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Sample GSM157212 Query DataSets for GSM157212
Status Public on Feb 01, 2007
Title CD4+CD25+ vs. NKT spleen Sort II
Sample type RNA
 
Channel 1
Source name CD4+CD25+
Organism Mus musculus
Characteristics C57BL/6 CD4+CD25+
Extracted molecule total RNA
Extraction protocol Trizol isolation + RNeasy purification
Label Cy3
Label protocol Agilent Technologies fluorescent linear amplification reaction
 
Channel 2
Source name NKT spleen
Organism Mus musculus
Characteristics C57BL/6 NKT spleen
Extracted molecule total RNA
Extraction protocol Trizol isolation + RNeasy purification
Label Cy5
Label protocol Agilent Technologies fluorescent linear amplification reaction
 
 
Hybridization protocol Agilent Technologies
Scan protocol Agilent Technologies
Description Antibodies
Antibodies against murine CD4, FasL, IL-4, IFN, TNF, CXCR4, Mac-1, B220, CD11c and CD8 were isolated from hybridoma cell lines. The alpha-GalCer tetramers were produced as previously described. Antibodies against murine NK1.1, CD3, CD25, LFA-1 and Streptavidin-PE-Cy7 were obtained from BD Bioscience (Heidelberg, Germany)
Isolation and purification of cells by MACS and FACS sorting
Isolation of spleen and liver lymphocytes, red blood cell lysis and tetramer stainings were performed as described elsewhere [28]. Magnetic cell sorting (MACS) with MicroBeads (Miltenyi Biotec, Bergisch Gladbach, Germany) was performed according to manufacturer’s protocol to enrich cell populations by positive selection. Subsequently, enriched cells were sorted using a FACS-Diva (BD Bioscience, Heidelberg, Germany). All manipulations were performed at 4°C. Cells were sorted into tubes containing cold PBS, 0.1% BSA to avoid activation of cells. Viable cells were detected by staining with PI (propidium iodid) or DAPI (Diamidino-phenylindol). The purity of sorted fractions was verified visually and by FACS reanalysis. At least 5 × 105 cells were isolated by FACS sorting and further used for microarray analysis. FACS sorts were repeated four times and duplicate samples of each sorted cell type were used for two independent microarray studies.
Preparation of RNA from single cell suspension
Total RNA was isolated by the TRIzol® Reagent RNA preparation method (Invitrogen, Karlsruhe, Germany). Briefly, cells were resuspended immediately after FACS sorting in 500 µl TRIzol, shock frozen and stored at –80°C. Cells were thawed and further processed for total RNA isolation as described by the manufacturer. The amount of RNA was determined by OD260/280 nm measurement and total RNA was purified by RNeasy (Qiagen, Hilden, Germany). The RNA integrity and the amount of total RNA were measured with a Bioanalyzer 2100 (Agilent Technologies, Waldbronn, Germany).
Data processing Features were extracted with an image analysis tool version A.6.1.1 (Agilent Technologies) using default settings. Data analysis was carried out on the Rosetta Inpharmics platform Resolver Version 5.0. Ratio profiles were combined in an error-weighted fashion with Resolver to create ratio experiments. A two fold change expression cut-off for ratio experiments was applied together with anti-correlation of ratio profiles rendering the microarray analysis set highly significant (P-value > 0.05), robust and reproducible.
 
Submission date Jan 22, 2007
Last update date Jan 22, 2007
Contact name Hans-Joachim Mollenkopf
E-mail(s) mollenkopf@mpiib-berlin.mpg.de
Phone +49 30 28460 482
Organization name Max-Planck-Institute for Infection Biology
Lab Microarray/Genomics Core Facility
Street address Charitéplatz 1
City Berlin
ZIP/Postal code 10117
Country Germany
 
Platform ID GPL1868
Series (1)
GSE6782 Natural killer T-cell characterization through gene expression profiling

Data table header descriptions
ID_REF
Fold Change
P-value
Intensity1
Intensity2
Log(Intensity)
Ratio
VALUE log(Ratio) with flagged values removed
Log(Error)
X Dev
Fail Code(s)
Flagged?

Data table
ID_REF Fold Change P-value Intensity1 Intensity2 Log(Intensity) Ratio VALUE Log(Error) X Dev Fail Code(s) Flagged?
633390 -2.09682 0.00444 219.48621 104.676 2.18063 0.47691 -0.32156 0.11302 -2.84508 OK No
633391 1.0673 5.66E-01 7162.51514 7644.56104 3.86921 1.0673 0.02829 0.04922 0.57468 OK No
633392 1.05109 0.66036 5056.89893 5315.27197 3.7147 1.05109 0.02164 0.04925 0.43942 OK No
633393 3.43624 1.75E-17 33903.23047 116499.6016 4.79828 3.43624 0.53608 0.063 8.50924 OK No
633394 1.12129 5.59E-01 208.7173 234.033 2.34442 1.12129 0.04972 0.08514 0.58396 OK No
633395 -1.06666 0.83265 128.71091 120.6667 2.0956 0.9375 -0.02803 0.13264 -0.21131 OK No
633396 -1.44218 1.55E-01 183.5338 127.2617 2.18421 0.6934 -0.15902 0.11194 -1.42053 OK No
633397 1.25761 1.92E-01 235.5938 296.28461 2.42194 1.25761 0.09955 0.07635 1.30373 OK No
633398 -1.74274 3.84E-06 17193.57031 9865.80664 4.11475 0.57381 -0.24123 0.05222 -4.61959 OK No
633399 -1.48137 0.0869 216.3311 146.0347 2.24979 0.67505 -0.17066 0.09969 -1.712 OK No
633400 -1.39472 4.07E-03 9089.76562 6517.2832 3.88631 0.71699 -0.14449 0.0503 -2.87275 OK No
633401 2.17151 3.31E-08 385.86569 837.91052 2.75482 2.17151 0.33676 0.06096 5.52413 OK No
633402 -1.05048 6.88E-01 760.57678 724.0246 2.87045 0.95194 -0.02139 0.05334 -0.40104 OK No
633403 -3.79691 3.53E-03 148.22549 39.03846 1.88121 0.26337 -0.57943 0.19859 -2.91776 OK No
633404 -1.40719 4.41E-03 1340.05505 952.28943 3.05295 0.71063 -0.14835 0.0521 -2.84732 OK No
633405 -1.22051 1.48E-01 506.91739 415.33139 2.66167 0.81933 -0.08654 0.05975 -1.44836 OK No
633406 1.18865 2.49E-01 332.32529 395.0191 2.55909 1.18865 0.07505 0.06508 1.15322 OK No
633407 -1.33382 0.28534 166.89951 125.1293 2.15991 0.74973 -0.1251 0.11709 -1.06841 OK No
633408 1.21045 0.60027 92.68344 112.1888 2.00848 1.21045 0.08295 0.15829 0.52402 OK No
633409 1.3191 0.05256 361.60541 476.99219 2.61837 1.3191 0.12028 0.06205 1.93852 OK No

Total number of rows: 8014

Table truncated, full table size 686 Kbytes.




Supplementary file Size Download File type/resource
GSM157212.tif.gz 29.1 Mb (ftp)(http) TIFF
GSM157212.txt.gz 2.0 Mb (ftp)(http) TXT
GSM157212.xml.gz 1.3 Mb (ftp)(http) XML

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