See
Genome Information for Burkholderia
To verify genes that are directly regulated by BysR, we used DNA affinity purification sequencing analysis (DAP-seq) for genome-wide recognition of BysR binding sites in vitro. The HALO-fusion BysR protein was successfully expressed and purified. After affinity purification and sequencing, at least 22 million double-end reads per sample were generated and with > 99 % of reads uniquely mapped to the JP2-270 genome. A total of 470 enriched common peaks of two replicates with –log10(P-value) ≥ 2 were called . The mean width of DAP-seq peaks was < 1,000. In total, 367 (78%) of these peaks were found to locate in the -1 kbp to 1 kbp regions by the analysis of peak summit positions relative to the start codons of JP2-270 open reading frames.
Overall design: Identification of the binding sites of BysR in vitro in the genom of Burkholderia sp. JP2-270.
| Accession | PRJNA798396; GEO: GSE193916 |
| Data Type | Epigenomics |
| Scope | Multiisolate |
| Organism | Burkholderia sp. JP2-270[Taxonomy ID: 2217913] Bacteria; Pseudomonadota; Betaproteobacteria; Burkholderiales; Burkholderiaceae; Burkholderia; Burkholderia sp. JP2-270 |
| Submission | Registration date: 18-Jan-2022
China national rice research institute |
| Relevance | Unknown |
Project Data:
| Resource Name | Number
of Links |
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| Sequence data |
| SRA Experiments | 3 |
| Other datasets |
| BioSample | 3 |
| GEO DataSets | 1 |