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Sample GSM5357150 Query DataSets for GSM5357150
Status Public on Jun 05, 2021
Title 499
Sample type SRA
 
Source name PBMC
Organism Homo sapiens
Characteristics cell type: PBMC
plate: SSF-1784
plate_location: P4
pid: 2810
stimulation: csp
visit: M3
site: BAGAMOYO
age: old
vaccine: comparator
case: case
match: 14
sid: 3092190
date_m0: 2009-10-27
date_m3_5: 2010-02-05
time_to_malaria: 195
malaria_status: 1
waz: -0.84
haz: 0.24
hb: 9.4
Sex: F
age_weeks: 36
malaria_before_m3_5: 0
malaria_transmission: Low
Extracted molecule polyA RNA
Extraction protocol RNA was extracted at the Center for Infectious Disease Research (CIDR, Seattle) using the Promega SV 96 RNA Isolation kit following the manufacturer’s protocol. Samples kept in RNAprotect were centrifuged at 4,000g for 7 minutes at 4°C, cell pellets were resuspended in 150 μL RLT Buffer, and 150 μL of 70% ethanol was added prior to processing with Promega SV 96 RNA Isolation kit. RNAs were eluted with 100 μL nuclease free water. Each 96-well extraction batch was spot checked by Bioanalyzer using Agilent RNA 6000 Pico chip and had an average RIN score of 7.4. RNA samples were distributed in 384 well plates for library preparation. Samples from the same individuals were in the same plate and key study variables (vaccine, site and cases-controls) were checked for balance across plates to avoid batch effects.
An optimized version of Digital Gene Expression (DGE) was used, further reducing the reverse transcriptase reaction volume. In brief, poly(A)+ mRNA from antigen-stimulated PBMCs was linked to unique molecular identifiers (UMIs) using a template-switching reverse transcriptase. Then, cDNA from multiple cells were pooled, amplified, and prepped for multiplexed sequencing using a transposon-based fragmentation method, enriching for 3′ ends and preserving strand information. Nextera XT library preparation and sequence paired-ends were employed on an Illumina NextSeq instrument at the Broad Institute.
SCRB-Seq
 
Library strategy RNA-Seq
Library source transcriptomic
Library selection cDNA
Instrument model Illumina NextSeq 500
 
Data processing reads were aligned using BWA Aln version 0.7.10 using UCSC RefSeq (Human 19) with mitochondrial genes added
Quantified samples were then quality controlled using mapping summary statistics to remove low quality samples based on predetermined minimum values for the total number of mapped reads, percent of mapped reads mapped to the human genome, etc.
Downstream analysis was applied only to reads that mapped uniquely to a UMI and only mapped to isoforms of the same gene (UMI.unq).
The TMM normalization method was applied to account for differing number of read counts and to address unwanted technical variation. The voom transformation from the limma R package was applied to transform the data into a form appropriate for linear models.
Genome_build: hg19
Supplementary_files_format_and_content: concatenated_unique_refseq_umi_counts.tsv contains the count matrix for all samples/cells
 
Submission date Jun 04, 2021
Last update date Jun 06, 2021
Contact name Carlota Dobaño
Organization name ISGlobal, Hospital Clínic - Universitat de Barcelona
Street address Rosselló 153
City Barcelona
ZIP/Postal code 08036
Country Spain
 
Platform ID GPL18573
Series (1)
GSE176156 A baseline transcriptional signature associates with clinical malaria risk in RTS,S/AS01-vaccinated African children
Relations
BioSample SAMN19570537
SRA SRX11069595

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

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