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Sample GSM283994 Query DataSets for GSM283994
Status Public on Apr 01, 2010
Title D2-CD133-G-CSF+AMD3100 - mAdbID:82733
Sample type RNA
 
Channel 1
Source name CD133 - GCSF plus AMD3100 Mobilized
Organism Homo sapiens
Characteristics Tissue: blood
Cell type: CD133
Treatment protocol Treatment type: compound
Agent: GCSF plus AMD3100
Treatment dose: 10 ug / kg (GCSF); 240 ug / kg (AMD3100)
Treatment time: 5 days (GCSF); 12 hours (AMD3100)
In-vivo treatment: Healthy donors recieved GCSF for 5 days. On the 5th day donors recieved one dose of AMD3100. 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: 3.19;; 3.6
Temperature: 26.17
Description mAdb experiment ID: 82733
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 -1.222060323 1 1 1 12462 3391 1854 966 15777 5198 1109 1025 0
6519905_1 NULL 1 1 2 1872 694 1730 796 1149 522 1112 635 -50
6519997_1 NULL 1 1 3 1699 783 1737 2658 1099 534 1103 1376 -50
6520089_1 NULL 1 1 4 2151 1183 1662 1098 1396 1099 1031 777 -50
6520181_1 -1.116308451 1 1 5 2769 936 1701 2203 2386 900 1048 843 0
6520273_1 NULL 1 1 6 2456 990 1626 2161 1336 1327 1101 863 -50
6520365_1 NULL 1 1 7 1795 898 1555 3476 1102 455 1073 1610 -50
6520385_1 NULL 1 1 8 1786 735 1596 1078 1184 747 1082 574 -50
6519885_2 -1.222060323 1 2 1 10394 4162 1718 1170 14414 5877 1026 950 0
6519905_2 NULL 1 2 2 1854 671 1728 1726 1101 463 1074 709 -50
6519997_2 NULL 1 2 3 1706 679 1612 801 1141 531 1103 556 -50
6520089_2 NULL 1 2 4 1752 778 1642 1287 1804 4025 1041 1359 -50
6520181_2 -1.116308451 1 2 5 2717 1030 1705 1301 2328 1012 1054 713 0
6520273_2 NULL 1 2 6 2360 2782 1623 853 1528 1701 1068 736 -50
6520365_2 NULL 1 2 7 1990 786 1641 1699 1316 635 1021 984 -50
6520385_2 NULL 1 2 8 1855 884 1650 2153 1362 1210 1102 2054 -50
6519889_1 -0.067682028 1 3 1 6327 2123 1570 2176 3831 1146 1162 1139 0
6519981_1 -1.504942536 1 3 2 2791 1022 1611 1345 3143 1387 1138 792 0
6520001_1 NULL 1 3 3 1683 852 1617 992 1472 1741 1165 1434 -50
6520093_1 NULL 1 3 4 1764 645 1578 766 1278 685 1101 1578 -50

Total number of rows: 1456

Table truncated, full table size 91 Kbytes.




Supplementary file Size Download File type/resource
GSM283994.gpr.gz 137.8 Kb (ftp)(http) GPR
Processed data included within Sample table

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