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Sample GSM7873382 Query DataSets for GSM7873382
Status Public on Jan 03, 2024
Title RSV visit, Comorbidity [A4398_472]
Sample type RNA
 
Source name whole blood
Organism Homo sapiens
Characteristics tissue: whole blood
gender / sex: Male
age in days: 200
age group: Above_six_months
visit: RSV visit
disease classification at rsv visit based on resvinet score: 2 - Mild
Extracted molecule total RNA
Extraction protocol The whole blood samples were collected in Paxgene tubes (PAXgene® Blood RNA Tube, BD) and stored at –80 °C until the processing. The RNA was extracted using QIAsymphony PAXgene Blood RNA Kit (QIAGEN) according to the manufacturer’s instructions. After the quality control, the RNA was further processed for Clariom™ GOScreen microarray (Thermo Fisher).
Label biotin
Label protocol First strand cDNA was synthesized with a combination of a Poly-dT and random primers containing a 5′-adaptor sequence. A 3’-adaptor was added to the single stranded cDNA followed by low-cycle PCR amplification. The cDNA was used as a template for in vitro transcription (IVT) that produces amplified amounts of antisense mRNA, (cRNA). The cRNA was then used as input for a second round of cDNA synthesis, producing double stranded cDNA.
 
Hybridization protocol After fragmentation, denaturation and end-labeling the targets are hybridized on the single GO Screen plate, according to manufacturer’s instructions (Thermo Fisher; GeneChip Pico Reagent Kit).
Scan protocol Single sample cartridge arrays were stained on a GeneChip Fluidics Station 450 and scanned on a GeneChip scanner 3000 7G while array plates were stained and imaged on the GeneTitan Multi-Channel Instrument.
Description Gene expression data of infants from RESCEU case-control cohort
Data processing Microarray data were preprocessed using R, Bioconductor package 40,41. Robust Multi-Array Average (RMA) function was used to normalize the raw data 42. Outliers were removed from the downstream data analysis based on visual guidance on principal component (PC) spectral map and sample clustering (Pearson correlation with complete linkage).
The clinical data necessary for batch correction (site of sample collection) is accessible by request only from the submitting party.
 
Submission date Oct 31, 2023
Last update date Jan 03, 2024
Contact name Deniz Oner
E-mail(s) deniz.oner@kuleuven.be
Organization name KU Leuven
Street address Gaston Geenslaan
City Leuven
ZIP/Postal code 3001
Country Belgium
 
Platform ID GPL31262
Series (1)
GSE246622 Single-cell immune profiling reveals markers of emergency myelopoiesis that distinguish severe from mild respiratory syncytial virus (RSV) disease in infants

Data table header descriptions
ID_REF
VALUE batch corrected

Data table
ID_REF VALUE
AFFX-BkGr-GC03_st 2.754912763
AFFX-BkGr-GC04_st 2.644543772
AFFX-BkGr-GC05_st 2.629135797
AFFX-BkGr-GC06_st 2.582843399
AFFX-BkGr-GC07_st 2.789950085
AFFX-BkGr-GC08_st 2.729824112
AFFX-BkGr-GC09_st 2.788803903
AFFX-BkGr-GC10_st 2.724529368
AFFX-BkGr-GC11_st 2.763757486
AFFX-BkGr-GC12_st 3.003814389
AFFX-BkGr-GC13_st 3.01818741
AFFX-BkGr-GC14_st 2.956377353
AFFX-BkGr-GC15_st 3.107408724
AFFX-BkGr-GC16_st 3.176260582
AFFX-BkGr-GC17_st 3.920242772
AFFX-BkGr-GC18_st 4.020252006
AFFX-BkGr-GC19_st 3.964947483
AFFX-BkGr-GC20_st 4.910526692
AFFX-BkGr-GC21_st 5.086867994
AFFX-BkGr-GC22_st 6.49805967

Total number of rows: 22593

Table truncated, full table size 673 Kbytes.




Supplementary file Size Download File type/resource
GSM7873382_A4398_472.CEL.gz 381.9 Kb (ftp)(http) CEL

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