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Sample GSM7077985

Query DataSets for GSM7077985

Status

Public on Apr 20, 2024

Title

B6_Ly49An_ATAC_rep2

Sample type

SRA

Source name

Spleen

Organism

Mus musculus

Characteristics

strain: C57BL/6J
tissue: Spleen
cell line: primary cells
cell type: Natural killer cells
subset: Ly49A-
genotype: WT
treatment: ex vivo
marker: singlet CD4-CD8-TCRBeta-CD19-NK1.1+NKp46+CD49a-CD49b+

Treatment protocol

Splenic NK cells were FACS-sorted from mice or rats

Extracted molecule

genomic DNA

Extraction protocol

DNA was extracted according to a previously published protocol (Wu, J. et al. Requisite Chromatin Remodeling for Myeloid and Erythroid Lineage Differentiation from Erythromyeloid Progenitors. Cell Reports 33, 108395 (2020).)
libraries were constructed using a previously published protocol (Wu, J. et al. Requisite Chromatin Remodeling for Myeloid and Erythroid Lineage Differentiation from Erythromyeloid Progenitors. Cell Reports 33, 108395 (2020).)

Library strategy

ATAC-seq

Library source

genomic

Library selection

other

Instrument model

Illumina NextSeq 500

Description

singlet CD4-CD8-TCRβ-CD19-NK1.1+NKp46+CD49a-CD49b+

Data processing

Mouse ATAC data were first processed using the AIAP (v1.1) pipeline. As a part of the pipeline: locations of Tn5 insertion events were inferred from properly paired, non-PCR duplicate reads with MAPQ >= 10; each Tn5 insertion event was extended from insertion site up and down 75 bp to generate a 150 bp “pseudo read”; pseudo reads were piled up to generate an ATAC signal profile, which was normalized against sequencing depth. The resulting normalized ATAC signal profile was used in genome browser views unless otherwise noted.
For Ly49 consensus views of mouse and rat ATAC data, we fine-tuned the alignment using a custom alignment pipeline (https://github.com/ChangxuFan/snakeATAC/): adaptors were removed using cutadapt (v1.18) with parameters “--quality-cutoff=15,10 --minimum-length=36”; reads were aligned to reference genomes using “bowtie2 --very-sensitive --xeq --dovetail --no-unal”; only reads with perfect match to the reference were kept (“sambamba view -f bam -F '[AS] == 0'”). This was applied because we aligned ATAC data against genomes assembled from exactly the same mouse/rat strains; when indicated, reads were filtered based on MAPQ (“sambamba view -f bam -F 'mapping_quality >= 8 '”); “methylQA48 atac -X 38 -Q 1 ” was used to remove PCR duplicates, identify Tn5 insertion sites, and generate smoothed ATAC signals through extending Tn5 insertion sites up and downstream 75 bp, similar to the AIAP package.
Assembly: B6 reads were aligned to mm10. Rat reads were aligned to rn7. 129 and NOD reads were aligned to custom-built genomes, which were detailed in the “Ly49 and genome sequences and annotations” method section in the manuscript, and available at https://github.com/ChangxuFan/Ly49evolution
Supplementary files format and content: bigwig: AIAPnorm.bw files are the normalized ATAC signals from the AIAP pipeline. unnorm.bw is the unnormalized ATAC signals from the snakeATAC pipeline (this study). MAPQ8 indicates that reads were filtered for MAPQ >= 8.

Submission date

Mar 02, 2023

Last update date

Apr 20, 2024

Contact name

Changxu Fan

E-mail(s)

fanc@wustl.edu

Organization name

Washington University in St. Louis

Department

Genetics

Lab

Ting Wang Lab

Street address

4515 McKinley Avenue, Room 5213

City

Saint Louis

State/province

Missouri

ZIP/Postal code

63110

Country

USA

Platform ID

GPL19057

Series (2)

GSE226498	Epigenetic evolution of the Ly49 gene family [ATAC-Seq]
GSE226502	Epigenetic evolution of the Ly49 gene family

Relations

BioSample

SAMN33571830

SRA

SRX19551590

Supplementary file	Size	Download	File type/resource
GSM7077985_B6_Ly49An_ATAC_rep2_AIAPnorm.bw	227.4 Mb	(ftp)(http)	BW
SRA Run Selector
Raw data are available in SRA
Processed data provided as supplementary file