横向扩散。束缚膜阵列表现出显著的稳定性和高迁移率,为膜相关蛋白提供了理想的宿主环境,并为这些蛋白的高通量分析开辟了新途径。

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