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Sample GSM607110 Query DataSets for GSM607110
Status Public on Oct 01, 2011
Title 800-001_Peripheral_R_POP_30MAR2007_BWR
Sample type RNA
 
Source name Peripheral plaque
Organism Homo sapiens
Characteristics tissue: Peripheral plaque
sample id: 800-001_Peripheral_R_POP_30MAR2007_BWR
Extracted molecule total RNA
Extraction protocol Samples are processed in parallel in 96-well plates to minimize potential variation. Reaction purification is achieved using magnetic binding beads for cDNA and Qiagen RNeasy kits for cRNA purification.
Label Biotin is incorporated during the amplification. This binds a streptavidin-conjugated phycoerythrin during the post-hybridization staining process that provides the measurable signal.
Label protocol The final in vitro transcription incorporates biotin moieties that are later labeled with phycoerythrin. After amplification, samples are put through a controlled fragmentation to improve hybridization sensitivity and consistency. The labeled molecules are biotinylated-cRNA.
 
Hybridization protocol GeneChip microarrays are loaded with the fragmented target sample/hybridization buffer mix using standard manual techniques. Arrays are hybridized for 18 hours at 45?C with vigorous mixing. Unbound sample is removed and staining is accomplished through the binding of streptavidin conjugated phycoerythrin to the hybridized target. Excess label is removed. Washing and staining steps are performed by the Affymetrix FS450 fluidics station using standard protocols.
Scan protocol Arrays are scanned using a GeneChip Scanner 3000 7G with a 48 array autoloader. The scanner maintains the optimal temperature for the arrays prior to and during scanning.
Description Gene expression profiling of peripheral plaque. 290 subjects from CISTER study
Data processing Data were loaded into the Rosetta Resolver? system (Rosetta Biosoftware, Seattle, WA) and processed using the RMA algorithm (http://www.ncbi.nlm.nih.gov/sites/entrez?cmd=Retrieve&db=PubMed&list_uids=12582260). Intensities were calculated based on RMA, a Rosetta-developed error, and a MAS-5 p-value. The Rosetta-developed error is used in the calculation of xdev for the ratio p-values as described in section 2.2 (http://bioinformatics.oxfordjournals.org/cgi/content/full/22/9/1111).
 
Submission date Oct 12, 2010
Last update date Oct 01, 2011
Contact name Oscar Puig
E-mail(s) oscar_puig@merck.com
Organization name Merck Research Laboratories
Department Molecular Profiling Research Informatics
Street address 126 East Lincoln Ave
City Rahway
State/province NJ
ZIP/Postal code 07065
Country USA
 
Platform ID GPL10687
Series (2)
GSE23314 Gene expression profiling of human atherosclerotic plaque
GSE24702 Gene expression profiling of human atherosclerotic plaque: 290 peripheral plaques

Data table header descriptions
ID_REF Rosetta generated unique probe identifier
VALUE Expression level
PVALUE P-value of expression level

Data table
ID_REF VALUE PVALUE
100139735_TGI_at 14.9666 4.4190e-001
100124814_TGI_at 60.8924 7.8125e-002
100144091_TGI_at 1663.8149 9.7656e-004
100160468_TGI_at 5.1832 3.9648e-001
100137900_TGI_at 13.7997 4.7754e-001
100144981_TGI_at 61.4076 9.5215e-002
100140150_TGI_at 380.5719 4.8828e-004
100141475_TGI_at 616.9932 2.4414e-004
100159303_TGI_at 618.2571 2.4414e-004
100126869_TGI_at 26.1135 8.7036e-001
100127239_TGI_at 80.3327 9.5215e-002
100143101_TGI_at 25.1848 6.0107e-001
100143552_TGI_at 1316.1700 9.7656e-004
100152826_TGI_at 14.8313 7.3779e-001
100161135_TGI_at 2668.0586 1.9531e-003
100153329_TGI_at 3261.2327 4.8828e-004
100146530_TGI_at 2064.5750 9.7656e-004
100152459_TGI_at 37.4812 8.8379e-002
100130582_TGI_at 8.0086 8.9355e-001
100132539_TGI_at 42.3216 2.6660e-001

Total number of rows: 37582

Table truncated, full table size 1378 Kbytes.




Supplementary file Size Download File type/resource
GSM607110_@52048500653486111108403660366014.CEL.gz 3.3 Mb (ftp)(http) CEL
Processed data included within Sample table

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