NCBI Logo
GEO Logo
   NCBI > GEO > Accession DisplayHelp Not logged in | LoginHelp
GEO help: Mouse over screen elements for information.
          Go
Sample GSM881310 Query DataSets for GSM881310
Status Public on Feb 28, 2013
Title Red_13433525_S01_FlippedLLtoURr
Sample type RNA
 
Channel 1
Source name SiControl, 16h
Organism Homo sapiens
Characteristics cell line: HCT116
cell type: colorectal carcinoma cells
genotype: control
time point: 16h
Treatment protocol See Cepeda et al. The ubiquitin ligase SCFFBXO28 regulates Myc-driven transcription through non-proteolytic ubiquitylation and is required for cell proliferation.
Growth protocol See Cepeda et al. The ubiquitin ligase SCFFBXO28 regulates Myc-driven transcription through non-proteolytic ubiquitylation and is required for cell proliferation.
Extracted molecule total RNA
Extraction protocol Total RNA was extracted using TRIzol reagent (Invitrogen) according to the manufacturer’s instructions.
Label Cy3
Label protocol RNA priming: To 20 ug total RNA, add 10 ug 20(T)VN primer (MWG Biotech AG), adjust total volume to 18.4 µl, 70C 10 min , ice > 2 min, Prepare 1x RT-mixture (all reagents from Invitrogen): 5x RT-buff 6 µl, 50x aa-dNTP* 0.6 µl, DTT (0.1M) 3 µl, SuperScript II (200 U/µl) 2 µl.
cDNA synthesis: To primed RNA, add 11.6 µl RT-mix, add 42C 1 h 45 min.
RNA degradation: Add 3 µl 200 mM EDTA, add 4.5 µl 1 M NaOH, 70 C 15 min.
Neutralisation: Add 3 µl 1 M HCl.
Cleanup 1: Add 70 µl H20 + 500 µl PB, transfer to MinElute column (Qiagen), 13000 rpm 60 s, reapply flow-though, 13000 rpm 1 min, discard flow-through, add 600 µl 80% EtOH, 13000 rpm 60 s, repeat EtOH wash, spin column dry, 13000 rpm 60 s, transfer column to new microtube, add 10 µl 0.1 M NaCO3 pH 9.0, incubate 2 min, 13000 rpm 60 s, add 10 µl 0.1 M NaCO3 pH 9.0, 13000 rpm 60 s, transfer elution to aliquot of Cy3-dye (Amersham)**, mix with pipette, briefly centrifuge, incubate 1.5 h in dark at room temperature, add 4.5 µl 1 M hydroxylamine Cleanup 2 add 60 µl H20 to cDNA, add 500 µl Buffer PB, apply to MinElute column, 13000 rpm 1 min, re-apply flow-though, 13000 rpm 1 min, discard flow-through, add 650 mL Buffer PE, 13000 rpm 1 min, dscard flow-through, repeat wash, spin column dry, 13000 rpm 60 s, transfer to fresh microtube, add 10 µl Buffer EB to center of filter, 2 minutes at RT, 13000 rpm 1 min, repeat elution with another 10 µl EB.
*50x aadNTP (4:1 aadUTP:dTTP): 10 µl each 100 mM dATP, dGTP, dCTP (Pharmacia), 8 µl 100 mM aminoallyl-dUTP (Sigma, #A0410), 2 µl 100 mM dTTP.
**Aliquot Cy3 dye: Dissolve 1 tube in 50 µl DMSO, add 5 µl to 8 tubes. Speed vac dry, store tubes in a dessicator in fridge.
 
Channel 2
Source name SiFbxo28, 16h
Organism Homo sapiens
Characteristics cell line: HCT116
cell type: colorectal carcinoma cells
genotype: FBXO28 knockdown
time point: 16h
Treatment protocol See Cepeda et al. The ubiquitin ligase SCFFBXO28 regulates Myc-driven transcription through non-proteolytic ubiquitylation and is required for cell proliferation.
Growth protocol See Cepeda et al. The ubiquitin ligase SCFFBXO28 regulates Myc-driven transcription through non-proteolytic ubiquitylation and is required for cell proliferation.
Extracted molecule total RNA
Extraction protocol Total RNA was extracted using TRIzol reagent (Invitrogen) according to the manufacturer’s instructions.
Label Cy5
Label protocol RNA priming: To 20 ug total RNA, add 10 ug 20(T)VN primer (MWG Biotech AG), adjust total volume to 18.4 µl, 70C 10 min , ice > 2 min, Prepare 1x RT-mixture (all reagents from Invitrogen): 5x RT-buff 6 µl, 50x aa-dNTP* 0.6 µl, DTT (0.1M) 3 µl, SuperScript II (200 U/µl) 2 µl.
cDNA synthesis: To primed RNA, add 11.6 µl RT-mix, add 42C 1 h 45 min.
RNA degradation: Add 3 µl 200 mM EDTA, add 4.5 µl 1 M NaOH, 70 C 15 min.
Neutralisation: Add 3 µl 1 M HCl.
Cleanup 1: Add 70 µl H20 + 500 µl PB, transfer to MinElute column (Qiagen), 13000 rpm 60 s, reapply flow-though, 13000 rpm 1 min, discard flow-through, add 600 µl 80% EtOH, 13000 rpm 60 s, repeat EtOH wash, spin column dry, 13000 rpm 60 s, transfer column to new microtube, add 10 µl 0.1 M NaCO3 pH 9.0, incubate 2 min, 13000 rpm 60 s, add 10 µl 0.1 M NaCO3 pH 9.0, 13000 rpm 60 s, transfer elution to aliquot of Cy3-dye (Amersham)**, mix with pipette, briefly centrifuge, incubate 1.5 h in dark at room temperature, add 4.5 µl 1 M hydroxylamine Cleanup 2 add 60 µl H20 to cDNA, add 500 µl Buffer PB, apply to MinElute column, 13000 rpm 1 min, re-apply flow-though, 13000 rpm 1 min, discard flow-through, add 650 mL Buffer PE, 13000 rpm 1 min, dscard flow-through, repeat wash, spin column dry, 13000 rpm 60 s, transfer to fresh microtube, add 10 µl Buffer EB to center of filter, 2 minutes at RT, 13000 rpm 1 min, repeat elution with another 10 µl EB.
*50x aadNTP (4:1 aadUTP:dTTP): 10 µl each 100 mM dATP, dGTP, dCTP (Pharmacia), 8 µl 100 mM aminoallyl-dUTP (Sigma, #A0410), 2 µl 100 mM dTTP.
**Aliquot Cy3 dye: Dissolve 1 tube in 50 µl DMSO, add 5 µl to 8 tubes. Speed vac dry, store tubes in a dessicator in fridge.
 
