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平行微流控表面等离子体共振成像阵列。

Parallel microfluidic surface plasmon resonance imaging arrays.

机构信息

Michael Smith Laboratories, University of British Columbia, Vancouver, BC, Canada V6T 1Z4.

出版信息

Lab Chip. 2010 Mar 7;10(5):581-8. doi: 10.1039/b920589f. Epub 2010 Jan 6.

DOI:10.1039/b920589f
PMID:20162233
Abstract

Surface plasmon resonance imaging (SPRi) is a label-free technique used for the quantitation of binding affinities and concentrations for a wide variety of target molecules. Although SPRi is capable of determining binding constants for multiple ligands in parallel, current commercial instruments are limited to a single analyte stream on multiple ligand spots. Measurement of binding kinetics requires the serial introduction of different analyte concentrations; such repeated experiments are conducted manually and are therefore time-intensive. To address these challenges, we have developed an integrated microfluidic array using soft lithography techniques for high-throughput SPRi-based detection and determination of binding affinities of antibodies against protein targets. The device consists of 264 element-addressable chambers isolated by microvalves. The resulting 700 pL chamber volumes, combined with a serial dilution network for simultaneous interrogation of up to six different analyte concentrations, allow for further speeding detection times. To test for device performance, human alpha-thrombin was immobilized on the sensor surface and anti-human alpha-thrombin IgG was injected across the surface at different concentrations. The equilibrium dissociation constant was determined to be 5.0 +/- 1.9 nM, which agrees well with values reported in the literature. The interrogation of multiple ligands to multiple analytes in a single device was also investigated and samples were recovered with no cross-contamination. Since each chamber can be addressed independently, this array is capable of interrogating binding events from up to 264 different immobilized ligands against multiple analytes in a single experiment. The development of high-throughput protein analytic measurements is a critical technology for systems approaches to biology and medicine.

摘要

表面等离子体共振成像(SPRi)是一种无标记技术,用于定量分析各种靶分子的结合亲和力和浓度。尽管 SPRi 能够并行确定多种配体的结合常数,但当前的商业仪器仅限于在多个配体点上进行单一分析物流的测量。结合动力学的测量需要串行引入不同的分析物浓度;这种重复实验是手动进行的,因此非常耗时。为了解决这些挑战,我们使用软光刻技术开发了一种集成的微流控阵列,用于高通量基于 SPRi 的检测和测定针对蛋白质靶标的抗体的结合亲和力。该设备由 264 个可寻址元件的腔室组成,由微阀隔开。由此产生的 700pL 腔室体积,结合同时询问多达六种不同分析物浓度的串联稀释网络,进一步加快了检测速度。为了测试设备性能,将人凝血酶原α固定在传感器表面,并以不同浓度将抗人凝血酶原α IgG 注入表面。平衡解离常数确定为 5.0 +/- 1.9 nM,与文献报道的值吻合良好。还研究了在单个设备中对多种配体进行多种分析物的询问,并且没有发生交叉污染而回收了样品。由于每个腔室都可以独立寻址,因此该阵列能够在单个实验中针对多个分析物询问多达 264 种不同固定配体的结合事件。高通量蛋白质分析测量的开发是生物学和医学系统方法的关键技术。

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