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High-Throughput Electrophoretic Mobility Shift Assays for Quantitative Analysis of Molecular Binding Reactions

机译:定量分析分子结合反应的高通量电泳迁移率分析

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We describe a platform for high-throughput electrophoretic mobility shift assays (EMSAs) for identification and characterization of molecular binding reactions. A photopatterned free-standing polyacrylamide gel array comprised of 8 mm-scale polyacrylamide gel strips acts as a chassis for 96 concurrent EMSAs. The high-throughput EMSAs was employed to assess binding of the Vc2 cyclic-di-GMP riboswitch to its ligand. In optimizing the riboswitch EMSAs on the free-standing polyacrylamide gel array, three design considerations were made: minimizing sample injection dispersion, mitigating evaporation from the open free-standing polyacrylamide gel structures during electrophoresis, and controlling unit-to-unit variation across the large-format free-standing polyacrylamide gel array. Optimized electrophoretic mobility shift conditions allowed for 10% difference in mobility shift baseline resolution within 3 min. The powerful 96-plex EMSAs increased the throughput to ~10 data/min, notably more efficient than either conventional slab EMSAs (~0.01 data/min) or even microchannel based microfluidic EMSAs (~0.3 data/min). The free-standing polyacrylamide gel EMSAs yielded reliable quantification of molecular binding and associated mobility shifts for a riboswitch-ligand interaction, thus demonstrating a screening assay platform suitable for riboswitches and potentially a wide range of RNA and other macromolecular targets.
机译:我们描述了用于鉴定和表征分子结合反应的高通量电泳迁移率变动分析(EMSA)的平台。由8毫米规模的聚丙烯酰胺凝胶条组成的光图案独立式聚丙烯酰胺凝胶阵列充当96个同时进行的EMSA的底盘。使用高通量EMSA评估Vc2环-di-GMP核糖开关与其配体的结合。在优化独立式聚丙烯酰胺凝胶阵列上的核糖开关EMSA时,进行了三个设计考虑:最小化样品进样分散,减轻电泳过程中开放式独立聚丙烯酰胺凝胶结构的蒸发以及控制整个单元之间的差异格式的独立式聚丙烯酰胺凝胶阵列。优化的电泳迁移率漂移条件允许在3分钟内迁移率漂移基线分辨率有10%的差异。强大的96重EMSA将吞吐率提高到〜10个数据/分钟,明显比常规平板EMSA(〜0.01数据/分钟)甚至基于微通道的微流EMSA(〜0.3数据/分钟)更高效。独立式聚丙烯酰胺凝胶EMSA可对核糖开关-配体相互作用进行分子结合和相关迁移率迁移的可靠定量,从而证明了适用于核糖开关以及潜在的广泛RNA和其他大分子靶标的筛选测定平台。

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