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SRX10185360: GSM5114318: [ChIP-seq] B. anthracis 34F2 AtxA-1xFLAG #2 enriched; Bacillus anthracis; ChIP-Seq
1 ILLUMINA (Illumina MiSeq) run: 2.5M spots, 256M bases, 84.9Mb downloads

Submitted by: NCBI (GEO)
Study: Direct regulons of the master virulence regulator AtxA of Bacillus anthracis
show Abstracthide Abstract
AtxA, the master virulence regulator of Bacillus anthracis, regulates the expression of three toxins that are required for the pathogenicity of Bacillus anthracis. Recent transcriptome analyses also showed that AtxA affects a large number of genes on both chromosome and plasmid, suggesting its role as a global regulator. Its mechanism of gene regulation nor binding target in vivo was, however, not well understood. In this work, we conducted ChIP-seq for cataloging binding sites of AtxA in vivo and Cappable-seq for catalogging the transcription start sites on the B. anthracis genome. For detected regulons, single knockout strains were constructed and RNA-seq was conducted for each strain. Overall design: ChIP-seq was conducted for genomic DNA of B. anthracis 34F2 WT and the strain that produce AtxA with 1xFLAG tag at its C-terminus. Cappable-seq was conducted for B. anthracis 34F2 WT and ?atxA. RNA-seq was conducted for B. anthracis 34F2 WT, ?atxA, ?xrrA, ?xrrB, and ?xrrC. All strains were grown in NBY medium supplemented with 8% NaHCO3 under 15% CO2 at 37°C.
Sample: [ChIP-seq] B. anthracis 34F2 AtxA-1xFLAG #2 enriched
SAMN18084044 • SRS8334216 • All experiments • All runs
Library:
Instrument: Illumina MiSeq
Strategy: ChIP-Seq
Source: GENOMIC
Selection: ChIP
Layout: SINGLE
Construction protocol: [ChIP-seq] Cells were pelleted and treated with 1% formaldehyde for for crosslinking. 250 mM glycine was added for quenching. After pelleting and resuspension in lysis buffer with cOmplete Mini Protease Inhibitor Cocktail, the samples were sonicated using Covaris S2. Supernatants were combined with Anti-FLAG M2 affinity gel for enrichment, followed by wash and protease K treatment at 65°C. [Cappable-seq] RNA was extracted using TRIzol after incubating the pellet with 2% SDS. After removing DNA with DNA-free DNA removal kit, RNA samples followed the protocol described before (Ettwiller et al, BMC Genomics 17:199, 2016) [3´-RACE] RNA was extracted using TRIzol after incubating the pellet with 2% SDS. DNA was removed with DNA-free DNA removal kit. [RNA-seq] RNA was extracted using TRIzol after incubating the pellet with 2% SDS. DNA was removed with DNA-free DNA removal kit. rRNA was depleted by the protocol described before (Culviner et al, mBio, 2020), followed by fragmentation with the treatment with a divalent cation and heat. [ChIP-seq] Library was constructed with NEBNext Ultra II DNA Library Prep Kit for Illumina. [Cappable-seq, 3´-RACE, and RNA-seq] Library was constructed with NEBNext Multiplex Small RNA Library Prep Set for Illumina.
Experiment attributes:
GEO Accession: GSM5114318
Links:
Runs: 1 run, 2.5M spots, 256M bases, 84.9Mb
Run# of Spots# of BasesSizePublished
SRR138016612,534,924256M84.9Mb2021-06-29

ID:
13312936

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