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Sample GSM284005 Query DataSets for GSM284005
Status Public on Apr 01, 2010
Title D5-CD34-G-CSF - mAdbID:83118
Sample type RNA
 
Channel 1
Source name CD34 - GCSF Mobilized
Organism Homo sapiens
Characteristics Tissue: blood
Cell type: CD34
Treatment protocol Treatment type: compound
Agent: GCSF
Treatment dose: 10 ug / kg
Treatment time: 5 days
In-vivo treatment: Healthy people recieved GCSF for 5 days. Then the PBSC were collected by aphoresis.
Extracted molecule total RNA
Extraction protocol RNA extraction with TRIZOL
Extraction method: TRIZOL
Other: Cells were lysed with TRIzol reagent (Invitrogen, Carlsbad, CA) and total RNA was isolated according to the manufacturers instructions. RNA integrity was assessed by the presence of 28S and 18S bands using Agilent bioanalyzer and quantified using nanodrop with A260/A280 ratios > 2.0 after dilution in DEPC water.
Label cy5
Label protocol Cy5 Sample Labeling Protocol
Other: Small RNA was enriched from 10ug total RNA by flashPAGE (Pre-cast Gel,Type A) (Ambion, Austin, TX, USA) and purified using flashPAGE reaction clean-up kit (Ambion, Austin, TX, USA) according to manufacture’s instruction. The same procedures were applied to obtain small RNA from the Epstein-Barr virus (EBV)-transformed lymphoblastoid cell lines that was used as the reference for the miRNA expression array assay. Fragmented small RNA were 3’-end tailed with amine-modified nucleotides and chemically coupled to CyDye fluors (Amersham Biosciences, piscatway, NJ, USA), which sample with Cy5 and the reference with Cy3 respectively, using the mirVana miRNA Labeling Kit (Ambion) following the recommended protocol by the manufactures’ instruction. After labeling, the samples and the reference were co-hybridized to the miRNA array at room temperature over night. Both the processed cDNA and the miRNA array slides were scanned by GenePix scanner Pro 4.0 (Axon, Sunnyvale, CA, USA).
 
Channel 2
Source name EBV-infected B cell line
Organisms Homo sapiens; human gammaherpesvirus 4
Characteristics Tissue: blood
Cell type: EBV-infected B cell
Extracted molecule total RNA
Extraction protocol RNA extraction with TRIZOL
Extraction method: TRIZOL
Other: Cells were lysed with TRIzol reagent (Invitrogen, Carlsbad, CA) and total RNA was isolated according to the manufacturers instructions. RNA integrity was assessed by the presence of 28S and 18S bands using Agilent bioanalyzer and quantified using nanodrop with A260/A280 ratios > 2.0 after dilution in DEPC water.
Label cy3
Label protocol Cy3 Sample Labeling Protocol
Other: Small RNA was enriched from 10ug total RNA by flashPAGE (Pre-cast Gel,Type A) (Ambion, Austin, TX, USA) and purified using flashPAGE reaction clean-up kit (Ambion, Austin, TX, USA) according to manufacture~Rs instruction. The same procedures were applied to obtain small RNA from the Epstein-Barr virus (EBV)-transformed lymphoblastoid cell lines that was used as the reference for the miRNA expression array assay. Fragmented small RNA were 3~R-end tailed with amine-modified nucleotides and chemically coupled to CyDye fluors (Amersham Biosciences, piscatway, NJ, USA), which sample with Cy5 and the reference with Cy3 respectively, using the mirVana miRNA Labeling Kit (Ambion) following the recommended protocol by the manufactures~R instruction. After labeling, the samples and the reference were co-hybridized to the miRNA array at room temperature over night. Both the processed cDNA and the miRNA array slides were scanned by GenePix scanner Pro 4.0 (Axon, Sunnyvale, CA, USA).
 
 
Hybridization protocol Sample Hybridization Protocol
Other: Small RNA was enriched from 10ug total RNA by flashPAGE (Pre-cast Gel,Type A) (Ambion, Austin, TX, USA) and purified using flashPAGE reaction clean-up kit (Ambion, Austin, TX, USA) according to manufacture’s instruction. The same procedures were applied to obtain small RNA from the Epstein-Barr virus (EBV)-transformed lymphoblastoid cell lines that was used as the reference for the miRNA expression array assay. Fragmented small RNA were 3’-end tailed with amine-modified nucleotides and chemically coupled to CyDye fluors (Amersham Biosciences, piscatway, NJ, USA), which sample with Cy5 and the reference with Cy3 respectively, using the mirVana miRNA Labeling Kit (Ambion) following the recommended protocol by the manufactures’ instruction. After labeling, the samples and the reference were co-hybridized to the miRNA array at room temperature over night. Both the processed cDNA and the miRNA array slides were scanned by GenePix scanner Pro 4.0 (Axon, Sunnyvale, CA, USA).
Scan protocol Creator: GenePix Pro 4.0.1.17
Scanner: GenePix 4000B [84945]
ScanPower: 33;; 33
LaserPower: 3.25;; 3.26
Temperature: 29.35
Description mAdb experiment ID: 83118
Data processing BRBArrayTools
Calculation Method: Fluorescence intensities generated by Cy5 and Cy3 probes hybridized onto the microarray slides were scanned were scanned on a GenePix 4000 (Axon Instruments, Union City, CA) at variable PMT voltage to obtain maximal signal intensities with < 1% probe saturation. Data were uploaded to National Institute of Health, NCI/CCR µArray database (http://nciarray.nci.nih.gov). Raw data were retrieved in BRB-ArrayTools(http://linus.nci.nih.gov/BRBArrayTools.html) format for analysis and normalization. Following filter criteria was applied to the data set: 1. spots were excluded if intensity < 100, and spot size less than 10um 2. genes were filtered out if >80% of experiment with missing data values. 3. log2 transformed data were normalized using lowess smoother, and intensity ratios were truncated if greater than 64. Transcriptional data were process by averaging results in replicate experiments for the same genes. Hierchical clustering analysis was performed on BRBArray tools using centered correlation as similarity metric and centroid linkage method: Cluster 3:0. Heat maps were generated using Eisen’s TreView Software.
 
