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Sample GSM286408 Query DataSets for GSM286408
Status Public on Nov 21, 2008
Title Lung cells_24hrHypoxia_rep1
Sample type RNA
 
Source name Lung Microvascular endothelial cells,hypoxia,24hr
Organism Homo sapiens
Characteristics Primary cells
Treatment protocol At experiment start, medium was changed and dishes were transferred to the hypoxia chamber (Coy Labs, USA) and cultured in an atmosphere of 1% O2, 5% CO2 and 94% N2 for 3hr, 24hr or 48hrs. Control conditions were achieved by culture in 21% O2, 5% CO2 and 74% N2 in a cell-culture incubator.
Growth protocol Primary human microvascular endothelial cells from lung and cardiac tissue were grown on sterile tissue culture dishes in Endothelial Growth Medium (EGM-2MV; Code: CC-3202) according to the manufacturers instructions (Lonza Bioscience formerly Cambrex, UK).
Extracted molecule total RNA
Extraction protocol At experiment end, cell medium was removed, cells washed with PBS and thoroughly lysed in RLT buffer (RNeasy Mini kit, Qiagen, UK). Total RNA extraction, with on-the-column DNase treatment, was carried out using RNeasy Mini Kits (Qiagen Ltd, UK) according to the maunfacturer's instructions.
Label Biotin
Label protocol Total RNA (5ug) was reverse transcribed to cDNA (one-cycle cDNA synthesis kit), clean up of double stranded cDNA, biotin labelling of anti-sense cRNA (integrity checked on the Bioanalyzer 2100, Agilent technologies, USA) and clean up and fragmentation of biotinylated cRNA were all carried out according to the manufacturers protocol (Affymetrix, USA).
 
Hybridization protocol Fragmented cRNA (15ug) was hybridised to chips for 16 hrs at 45ÂșC in a hybridisation oven (AffyMetrix, USA) with rotation at 60rpm. Immediately following hybridisation, the array underwent automated washing and staining protocol on the automatic fluidics station 400, (AffyMetrix, USA).
Scan protocol Arrays were scanned on a GeneChip 3000 scanner (AffyMetrix, USA).
Description All cells used in these experiments were passage 6-7 and were routinely checked for mycoplasma contamination using the VenorGeM PCR kit (Cambio Ltd, UK.).
Data processing Affymetrix .cel files were imported and normalised using algorithms of GeneSpring 6.0 software i.e. data was normalised by applying the following data transformation criteria: a) measurements less than 0.01 were set to 0.01, b) per chip: normalised to 50th percentile and c) per gene: normalise to median. Genes that were absent in a majority of chips were eliminated from further analyses.
 
Submission date May 05, 2008
Last update date Nov 21, 2008
Contact name Christine Marie Costello
Phone 00353 01 7166738
Fax 00353 01 7166892
Organization name Conway Institute
Street address University College Dublin
City Dublin
ZIP/Postal code Dublin 4
Country Ireland
 
Platform ID GPL96
Series (1)
GSE11341 Lung selective gene responses to alveolar hypoxia

Data table header descriptions
ID_REF
VALUE Normalised value after per chip normalisation to 50th percentile, per gene normalisation to median and data transformation to set all measurements below 0.001 to 0.001
ABS_CALL

Data table
ID_REF VALUE ABS_CALL
1007_s_at 0.713 P
1053_at 0.510 P
117_at 1.000 A
121_at 1.137 P
1255_g_at 0.424 A
1294_at 1.080 P
1316_at 1.167 P
1320_at 1.168 A
1405_i_at 0.923 A
1431_at 1.394 M
1438_at 0.484 A
1487_at 1.245 P
1494_f_at 1.202 P
1598_g_at 1.243 P
160020_at 0.785 P
1729_at 1.196 P
1773_at 1.218 A
177_at 1.155 P
179_at 0.987 M
1861_at 1.134 P

Total number of rows: 22283

Table truncated, full table size 412 Kbytes.




Supplementary file Size Download File type/resource
GSM286408.CEL.gz 3.3 Mb (ftp)(http) CEL
Processed data included within Sample table

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