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Sample GSM2464655 Query DataSets for GSM2464655
Status Public on Mar 06, 2017
Title Control CD1a+ replicate 3
Sample type SRA
 
Source name Control CD1a+
Organism Homo sapiens
Characteristics cell type: Cord blood CD34+ cells
transduced with: scrambled control shRNA lentivral vector containing a GFP reporter
cell populatione: CD45+GFP+CD7+CD1a+ T-cell precursors
experiment number: 3
Treatment protocol CD34+ enriched cord blood cells (enriched by magnetic activated cell sorting) were cultured for 16 hours in 100 microliters of transduction medium (X-Vivo 15 [Lonza, Walkersville, MD], thrombopoietin [50ng/ml], FLT3 ligand (50 ng/ ml], Stem cell factor [50 ng/ ml], and l-glutamine [2 mM, Cellgro, Manassas, VA]) on retronectin (50 ng/ ml, Clontech) coated non tissue culture treated 48 well plates (100,000 cells/ well). ShRNA Lentiviral supernatant (multiplicity of infection=10) along with additional transduction medium (to achieve a 1:1 volume ratio for supernatant and transduction medium) was then added. 125 microliters of transduction medium was added 24 hours after the dose of lentivirus. After 48 hours of exposure to lentivirus, CD34+GFP+lin(CD3, CD4, CD8,CD19)- cells were sorted for co-culture with OP9DLL1 stroma.
Growth protocol CD34+ cord blood (CB) cells were transduced with knockdown or scrambled control shRNA (multiplicity of Infection [MOI]=10) lentivirus. CD34+GFP+lin- CB cells were sorted (fluorescence activation cell sorting, FACS) and then co-cultured with OP9DLL1. The medium for OP9DLL1 co-cultures medium consisted of alpha-MEM (ThermoFisher), 20% fetal bovine serum (FBS, Hyclone, lot no. AXF42576), L-glutamine (2 mM, Cellgro, Manassas, VA), Pencillin-streptomycin (0.5X, CellGro), IL-7 (5 ng/ ml), and Flt3 ligand (5 ng/ml). On day 14 of co-culture, CD45+GFP+CD7+CD1a- and CD45+GFP+CD7+CD1a+ T-cell precursors were isolated from control and knockdown co-cultures by FACS and analyzed by RNA-Seq to determine the effect of BCL11B knockdown on the transcriptome of T-cell precursors.
Extracted molecule total RNA
Extraction protocol The Trizol method (Mirneasy RNA extraction mini kit, Qiagen, Valencia, CA) was used to extract total RNA from CD45+GFP+CD7+CD1a- and CD45+GFP+CD7+CD1a+ T-cell precursors isolated by FACS on day 14 of cord blood cells-OP9DLL1 co-cultures .
The Ovation Human FFPE RNA‑Seq System (NuGen) was used to convert 25 ng of total RNA from T-cell precursors into amplified cDNA libraries. The cDNA was sheared using a S220 focused ultrasonicator (Covaris, Woburn, MA) to generate an average fragment size of 300 base pairs. twenty cycles of PCR were used to ampify the libraries.
Libraries were sequenced on Illumina Nextseq500 (paired end 75 base pair sequencing)
 
Library strategy RNA-Seq
Library source transcriptomic
Library selection cDNA
Instrument model Illumina NextSeq 500
 
Description Sample 10
Data processing Read alignment: Tophat v2.0.14 was used to align paired end reads to the human transcriptome and genome (hg 19)
Estimation of gene level counts: HTseq v0.6.1p1, whole genome annotation file of protein coding and long non-coding RNA genes published in Casero et al, Nature Immunology 2015 (PMID: 26502406) was used for the Htseq analysis.
Differential expression analysis: DESeq2, experiment identifier (experiment number 1, 2 or 3) was used as a covariate
Genome_build: hg19
Supplementary_files_format_and_content: Raw counts for genes (HTseq output)
 
Submission date Jan 21, 2017
Last update date May 15, 2019
Contact name chintan parekh
E-mail(s) cparekh@chla.usc.edu
Organization name Children's Hospital Los Angeles
Department Pediatrics
Street address 4650 sunset blvd, mail stop 54
City Los Angeles
State/province California
ZIP/Postal code 90027
Country USA
 
Platform ID GPL18573
Series (2)
GSE84678 BCL11B
GSE93902 Effect of BCL11B knockdown on transcriptome of human T-cell precursors
Relations
BioSample SAMN06248726
SRA SRX2510067

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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