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Bar-coded hydrogel microparticles for protein detection: Synthesis, assay and scanning

机译:用于蛋白质检测的条形码水凝胶微粒:合成,分析和扫描

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This protocol describes the core methodology for the fabrication of bar-coded hydrogel microparticles, the capture and labeling of protein targets and the rapid microfluidic scanning of particles for multiplexed detection. Multifunctional hydrogel particles made from poly(ethylene glycol) serve as a sensitive, nonfouling and bio-inert suspension array for the multiplexed measurement of proteins. Eeach particle type bears a distinctive graphical code consisting of unpolymerized holes in the wafer structure of the microparticle; this code serves to identify the antibody probe covalently incorporated throughout a separate probe region of the particle. Tthe protocol for protein detection can be separated into three steps: (i) synthesis of particles via microfluidic flow lithography at a rate of 16,000 particles per hour; (ii) a 3-4-h assay in which protein targets are captured and labeled within particles using an antibody sandwich technique; and (iii) a flow scanning procedure to detect bar codes and quantify corresponding targets at rates of 25 particles per s. By using the techniques described, single-or multiple-probe particles can be reproducibly synthesized and used in customizable multiplexed panels to measure protein targets over a three-log range and at concentrations as low as 1 pg ml~(-1).
机译:该协议描述了制造条形码水凝胶微粒,捕获和标记蛋白质靶标以及对微粒进行快速微流扫描以进行多重检测的核心方法。由聚乙二醇制成的多功能水凝胶颗粒可作为灵敏,无污染和生物惰性的悬浮液阵列,用于蛋白质的多重测量。每种颗粒类型都有一个独特的图形代码,该代码由微粒的晶片结构中未聚合的孔组成;该代码用于鉴定共价掺入整个颗粒的单独探针区域中的抗体探针。用于蛋白质检测的方案可分为三个步骤:(i)通过微流体流式光刻以每小时16,000个颗粒的速率合成颗粒; (ii)3-4-h分析,其中使用抗体夹心技术捕获蛋白质靶标并在颗粒内进行标记; (iii)流扫描程序,以每秒25个粒子的速度检测条形码并量化相应的目标。通过使用所描述的技术,可重复合成单探针或多探针颗粒,并将其用于可定制的多重面板中,以测量三对数范围内且浓度低至1 pg ml〜(-1)的蛋白质靶标。

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