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Sample GSM747178 Query DataSets for GSM747178
Status Public on Jul 19, 2011
Title 2HR-C
Sample type RNA
 
Source name KH2 mES
Organism Mus musculus
Characteristics ra exposure: 2 hours
Treatment protocol Media was changed 3 hours before passaging them. Media was aspirated and washed twice with PBS. 2 ml of pre warmed Trypsin/EDTA solution were added and placed in incubator at 370 C for 1minute. During this period colonies float off when flicking the plate. Trypsin activity was stopped by adding 5ml of FCS-ES medium to flask. Colonies were dissociated into single cells by pipetting up and down for several times and pelleting the cells by centrifugation at 1000 rpm for 5 minutes. Media was aspirated and the cells were resuspended in appropriate volume of fresh ES cell medium and cells were seeded in 1:6. ratio into fresh T75 flask with feeders. Plate was tilted several times to distribute the cells evenly and placed in the incubator. Next day media was changed. Cells treated for 2, 4 and and 6 hours with RA were supplemented with differentiation media ( DMEM + 10% Serum + NAA+ 0.3uM RA) . After required period of induction, Media was aspirated and washed twice with PBS. 2 ml of pre warmed Trypsin/EDTA solution were added and placed in incubator at 370 C for 1minute. During this, period colonies float off when flicking the plate. Trypsin activity was stopped by adding 5ml of FCS-ES medium to flask. Colonies were dissociated into single cells by pipetting up and down for several times. Additional 15 ml of Differentiation media (without RA) was added and plated into freshly gelatinized plates. For gelatinized plates, Culture plates were treated half an hour before seeding with 0.1% Gelatin. Gelatin was later aspirated just before seeding of cells. After half an hour media was aspirated and centrifuged for 5 min at 1000 rpm. Pellets were dislodged by gentle tapping and 2 ml trizol were added. These tubes were stored at -80 until RNA isolation.
Growth protocol One day before of thawing, T25 plates with feeders were prepared. Aseptically the cell suspension was transferred into a sterile centrifuge tube containing several ml of warm FCS-ES media. Cells were pelleted by centrifuging at 1000 rpm for 5 minutes. Supernatant was aspirated and cells were resuspended into required quantity of fresh media. Cells were distributed evenly by tilting plates several times and then were placed in incubator (at 370 C and 5% CO2). Passage/expand of ES cells: Media was changed 3 hours before passaging them. Media was aspirated and washed twice with PBS. 800l of pre warmed Trypsin/EDTA solution were added and placed in incubator at 370 C for 1minute. During this period colonies float off when flicking the plate. Trypsin activity was stopped by adding 5ml of FCS-ES medium to flask. Colonies were dissociated into single cells by pipetting up and down for several times and pelleting the cells by centrifugation at 1000 rpm for 5 minutes. Media was aspirated and the cells were resuspended in appropriate volume of fresh ES cell medium and cells were seeded in 1:6 ratio into T75 flask. Plate was tilted several times to distribute the cells evenly and placed in the incubator.
Extracted molecule total RNA
Extraction protocol RNA for microarray analysis was isolated from ES cells grown on feeder cells. After induction, cells were washed in PBS, trypsinized, and replated onto a fresh gelatinized plate for 30 minutes. Media and unbound cells were aspirated. Adhered cells were resuspended in Trizol, aliquoted and flash frozen until needed. RNA were isolated as described per manufacture’s instruction and cleaned using RNAeasy Kit ( Quiagen). Quality and quantity of RNA were analyzed by Agilent Bioanlayzer 2100.
Label biotin
Label protocol Biotin labelling was done with 200 ng total RNA with the Ambion MessageAmp III kit.
 
Hybridization protocol Following fragmentation, 12.5 ug of aRNA were hybridized for 16 hr at 45C on Affymetrix Mouse Genome 430 2.0 array. GeneChips were washed and stained in the Affymetrix Fluidics Station 450.
Scan protocol Arrays were scanned with GeneChip 3000.
Data processing Affymetrix Mouse 430 v2 arrays were analyzed in R, version 2.11.1, using the packages affy (Gautier et al. 2004), version 1.26.1, and limma (Smyth et al., 2005), version 3.4.3. Normalization was done using rma.
 
Submission date Jun 23, 2011
Last update date Jul 19, 2011
Contact name Alexander (Garrett) Garruss
E-mail(s) asg@stowers.org
Organization name Stowers Institute for Medical Research
Lab Shilatifard
Street address 1000 East 50th Street
City Kansas CIty
State/province Missouri
ZIP/Postal code 64110
Country USA
 
Platform ID GPL1261
Series (2)
GSE30176 Retinoic acid (RA) induction time-course to profile gene expression during mES cell differentiation.
GSE30268 Dynamic transcriptional events in embryonic stem cells mediated by the super elongation complex (SEC).

Data table header descriptions
ID_REF
VALUE log2 RMA normalized signal

Data table
ID_REF VALUE
1415670_at 9.939683905
1415671_at 12.18935174
1415672_at 12.47808067
1415673_at 10.62681216
1415674_a_at 10.29275127
1415675_at 8.958890128
1415676_a_at 12.86019121
1415677_at 9.224824814
1415678_at 11.76013351
1415679_at 11.63013099
1415680_at 10.35668937
1415681_at 10.64905401
1415682_at 10.14825305
1415683_at 12.17798396
1415684_at 9.35824889
1415685_at 9.171401457
1415686_at 9.668450773
1415687_a_at 11.03858873
1415688_at 11.60009071
1415689_s_at 9.405707463

Total number of rows: 45101

Table truncated, full table size 1026 Kbytes.




Supplementary file Size Download File type/resource
GSM747178.CEL.gz 3.6 Mb (ftp)(http) CEL
Processed data included within Sample table

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