NCBI Logo
GEO Logo
   NCBI > GEO > Accession DisplayHelp Not logged in | LoginHelp
GEO help: Mouse over screen elements for information.
          Go
Sample GSM241715 Query DataSets for GSM241715
Status Public on Nov 13, 2007
Title shma-p53null 24h 0.5 BPDE A
Sample type RNA
 
Channel 1
Source name sh241005-p53null 24h DMSO A(sh241005-p53null 24h DMSO A )
Organism Homo sapiens
Characteristics tissue type: tumor
Extracted molecule total RNA
Extraction protocol Cell pellets were collected and total RNA extracted using the Qiagen RNeasy Mini Kit protocol (RNeasy Mini Handbook, Qiagen, UK). After addition of lysis buffer (RLT, Qiagen) samples were homogenized using QIAshredders (Qiagen).
Label Cy3
Label protocol Total RNA (4 ug) was reversed transcribed into cDNA and fluorescently labelled with Cy3 or Cy5 mono-reactive dyes (Amersham Biosciences, UK) using the Invitrogen Indirect cDNA Labelling Kit protocol (Invitrogen, UK) according to the manufacturer's instructions. After labelling, repetitive sequences within the cDNA samples were blocked with 16 ug Human Cot-1 DNA (Invitrogen, UK) to prevent non-specific sequences binding to the cDNA probes.
 
Channel 2
Source name sh241005-p53null 24h 0.5 BPDE A(sh241005-p53null 24h 0.5 BPDE A )
Organism Homo sapiens
Characteristics tissue type: tumor
Extracted molecule total RNA
Extraction protocol Cell pellets were collected and total RNA extracted using the Qiagen RNeasy Mini Kit protocol (RNeasy Mini Handbook, Qiagen, UK). After addition of lysis buffer (RLT, Qiagen) samples were homogenized using QIAshredders (Qiagen).
Label Cy5
Label protocol Total RNA (4 ug) was reversed transcribed into cDNA and fluorescently labelled with Cy3 or Cy5 mono-reactive dyes (Amersham Biosciences, UK) using the Invitrogen Indirect cDNA Labelling Kit protocol (Invitrogen, UK) according to the manufacturer's instructions. After labelling, repetitive sequences within the cDNA samples were blocked with 16 ug Human Cot-1 DNA (Invitrogen, UK) to prevent non-specific sequences binding to the cDNA probes.
 
 
Hybridization protocol Corresponding control and treated samples labelled with different fluorophores were combined in a 50 ul hybridisation mix (19 ul Microarray Hybridisation Solution purchased from GE Healthcare and 50% deionised formamide) and heated at 70°C for 2 min and then at 37°C for 10 min. Sample was pipetted onto a microarray slide and covered with a glass cover slip. A 150ul aliquot of 6 X SSPE was pipetted underneath the slide to prevent dehydration. The hybridisation chamber was sealed and incubated at 42°C for 72 h. Type 7* slides were washed three times in 4 X SSPE, 10 mM EDTA pH 8.0 as above, followed by a 10 s wash in 50% deionised formamide, 6 X SSPE, before a brief rinse in HPLC grade water and drying with nitrogen gas.
Scan protocol Scanner: Axon4000A. Voltage: 4.09 3.62. Resolution (micrometers): 10.
Description Labelled sample was reduced down to 3 µl using Microcon YM-30 centifugal filters (Millipore, UK). Corresponding control and treated samples labelled with different fluorophores were combined in a 50 µl hybridisation mix (19 µl Microarray Hybridisation Solution purchased from GE Healthcare and 50% deionised formamide) and heated at 70degC for 2 min and then at 37degC for 10 min. Sample was pipetted onto a microarray slide and covered with a glass cover slip. A 150µl aliquot of 6 X SSPE was pipetted underneath the slide to prevent dehydration. The hybridisation chamber was sealed and incubated at 42degC for 72 h.
Data processing Regions were used for normalizing samples 1-24. A Lowess curve was fit to the log-intensity versus log-ratio plot. 20.0% of the data was used to calculate the Lowess fit at each point. This curve was used to adjust the control value for each measurement. If the control channel was lower than 10 then 10 was used instead.
 
