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Sample GSM356608 Query DataSets for GSM356608
Status Public on May 11, 2009
Title Treg_culture_CD4+CD25+CD45RA+_rep1
Sample type RNA
 
Source name Treg expansion culture
Organism Homo sapiens
Characteristics Treg culture CD4+CD25+CD45RA+
Treatment protocol Treg and Tconv cell FACS sorting and expansion culture was performed as previously described by Hoffmann et al. 2004 (Blood. Aug 1;104(3):895-903). Cell-culture was performed according to Hoffmann et al. 2006 (Blood. Dec 15;108(13):4260-7).
Growth protocol Treg and Tconv cell isolation and expansion culture was performed as previously described by Hoffmann et al. 2004 (Blood. Aug 1;104(3):895-903). Cell-culture was performed according to Hoffmann et al. 2006 (Blood. Dec 15;108(13):4260-7).
Extracted molecule total RNA
Extraction protocol Total cellular RNA of the different cell types was isolated using the RNeasy Kit (Qiagen). RNA concentration was measured with a ND-1000 Spectrophotometer (NanoDrop, Thermo Fisher Scientific) and quality was controlled on agarose gels or using the Agilent Bioanalyzer.
Label Cy3
Label protocol Labeling and hybridization were performed using the Agilent Gene Expression system according to the manufacturer’s instructions. In brief, 200 ng to 1000 ng of high-quality RNA were amplified and Cyanine 3-CTP labeled with the One Color Low RNA Input Linear Amplification Kit (Agilent). Labeling efficiency was controlled using the NanoDrop spectrophotometer.
 
Hybridization protocol Samples were hybridized using a stringent protocol according to the manufacture's instruction. 1.65 µg labeled cRNA was supplemented with 11 µl Agilent 10x blocking agent, 2.2 µl Agilent 25x fragmentation buffer and nuclease-free water up to 55 µl final volumen. The sample was incubated at 60°C for 30 minutes, supplemented with 55 µl 2x hybridisation buffer and 100 µl of the mix was hybridisized for 16h at 65°C using an SureHyb chamber and an Agilent hybridization oven. Arrays were disassembled and washed for 1 minute in Agilent gene Expression (GE) wash buffer 1 followed by washing 1 minute in prewarmed (37°C) GE wash buffer 2.
Scan protocol Images were scanned immediately after washing using a DNA microarray scanner (Agilent) at 5 µm resolution.
Description gender: male
Data processing Data was processed using Feature Extraction Software (Agilent) and further analyzed using GeneSpring GX software version 7.
 
Submission date Dec 30, 2008
Last update date May 11, 2009
Contact name Christian Schmidl
E-mail(s) christian.schmidl@klinik.uni-regensburg.de
Organization name Rengensburg Center for Interventional Immunology
Lab Schmidl Lab
Street address Franz-Josef-Strauss-Allee 11
City Regensburg
ZIP/Postal code 93053
Country Germany
 
Platform ID GPL6480
Series (2)
GSE14232 Transcriptome analysis of freshly sorted and expanded regulatory and conventional T cells
GSE14281 Regulatory and conventional T-cells

Data table header descriptions
ID_REF
VALUE normalized log2 values: standard agilent feature extraction protocol 'GE1-v5_95_Feb07', polynomial datafit with a multiplicative detrendDegree of 4.

Data table
ID_REF VALUE
A_23_P100001 -1.1540701
A_23_P100011 0.031065097
A_23_P100022 0.31562155
A_23_P100056 0.16270526
A_23_P100074 0.077300474
A_23_P100092 0.0986493
A_23_P100103 0.7254808
A_23_P100111 0.31971055
A_23_P100127 1.6259028
A_23_P100133 1.0147558
A_23_P100141 1.004613
A_23_P100156 0.6083163
A_23_P100177 -0.17022036
A_23_P100189 -1.1474714
A_23_P100196 0.19383919
A_23_P100203 -0.11007527
A_23_P100220 -0.36074045
A_23_P100240 0.056333087
A_23_P10025 -5.6112537
A_23_P100263 -0.28973576

Total number of rows: 41046

Table truncated, full table size 957 Kbytes.




Supplementary file Size Download File type/resource
GSM356608.txt.gz 7.7 Mb (ftp)(http) TXT
Processed data included within Sample table

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