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Sample GSM142528 Query DataSets for GSM142528
Status Public on Dec 01, 2006
Title p63_ChIP-chip_B3, (-)ActD, chip 04 of 14
Sample type genomic
 
Source name Cervical carcinoma
Organism Homo sapiens
Characteristics Age: 66 yrs Gender: Female Ethnicity: Caucasian
Biomaterial provider Peter Howley, Harvard Medical School, Boston, MA
Treatment protocol Cells were treated with 5nM Actinomycin D or ethanol (vehicle control) for 24-26 hrs before harvesting by trypsinization
Growth protocol Cells were grown in Dulbecco's Modified Eagle Medium (DMEM) supplemented with 10% Fetal Bovine Serum
Extracted molecule genomic DNA
Extraction protocol 1. Trypsinized cells were placed into fresh media and cross-linked by the addition of formaldehyde.
2. Cells were then spun down and the cell pellet was then resuspended in micrococcal nuclease (MNase) reaction buffer.
3. The chromatin was then sonicated, spun down and the supernatant was diluted with IP-dilution buffer.
4. Diluted chromatin was precleared with protein A/G sepharose beads, and a portion reserved for control, or 'input', DNA (i.e. omitting immunoprecipitation).
5. The remaining chromatin was incubated with 4A4 anti-p63 antibody-coupled protein A/G sepharose beads.
6. Input and eluted material was de-crosslinked and purified.
Label Biotin
Label protocol Amplified ChIP (or matching input) DNA was fragmented with DNase I, and then biotin-labeled using terminal transferase (TdT).
 
Hybridization protocol Biotinylated DNA was hybridized to the Affymetrix tiled, human whole genome arrays, washed, and stained according to manufacturer's instructions.
Scan protocol The microarrays were scanned using a custom-built Affymetrix scanner with a laser spot size of 3.5 um and a resolution (pixel size) of 1.0 um. Thus each feature on the array with the size of 5x5 um was represented by 25 data points (pixels). To estimate the intensity of each feature, the outer rim of pixels was discarded and the 75th-percentile of the remaining 9 pixels was used as the estimate of the intensity.
Description Input and ChIP DNA was amplified by two rounds of primer extension (Round A) with random primers, followed by purification and two successive rounds of PCR (Round B and C).
The samples were then purified using column purification and ready for array hybridization protocols.
Data processing A binding P-value for each genomic position was determined by the Wilcoxon rank sum test.
 
Submission date Oct 27, 2006
Last update date Sep 02, 2008
Contact name Kevin Struhl
Organization name Harvard Medical School
Department Dept. Of Biological Chemistry & Molecular Pharmacology
Lab Struhl lab
Street address 240 Longwood Ave.
City Boston
State/province MA
ZIP/Postal code 02115
Country USA
 
Platform ID GPL4492
Series (1)
GSE6132 Whole genome mapping of p63 binding sites in ME180 human cervical carcinoma cells

Data table header descriptions
ID_REF
VALUE signal
P-VALUE binding P-value -10*log10(P)

Data table
ID_REF VALUE P-VALUE
3_162000532_2392_1503 0 1.82506
3_162000556_808_1707 0 1.82506
3_162000587_2405_959 0 2.8196
3_162000623_2090_279 0 3.30316
3_162000660_1202_2377 0 3.24004
3_162000696_385_1269 0 2.78928
3_162000742_598_2453 0 2.09733
3_162000775_746_725 0 3.09213
3_162000814_1256_563 0 4.06894
3_162000850_2404_1841 0 5.13365
3_162000891_2552_1853 0 4.25839
3_162000928_2127_1387 0 3.7149
3_162000959_298_2219 0 3.43949
3_162000995_1524_1549 0 3.18028
3_162001028_1733_2201 0 3.13992
3_162001066_1415_1389 0 2.78944
3_162001102_2495_1715 0 2.91994
3_162001140_1351_333 0 2.96281
3_162001181_768_1347 0 2.92807
3_162001216_933_795 0 5.0028

Total number of rows: 2960773

Table truncated, full table size 89811 Kbytes.




Supplementary file Size Download File type/resource
GSM142528.CEL.gz 29.2 Mb (ftp)(http) CEL

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