Submission date Nov 08, 2007
Last update date Apr 24, 2013
Contact name Ian Giddings
E-mail(s) [email protected], [email protected]
Phone +44 20 8722 4293
Fax +44 20 8722 4141
URL http://www.crukdmf.icr.ac.uk
Organization name Institute of Cancer Research
Department Section of Molecular Carcinogenesis
Lab CANCER RESEARCH UK DNA Microarray Facility
Street address 15 Cotswold Road
City Sutton
State/province Surrey
ZIP/Postal code SM2 5NG
Country United Kingdom
 
Platform ID GPL4348
Series (1)
GSE9547 p53 status and BaP or BPDE gene expression response

Data table header descriptions
ID_REF IMAGE clone ID if the value is numeric. Else, it is an oligo ID. the suffix _ is used for copies
VALUE log2-transformed normalised ratio (Cy5/Cy3)
CH1_MEDIAN channel 1 signal intensity median - Cy3 (cyanine 3)
CH1_MEAN channel 1 signal intensity mean
CH1_SD channel 1 signal intensity standard deviation
CH1_AREA Number of pixels used to determine channel 1 signal intensity
CH1_BKD_MEDIAN channel 1 background signal intensity median
CH1_BKD_MEAN channel 1 background signal intensity mean
CH1_BKD_SD channel 1 background signal intensity standard deviation
CH1_BKD_AREA Number of pixels used to determine channel 1 background signal intensity
CH2_MEDIAN channel 2 signal intensity median - Cy5 (cyanine 5)
CH2_MEAN channel 2 signal intensity mean
CH2_SD channel 2 signal intensity standard deviation
CH2_AREA Number of pixels used to determine channel 2 signal intensity
CH2_BKD_MEDIAN channel 2 background signal intensity median
CH2_BKD_MEAN channel 2 background signal intensity mean
CH2_BKD_SD channel 2 background signal intensity standard deviation
CH2_BKD_AREA Number of pixels used to determine channel 2 background signal intensity
RATIO normalised ratio (Cy5/Cy3)

Data table
ID_REF VALUE CH1_MEDIAN CH1_MEAN CH1_SD CH1_AREA CH1_BKD_MEDIAN CH1_BKD_MEAN CH1_BKD_SD CH1_BKD_AREA CH2_MEDIAN CH2_MEAN CH2_SD CH2_AREA CH2_BKD_MEDIAN CH2_BKD_MEAN CH2_BKD_SD CH2_BKD_AREA RATIO
22170 -0.0923 65535 64814 3104 52 9611 11978 8087 52 65535 63650 6482 52 4828 6766 7557 52 0.9380
21642 -0.0923 65535 58827 15103 80 8609 10247 6828 80 65535 57274 17652 80 4850 6292 6348 80 0.9380
22209 0.0356 64850 59872 9572 52 8303 11519 11070 52 58967 56567 10397 52 4763 7967 11085 52 1.0250
22121 0.0144 50886 50982 8266 52 7733 9573 6857 52 45629 44850 7652 52 4478 6057 5850 52 1.0100
24284 0.0257 48694 49090 6568 52 7258 9210 7396 52 43108 43735 7874 52 4752 6532 6753 52 1.0180
66999 -0.0923 65535 62543 10019 52 6179 7455 5849 52 65535 61914 12410 52 3920 5141 5329 52 0.9380
110223 -0.0306 34953 34621 2875 52 5580 6925 5693 52 31007 30588 3593 52 3495 4808 4809 52 0.9790
110202 -0.0160 28196 28639 3610 52 5039 5512 1936 52 24265 25029 3651 52 3284 3743 1467 52 0.9890
21744 -0.0336 21154 20584 3499 52 4798 5004 1338 52 17849 17654 3042 52 3084 3414 1138 52 0.9770
22739 -0.1313 30092 29903 5061 52 4504 4673 1092 52 28253 27275 5136 52 3038 3280 899 52 0.9130
53153 -0.0439 17796 19159 4709 52 4200 4378 1069 52 14780 16122 4447 52 2925 3209 897 52 0.9700
22559 -0.1408 22941 21057 6338 80 4031 4147 871 80 21174 19121 6187 80 2841 2968 513 80 0.9070
66951 0.2975 3815 3932 731 156 3921 4093 879 156 2876 2944 421 156 2781 2898 448 156 1.2290
23643 0.1570 23048 22658 2981 52 3981 4135 899 52 17078 17055 2193 52 2820 2946 446 52 1.1150
108692 -0.1016 8892 8870 834 52 3508 3664 976 52 7566 7674 902 52 2774 2850 346 52 0.9320
108718 0.2388 16411 16302 1727 52 3567 3756 996 52 10957 10882 1302 52 2720 2826 527 52 1.1800
115266 0.0731 9148 9000 926 52 3500 3711 1167 52 6896 6930 669 52 2733 2918 743 52 1.0520
121091 0.1124 20785 20606 2101 52 3362 3702 1710 52 15735 15593 1516 52 2716 2910 1105 52 1.0810
125723 0.1440 9059 8969 1096 52 3429 3585 744 52 6527 6463 563 52 2735 2776 290 52 1.1050
125145 0.3785 16851 16075 3690 52 3311 3420 911 52 10214 9748 1495 52 2732 2809 330 52 1.3000

Total number of rows: 19346

Table truncated, full table size 1722 Kbytes.




Supplementary file Size Download File type/resource
GSM241715.gpr.gz 2.2 Mb (ftp)(http) GPR
Processed data included within Sample table

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