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Sample GSM568924 Query DataSets for GSM568924
Status Public on Jul 20, 2011
Title 11 UT
Sample type RNA
 
Source name HUVEC, untreated, cultured in fully supplemented media
Organism Homo sapiens
Characteristics tissue: Primary endothelial cells
culture: Passage 4 cultured HUVECs
Treatment protocol Passage 4 cultured HUVEC isolates were untreated in fully supplemented media to maintain basal growth conditions.
Growth protocol HUVEC isolates from different individuals were cultured in fully supplemented media until passage 4 (P4).
Extracted molecule total RNA
Extraction protocol Cell cultures were washed with 1 x PBS and lysed using TRIzol® reagent. Total RNA was extracted using phenol chloroform, with the precipitated RNA washed in 70% ethanol and resuspended in RNase free water. RNA concentration and quality was assess by spectrophotometer and Agilent BioAnalyser.
Label Biotin
Label protocol Total RNA was converted to cDNA. This was then used in an invitro transcription (IVT) reaction with biotin to generate biotin incorporated cRNA.
 
Hybridization protocol 10 µg biotin incorporated cRNA was fragmented and then denatured. The denatured cRNA was slowly loaded into the bioarray flex chamber without the introduction of air bubbles. All samples were loaded within 30 minutes of cRNA denaturation. The sealed bioarrays were left to hybridise in a 37°C shaker-incubator for 18 hours. The slides were washed and placed in a solution of Cy5-streptavidin for 30 minutes, before stringent washes were used to remove any unbound dye.
Scan protocol All microarray slides were scanned using an Axon 4100B scanner at the following settings; 635mn wavelength, 600V PMT voltage, 100% laser power, 10µm pixel size
Description HUVEC Isolate 11 UT Biological replicate 12
Data processing The scanned Tagged Image File Format (TIFF) files were pre-processed using CodeLink Expression Analysis v4.0 software. Subsequent normalisation was carried out using Loess normalisation in R.
 
Submission date Jul 21, 2010
Last update date Jul 20, 2011
Contact name Muna Affara
E-mail(s) muna.affara@gmail.com
Organization name University of Cambridge
Department Pathology
Street address Tennis Court Road
City Cambridge
ZIP/Postal code CB2 1QP
Country United Kingdom
 
Platform ID GPL10716
Series (2)
GSE23068 Gene expression profiling of HUVEC under basal (resting) conditions
GSE23070 *MMP1* bimodal expression and differential response to inflammatory mediators is linked to promoter polymorphisms

Data table header descriptions
ID_REF
VALUE Loess normalised signal intensity

Data table
ID_REF VALUE
1453966.2_PROBE1 0.924
NM_032763.1_PROBE1 1.73
7472777CB1_PROBE1 0.124
1329470.331_PROBE1 3.17
NM_005608.1_PROBE1 1.27
NM_033439_PROBE1 10.3
AI826118_PROBE1 1.02
NM_021135.1_PROBE1 0.996
NM_003665.1_PROBE1 3.02
148412.2_PROBE1 4.4
L39833_PROBE1 24.9
NM_015362.1_PROBE1 22.5
NM_030807.1_PROBE1 674
NM_003787.1_PROBE1 7.08
997975.1_PROBE1 2.12
NM_003832.1_PROBE1 720
U63721_PROBE1 463
2291926CB1_PROBE1 2.24
1501918.5_PROBE1 0.49
AJ010230_PROBE1 1.78

Total number of rows: 14446

Table truncated, full table size 314 Kbytes.




Supplementary data files not provided
Processed data included within Sample table

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