 
Hybridization protocol Slide preparation: Slides were pre-hybridised at 42°C for 45 min in the GeneTac hybridisation station. The pre-hybridisation mix consisted of 5x SSC, 1% BSA (Sigma-Aldrich), 0.1% SDS, 40 µg poly(dA) (Sigma-Aldrich) and 20 µg tRNA (Sigma-Aldrich).
Target preparation: Purified targets were pooled for each hybridisation. Hybridisation mixture was added to a final hybridisation composition of 5x SSC, 25% formamide, 0.1% SDS, 40 µg poly(dA) and 20 µg tRNA. The mixture was denaturated at 95 °C for 2 minutes and stored on ice.
Hybridisation: Hybridisation in a total volume of 110 µl was carried out for 16-18 hours at 42 °C using continuous agitation.
Wash: Hybridised slides were washed for five minutes with 2x SSC and 0.1% SDS at 42°C, followed by 0.1x SSC and 0.1% SDS at room temperature (five minutes) and finally by three one-minute washes with 0.1x SSC at room temperature. Washed slides were immediately dried using a slide centrifuge (Telechem).
Scan protocol Slides were scanned at 10-µm resolution immediately after washing. The photomultiplier tube setting was kept at 100 for all scans. Obtained images were rotated and the mirror image created using the provided software.
Description Control 16h vs. knockdown 16h.
Data processing Raw data files were imported into R using the KTH package for microarray analysis. Spots that were either saturated, flagged or had a foreground signal within two standard deviations from that spot's background were removed from further analysis. Individual channel data was converted into MA-format (M=log2 [Cy5/Cy3] ratio, A=log intensity) and within-slide print-tip normalisation was carried out. After manual evaluation of the distrubtion of M- and A-values across arrays, no between-slide normalisation was performed.
 
Submission date Feb 27, 2012
Last update date Feb 28, 2013
Contact name Daniel Klevebring
E-mail(s) daniel.klevebring@ki.se
Phone +46709499915
Organization name Karolinska Institutet
Department Medical Epidemiology and Biostatistics
Street address Nobels väg 12A
City Stockholm
ZIP/Postal code 17177
Country Sweden
 
Platform ID GPL15279
Series (1)
GSE36112 The SCFFBXO28 ubiquitin ligase coordinates CDK activity with MYC-mediated transcription in the cell cycle and predicts poor survival in breast cancer

Data table header descriptions
ID_REF
VALUE Print-tip normalized log2 (Cy5/Cy3) ratio (M-value)

Data table
ID_REF VALUE
HUMv301D01 -0.37664978976107
HUMv301H01 0.00758166975371299
HUMv301L01 -0.0318218576250692
HUMv301P01 -0.139632073047315
HUMv301D13 -0.23928387107317
HUMv301H13 -0.384455686680063
HUMv301L13 -0.0852995693614492
HUMv301P13 -0.230139971460926
HUMv302D01 -0.176295173424818
HUMv302H01 0.0958013797715349
HUMv302L01 -0.323975624668891
HUMv302P01 -0.359275866797802
HUMv302D13 -0.0551578442048166
HUMv302H13 -0.172669911329418
HUMv302L13 -0.325705123342237
HUMv302P13 -0.183710060393612
HUMv303D01 -0.620216457225807
HUMv303H01 -0.235131427160716
HUMv303L01 -0.220059265285964
HUMv303P01 -0.456217601435065

Total number of rows: 35712

Table truncated, full table size 912 Kbytes.




Supplementary file Size Download File type/resource
GSM881310_Red_13433525_S01_FlippedLLtoUR.gpr.gz 3.1 Mb (ftp)(http) GPR
Processed data included within Sample table

| NLM | NIH | GEO Help | Disclaimer | Accessibility |
NCBI Home NCBI Search NCBI SiteMap