Submission date Apr 23, 2008
Last update date Mar 23, 2009
Contact name Francesco Maria Marincola
E-mail(s) fmarincola@sidra.org
Phone 301-793-8210
Organization name Sidra Medical and Research Center
Street address Al Nasr Tower, AL Corniche Street, PO Box 26999
City Doha
ZIP/Postal code PO Box 26999
Country Qatar
 
Platform ID GPL6773
Series (2)
GSE11248 Peripheral blood stem cell microRNA profiling
GSE11255 Peripheral blood stem cell gene and microRNA profiling

Data table header descriptions
ID_REF NCI mAdb well id plus replicate number
VALUE log2 of the Calibrated Ratio (Cy5 channel/Cy3 channel)
Slide_block Array block location
Slide_column Array column location
Slide_row Array row location
CY5_mean Red Channel Sample mean Signal (Background Subtracted)
CY5_SD Red Channel Sample Standard Deviation
CY5_BKD_median Red Channel Sample median Background Level
CY5_BKD_SD Red Channel Sample Background Standard Deviation
CY3_mean Green Channel Sample mean Signal (Background Subtracted)
CY3_SD Green Channel Sample Standard Deviation
CY3_BKD_median Green Channel Sample median Background Level
CY3_BKD_SD Green Channel Sample Background Standard Deviation
Flag Quality flag 0->good, -50->Not found, -100->Bad

Data table
ID_REF VALUE Slide_block Slide_column Slide_row CY5_mean CY5_SD CY5_BKD_median CY5_BKD_SD CY3_mean CY3_SD CY3_BKD_median CY3_BKD_SD Flag
6519885_1 -1.721481681 1 1 1 11658 4080 3202 986 16187 6113 2508 763 0
6519905_1 NULL 1 1 2 3334 1528 3060 997 2751 1524 2362 928 -50
6519997_1 NULL 1 1 3 2816 1001 3043 987 2834 2548 2427 858 -50
6520089_1 NULL 1 1 4 3063 932 3040 1789 2544 854 2321 836 -50
6520181_1 -3.138143778 1 1 5 4519 1377 3024 986 5527 3983 2288 912 0
6520273_1 NULL 1 1 6 3969 1274 3087 1090 2873 1584 2405 813 -50
6520365_1 NULL 1 1 7 3761 1454 3189 1096 3190 2886 2387 996 -50
6520385_1 NULL 1 1 8 3660 2144 3302 1055 3012 2616 2387 874 -50
6519885_2 -1.721481681 1 2 1 11459 3697 3143 1073 16763 6335 2387 815 0
6519905_2 NULL 1 2 2 3246 1288 3155 1066 2885 2257 2370 1614 -50
6519997_2 NULL 1 2 3 3039 1161 2949 960 2802 3801 2338 755 -50
6520089_2 NULL 1 2 4 3413 1150 3096 1015 3093 3726 2406 771 -50
6520181_2 -3.138143778 1 2 5 3992 1115 3271 1082 5043 4676 2335 800 0
6520273_2 NULL 1 2 6 4000 1345 3262 1823 2665 721 2452 938 -50
6520365_2 NULL 1 2 7 3738 1258 3423 1080 2745 1304 2548 1250 -50
6520385_2 NULL 1 2 8 3491 1919 3339 1155 3406 4243 2397 1016 -50
6519889_1 0.784479797 1 3 1 11933 3474 3004 1028 4470 1502 2418 819 0
6519981_1 -2.287443399 1 3 2 9280 15372 2902 940 8111 9245 2275 705 0
6520001_1 NULL 1 3 3 2938 1517 2876 1061 2462 941 2257 813 -50
6520093_1 NULL 1 3 4 2752 895 3031 1018 2287 740 2289 794 -50

Total number of rows: 1456

Table truncated, full table size 93 Kbytes.




Supplementary file Size Download File type/resource
GSM284005.gpr.gz 140.7 Kb (ftp)(http) GPR
Processed data included within Sample table

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