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Sample GSM3163391

Query DataSets for GSM3163391

Status

Public on Jun 11, 2019

Title

Macro-8

Sample type

SRA

Source name

Dermis

Organism

Mus musculus

Characteristics

strain: Cx3cr1+/gfp
tissue: ear skin
age: 7 weeks
cell type: Cx3cr1gfp/+ Dermis Macrophages

Treatment protocol

untreated

Growth protocol

SPF animal facility, no earclipping

Extracted molecule

total RNA

Extraction protocol

Mouse ears were digested with Dispase (0.25 U/ml), Collagenase II (1 mg/ml), and DNase I in HBSS with 10% FCS for 2 h at 1400 rpm and 37°C. Cells were filtered, stained and sorted as CD45+, CD11b+, CD64+, Lin- in a 384-well plate.
As described in CEL-Seq2 protocol (Hashimshony et al. 2016)
Adapted from TruSeq Small RNA Library Preparation Protocol

Library strategy

RNA-Seq

Library source

transcriptomic

Library selection

cDNA

Instrument model

Illumina HiSeq 3000

Description

library of 96 Cx3cr1gfp/+ Dermis Macrophages

Data processing

For image aquisition, intensity extraction and basecalling HiSeq Control Software 2.0.2, RTA 2.4.11 / Recipe Fragment 2.0.0.2(Hiseq2500) or Control Software HD 3.4.0.38 / RTA2.7.7 / Recipe Fragment HD 3.5.0.4(Hiseq3000) was used. Conversion of bcl2fastq files was performed using bcl2fastq 2.17.1.14
Paired end reads were aligned to the transcriptome using bwa (version 0.6.2-r126) with default parameters. The transcriptome contained all gene models based on the mouse ENCODE VM9 release downloaded from the UCSC genome browser comprising 57,207 isoforms derived from 57,207 gene loci with 57,114 isoforms mapping to fully annotated chromosomes (1 to 19, X, Y, M). All isoforms of the same gene were merged to a single gene locus. Furthermore, gene loci overlapping by >75% were merged to larger gene groups. In addition we annotated the EGFP sequence from the pEGFP-N1 vector (https://www.ncbi.nlm.nih.gov/nuccore/U55762) used to generate the CX3CR1-GFP reporter mice. This procedure resulted in 34,112 gene groups.
The right mate of each read pair was mapped to the ensemble of all gene loci and to the set of 92 ERCC spike-ins in sense direction. Reads mapping to multiple loci were discarded. The left read contains the barcode information: the first six bases correspond to the cell specific barcode followed by six bases representing the unique molecular identifier (UMI). The remainder of the left read contains a poly(T) stretch. The left read was not used for quantification. For each cell barcode, the number of UMIs per transcript was counted and aggregated across all transcripts derived from the same gene locus.
Based on binomial statistics, the number of observed UMIs was converted into transcript counts (Gruen et al., 2014).
Genome_build: ENCODE VM9 + gfp sequence from pEGFP-N1 vector (https://www.ncbi.nlm.nih.gov/nuccore/U55762)
Supplementary_files_format_and_content: TSV files, columns represent CXR3CR1 high/mid/low macrophages, rows represent the geneid and the values in the file are the quantified number of transcripts.

Submission date

May 29, 2018

Last update date

Jun 11, 2019

Contact name

Patrice Zeis

E-mail(s)

zeis@ie-freiburg.mpg.de

Organization name

Max Planck Institute of Immunobiology and Epigenetics

Lab

Dominic Grün

Street address

Stübeweg 51

City

Freiburg

ZIP/Postal code

79108

Country

Germany

Platform ID

GPL21493

Series (2)

GSE114526	Genome-wide expression study of macrophage subsets in mouse skin
GSE115030	A subset of skin macrophages modulates surveillance and regeneration of local nerves

Relations

BioSample

SAMN09275765

SRA

SRX4136238

Supplementary file	Size	Download	File type/resource
GSM3163391_Macro-8.coutt.tsv.gz	298.2 Kb	(ftp)(http)	TSV
GSM3163391_readme_Macro-8.coutt.tsv.gz	1.2 Kb	(ftp)(http)	TSV
SRA Run Selector
Raw data are available in SRA
Processed data provided as supplementary file
Processed data are available on Series record