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Sample GSM25718 Query DataSets for GSM25718
Status Public on Jun 23, 2004
Title PDGF_24h_e
Sample type RNA
 
Channel 1
Source name starved fibroblasts (control 24h)
Organism Homo sapiens
Extracted molecule total RNA
 
Channel 2
Source name PDGF-treated fibroblasts (24h)
Organism Homo sapiens
Extracted molecule total RNA
 
 
Description Subconfluent AG01518 fibroblasts were starved for 16 hours in the presence of 0.1% BSA, and then stimulated for 1, 4, 10 or 24 hours with PDGF-BB (10 ng/ml in starvation medium), or left untreated for the same periods of time. Total RNA was isolated using the RNeasy kit (Qiagen). The RNA quality was checked by formaldehyde agarose gel electrophoresis (RNeasy protocol, Qiagen). Total RNA (40 mg) from cells treated for a given period of time with PDGF or starvation medium alone were labelled in reverse transcription reactions (Superscript II kit, Invitrogen) with dCTP-Cy5 and dCTP-Cy3, respectively (Amersham). In every second replicate experiment the fluorescent deoxynucleotides were swapped. Purified cDNA probes labelled with Cy3 and Cy5 were mixed per pair, and hybridized to cDNA microarray chips (hver1.2.1) from the Sanger Institute/LICR/CRUK Consortium (see http://www.sanger.ac.uk/Projects/Microarrays/
for details and hybridization protocols). For each time point, we performed at least four independent hybridizations, and used at least two different batches of RNA. Chips were scanned in a Perkin Elmer/GSI Lumonics ScanArray 4000 scanner and spot intensities were measured using the QuantArray software (histogram method with background subtraction). Normalization and statistical analysis of the quadruplicate data sets were performed using GeneSpring 5.0 analysis software (Silicon Genetics). A Lowess non-linear normalization was applied and the median of the ratio distribution for each array was set to 1. Regulated spots were selected based on the average ratio values above 1.750 for up-regulated genes and below 0.571 for down-regulated genes. In addition, we considered only genes that were significantly regulated (t-test, p<0.05) based on replicate hybridizations (global error model, GeneSpring). For all features selected using this protocol, the signal was significantly above the background, indicating that the expression of these genes was detectable. Finally, Hver1.2.1 microarrays contain replicate spots (1 to 6) corresponding to the same gene. Genes represented by spots that were not regulated in a similar manner were discarded. We show the average ratio of one representative spot for each regulated gene, with standard error calculated from multiple hybridizations and with the annotation provided by the microarray facility (Hver1.2.1_NCBI33).
Lot batch = 41
 
Submission date Jun 17, 2004
Last update date May 27, 2005
Contact name Jean-Baptiste Demoulin
Organization name Université catholique de Louvain
Department de Duve Institute
Lab UCL - MEXP
Street address av Hippocrate 75, B1.74.05
City Brussels
ZIP/Postal code B-1200
Country Belgium
 
Platform ID GPL506
Series (1)
GSE1484 PDGF stimulation kinetics

Data table header descriptions
ID_REF
VALUE log ratio (log2 of PRE_VALUE)
CH2_RAW raw signal - PDGF-treated cells
CH1_RAW raw signal - control cells
QUALITY 0 = low quality spot
PRE_VALUE normalized induction ratio by PDGF

Data table
ID_REF VALUE CH2_RAW CH1_RAW QUALITY PRE_VALUE
341137_A -0.4469733 319.4524 435.47018 1 0.73358035
127197_A -0.5042613 648.792 920.2443 1 0.70502144
810316_A 0.2761103 608.271 502.31912 1 1.2109253
327150_A -0.4903993 256.44678 360.26492 1 0.7118283
753587_A 0.4141493 406.36694 304.963 1 1.3325123
365930_A 0.2862223 2984.5552 2447.4753 1 1.2194424
282310_A 0.4786973 711.0742 510.285 0 1.3934845
364329_A 0.8460843 777.7738 432.6699 1 1.7976148
stSG89412 -0.3703203 371.08752 479.6824 1 0.7736109
stSG89417 -0.8619223 294.9972 536.14496 0 0.55021906
stSG89420 0.6611613 948.306 599.6794 1 1.5813551
stSG89488 0.8366143 866.6463 485.284 1 1.7858539
stSG89491 1.4101803 1776.4397 668.41144 0 2.6577039
stSG89493 0.4298753 1977.0287 1467.5995 1 1.3471173
stSG89495 1.4550093 954.9271 348.31226 1 2.7415836
30665_A -0.8831403 843.306 1555.3816 1 0.54218596
1571646_A 0.1543743 360.1709 323.62155 1 1.1129385
486118_A -0.3630583 313.2108 402.83582 1 0.77751476
24032_A 0.4010653 461.60294 349.57138 1 1.3204827
43181_A 0.1852563 435.41458 382.94418 0 1.1370184

Total number of rows: 9928

Table truncated, full table size 492 Kbytes.




Supplementary data files not provided

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