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Sample GSM7666370 Query DataSets for GSM7666370
Status Public on Feb 20, 2024
Title SA-3h, replicate 1, scRNA-seq
Sample type SRA
 
Source name bacterial cell
Organism Staphylococcus aureus
Characteristics strain: S. aureus 25923
cell type: bacterial cell
genotype: WT
treatment: exponential growth phase
Extracted molecule total RNA
Extraction protocol For RiboD-mSPLiT, all cells were from pure culture in vitro. Cells were harvested by centrifuge;
For RiboD-mSPLiT, library was performed accarding to the Materials and Methods section;
 
Library strategy RNA-Seq
Library source transcriptomic single cell
Library selection cDNA
Instrument model Illumina NovaSeq 6000
 
Description mSPLiT
0119-E
SA rRNA and mRNA reads.txt
Data processing The demultiplexing, barcodes processing, gene counting and aggregation of scRNA-seq data were made by scripts compiled in Python 2.7.15 as previously described with some modifications. [lattman, W. Jiang, P. Oikonomou, S. Tavazoie, Prokaryotic single-cell RNA sequencing by in situ combinatorial indexing. Nature microbiology 5, 1192 (Oct, 2020).]. Downstream analysis of single cell data was performed using pipelines detailed in Seurat v4.3.0.
For corralation analysis of bulk RNA-Seq and scRNA-seq data, scRNA-seq data was combined with the UMI sums of all cells. Single-cell and bulk transcriptomes of E.coli were compared by computing the Pearson correlation of log2 transcripts reads of each gene between the two measurements.
For scRNA-seq data mRNA / total RNA ratio analysis, we removed the barcodes sequence contained in the front, and the interference of the last ten bases, and kept only 20 bases for mapping. Then we mapped the data from the different species to the corresponding reference genomes.
(Detailed codes were saved in "Detailed Computational Pipeline.docx" and "scripts" compressed package .)
Assembly: E.coli MG1655 K12
Supplementary files format and content: matrix files
Supplementary files format and content: xlsx file include raw counts for RNA-seq and UMI sums of scRNA-seq data
Supplementary files format and content: tab-delimited files includes raw counts for samples of the same species
 
Submission date Jul 28, 2023
Last update date Feb 20, 2024
Contact name Xiaodan Yan
E-mail(s) 2019206500042@whu.edu.cn
Phone 13283874287
Organization name Wuhan University
Department Medical Research Institute
Street address Donghu Road, No. 115, Wuchang District,
City Wuhan
State/province Hubei Province
ZIP/Postal code 430071
Country China
 
Platform ID GPL27158
Series (2)
GSE239504 Bacterial single cell RNA-seq unveils cyclic-di-GMP as an antitoxin critical for antibiotic tolerance in biofilm [scRNA-seq]
GSE239505 Bacterial single cell RNA-seq unveils cyclic-di-GMP as an antitoxin critical for antibiotic tolerance in biofilm.
Relations
BioSample SAMN36737316
SRA SRX21179111

Supplementary data files not provided
SRA Run SelectorHelp
Raw data are available in SRA
Processed data are available on Series record

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