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Sample GSM7689348 Query DataSets for GSM7689348
Status Public on Sep 20, 2023
Title LagPhase_Rep1_195min
Sample type SRA
 
Source name cells, 195 min after inoculation on soft-agar, rep.1
Organism Bacillus subtilis
Characteristics cell type: Bacteria
genotype: WT chromosome; comI_Q12L in natual plasmid
strain: NCIB3610
time after_inoculation_(min): 195
Treatment protocol Cells that started swarm expansion were collected into the lysis buffer by our custom sampling robot. Cells before swarm expansion (lag phase) were collected by being suspened in the lysis buffer.
Growth protocol Bacterial cells were spotted onto the center of a 9 cm petri dish filled with LB soft-agar (0.5% agar) medium and incubated at 30°C for swarm expansion.
Extracted molecule total RNA
Extraction protocol RNA was isolated by the hot phenol method (Jahn et al, J Microbiol Methods, 2008) with some modifications. Prepared RNA was DNase-digested and cleaned up using RNACleanXP. Depletion of ribosomal RNA was performed using DIY method (Culviner et al, mBio, 2020). Integrity of the prepared RNA was tested using a TapeStation.
Directional cDNA libraries were prepared using the NEBNext Ultra II Directional RNA Libary Prep Kit for Illumina (NEB, E7760) according to the manufacturers instructions. Quality of the prepared libraries was tested using a TapeStation.
 
Library strategy RNA-Seq
Library source transcriptomic
Library selection cDNA
Instrument model Illumina NovaSeq 6000
 
Data processing Sequencing of the cDNA libraries was performed by MPGC (Cologne, Germany) or D-BSSE genomics facilty (Basel, Switzerland)
Sequence reads were trimmed for adaptor sequence/short sequence (<35 nt) using Trimmomatic v0.39
Trimmed sequence reads were mapped to B. subtilis NCIB3610 genome and plasmid (NCBI Accession number: NZ_CP020102 and NZ_CP020103) using HISAT2 v2.2.1 in single-end mode.
Reads mapped to all cetegory of genes (CDS, ncRNA, tmRNA, signal recognition particle RNA, ribonuclease P RNA, tRNA, rRNA) were counted using featureCounts v2.0.1 with fractional counting for multi-mapping and multi-overlapping reads (-OM --fraction) in a strand-specific manner (-s 2). Of those, reads mapped in tRNA and rRNA were removed and the remaining reads were used for the downstream analysis.
All genes for which there were at least 2 samples with a read count of at least 10 were used for the downstream analysis. Samples with remaining reads of < 1 million reads were excluded and the rest of the samples were used for normalization using edgeR (version 3.6.1) and transformed (log2).
Supplementary files format and content: comma-separated files include mapped read count data for each sample
Supplementary files format and content: comma-separated files include edgeR-normalized log2 count data for each of the samples at expansion phase
Supplementary files format and content: comma-separated files include edgeR-normalized log2 count data for each of the samples at lag and expansion phase
 
Submission date Aug 07, 2023
Last update date Sep 20, 2023
Contact name Kazuki Nosho
Organization name University of Basel
Department Biozentrum
Street address Spitalstrasse 41
City Basel
ZIP/Postal code 4056
Country Switzerland
 
Platform ID GPL30886
Series (1)
GSE224332 Spatiotemporal trascriptomics of Bacillus subtilis swarming colony
Relations
BioSample SAMN36873066
SRA SRX21280838

Supplementary file Size Download File type/resource
GSM7689348_LagPhase_Rep1_195min_mappedReads.csv.gz 83.3 Kb (ftp)(http) CSV
GSM7689348_LagPhase_Rep1_195min_normalizedCounts2.csv.gz 99.5 Kb (ftp)(http) CSV
SRA Run SelectorHelp
Raw data are available in SRA
Processed data provided as supplementary file

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