High-throughput assay for determining specificity and affinity of protein-DNA binding interactions

被引:0
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作者
Outi Hallikas
Jussi Taipale
机构
[1] Molecular/Cancer Biology Program,and Department of Molecular Medicine
[2] Institute of Biomedicine,undefined
[3] University of Helsinki,undefined
[4] National Public Health Institute (KTL),undefined
[5] Biomedicum,undefined
[6] P.O. Box 63 (Haartmaninkatu 8),undefined
[7] FIN-00014 University of Helsinki,undefined
来源
Nature Protocols | 2006年 / 1卷
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摘要
Limited information exists for the binding specificities of many important transcription factors. To address this, we have previously developed a microwell-based assay for directly measuring the affinity of DNA-protein binding interactions. We describe here the detailed protocol for determining sequence specificities of DNA-binding proteins using this assay. The described method is rapid; after preparation of the reagents, the assay can be run in a single day, and its throughput can be increased further by automation. The method is quantitative but requires prior knowledge of one high-affinity binding site for the protein of interest. The protocol can be adapted for determining the effect of protein modifications and protein-protein interactions on DNA-binding specificity, and for engineering proteins with new DNA-binding specificities. In addition, the method is suitable for high-throughput screening to identify proteins or small molecules that modulate protein-DNA binding interactions.
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页码:215 / 222
页数:7
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