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Sample GSM766369 Query DataSets for GSM766369
Status Public on Jul 26, 2011
Title ID3 Whole Blood 2
Sample type RNA
 
Source name WholeBlood
Organism Homo sapiens
Characteristics method: PAXgene
individual (indiv.id): ID3
visit: 2
ChIP: 3
yield: 2.3902
rin: 7.3
tissue: Whole Blood
Treatment protocol For each individual, five different post venipuncture methods were performed. B Lymphocytes from 10ml of blood were isolated by tubes with sodium citrate. LCLs were generated by EBV-mediated transformation and cells were grown for eight weeks.
Extracted molecule total RNA
Extraction protocol For the isolation of CD19 and CD20 B-cells, 40ml whole blood from EDTA tubes was collected and PBMCs were isolated by using a Ficoll-Paque™ gradient (Amersham). CD19 and CD20 B-cells were prepared by positive selection from the PBMCs by incubation with magnetic anti-CD19 or CD20 mAb-coated microbeads (MACS, Miltenyi Biotec). For the isolation of PBMCs from whole blood, BD Vacutainer® CPT Mononuclear Cell Preparation Tubes (Becton and Dickinson) were used. Total RNA was isolated from 5 ml of whole blood samples with the PAXGene Blood RNA system (Qiagen) and samples were left at room temperature for 24 hours before processing according to manufacturer’s instructions.Only two people at a time were sampled on any one day for logistical reasons. After blood draw standard protocols were followed for cell isolation, transformation or RNA extraction. With the exception of the PAXgene samples all RNA was isolated using TRI™ reagent (SIGMA) and resuspended in RNase free water.
Label biotin
Label protocol Manufacturer’s instructions
 
Hybridization protocol Arrays were hybridised with labelled cRNA material and scanned according to manufacturer’s instructions.
Scan protocol Manufacturer’s instructions
Description 1718911543_D
source name = post venipuncture method; Indiv.id = Individual Identifier; Visit: Visit number
Data processing The resultant data was parsed with the software package BeadStudio to produce raw intensity values for all probes. Signal was checked for quality using hybridisation and labelling controls internal to each array and subtracted for background within the statistical scripting environment, R v2.4.1. Signal was transformed and normalised using the variance stabilization algorithm as implemented in the vsn2 Bioconductor package.
 
Submission date Jul 25, 2011
Last update date Jul 26, 2011
Contact name Josine Min
E-mail(s) jlmin@well.ox.ac.uk
Organization name The Wellcome Trust Centre for Human Genetics
Street address Roosevelt Drive
City Oxford
ZIP/Postal code OX3 7BN
Country United Kingdom
 
Platform ID GPL7350
Series (1)
GSE30916 Variability of gene expression profiles in human blood and lymphoblastoid cell lines

Data table header descriptions
ID_REF
VALUE VSN normalized signal

Data table
ID_REF VALUE
ILMN_10000 5.826836463
ILMN_100000 1.093333629
ILMN_100007 3.189035564
ILMN_100009 1.298797564
ILMN_10001 7.600052562
ILMN_100010 5.180607719
ILMN_10002 0.465568112
ILMN_100028 7.288262554
ILMN_100030 0.922117514
ILMN_100031 2.507270528
ILMN_100034 -0.550833332
ILMN_100037 2.69194001
ILMN_10004 6.668539579
ILMN_10005 4.211576089
ILMN_100054 2.364069111
ILMN_100059 3.386521508
ILMN_10006 3.207759166
ILMN_100075 4.42166368
ILMN_100079 1.826275843
ILMN_100083 3.730474948

Total number of rows: 46713

Table truncated, full table size 1052 Kbytes.




Supplementary data files not provided
Processed data included within Sample table
Processed data are available on Series record

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