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Status |
Public on Aug 29, 2020 |
Title |
DNA mismatches reveal conformational penalties in protein-DNA recognition III |
Organism |
synthetic construct |
Experiment type |
Other
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Summary |
Transcription factors (TF) recognize specific genomic sequences to regulate complex gene expression programs. Although it is well established that TFs bind specific DNA sequences using a combination of base readout and shape recognition, some fundamental aspects of protein-DNA binding remain poorly understood. Many DNA-binding proteins induce changes in the DNA structure outside the intrinsic B-DNA envelope. However, how the energetic cost associated with distorting DNA contributes to recognition has proven difficult to study because the distorted DNA exists in low-abundance in the unbound ensemble. Here, we use a novel high-throughput assay called SaMBA (Saturation Mismatch-Binding Assay) to investigate the role of DNA conformational penalties in TF-DNA recognition. In SaMBA, mismatches are introduced to pre-induce DNA structural distortions much larger than those induced by changes in Watson-Crick sequence. Strikingly, approximately 10% of mismatches increased TF binding, and at least one mismatch was found that increased the binding affinity for each of 22 examined TFs. Mismatches also converted non-specific sites into high-affinity sites, and high-affinity sites into super-sites stronger than any known canonical binding site. Determination of high-resolution X-ray structures, combined with NMR measurements and structural analyses revealed that many of the mismatches that increase binding induce distortions similar to those induced by protein binding, thus pre-paying some of the energetic cost to deform the DNA. Our work indicates that conformational penalties are a major determinant of protein-DNA recognition, and reveals mechanisms by which mismatches can recruit TFs and thus modulate replication and repair activities in the cell.
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Overall design |
Saturation mismatch-binding assays (SaMBA) were performed for 22 eukaryotic transcription factors. Briefly, the SaMBA assays involved binding of tagged transcription factors to double-stranded Agilent microarrays in order to determine their binding specificity for putative DNA binding sites as well as sites containing all possible DNA mismatches (or mispairs). Each sequence of interest was represented on the array in 8-20 replicate spots. We report the signal intensity for each spot.
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Contributor(s) |
Gordan R |
Citation(s) |
33087930 |
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Submission date |
Aug 28, 2020 |
Last update date |
Nov 12, 2020 |
Contact name |
Raluca Gordan |
E-mail(s) |
raluca.gordan@duke.edu
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Organization name |
Duke University
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Department |
Center for Genomic and Computational Biology
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Street address |
101 Science Dr, CIEMAS 2179
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City |
Durham |
State/province |
NC |
ZIP/Postal code |
27708 |
Country |
USA |
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Platforms (1) |
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Samples (7)
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This SubSeries is part of SuperSeries: |
GSE156375 |
DNA mismatches reveal conformational penalties in protein-DNA recognition |
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Relations |
BioProject |
PRJNA660007 |