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Sample GSM361187 Query DataSets for GSM361187
Status Public on Oct 09, 2009
Title Monocyte_HVL_014
Sample type RNA
 
Source name monocytes, HVL
Organism Homo sapiens
Characteristics viral load: 72000
cd4: 472
age: 51
Extracted molecule total RNA
Extraction protocol Total RNA extracted with Qiagen Rneasy Micro kit
Label Biotin
Label protocol 0.5 ug total RNA, 2.5 ul 1:1000 - 1:2^10 bacterial mRNA controls, 1ul T7 Oligo(dT) primer, add water to 12ul. Incubate for 10min at 70C. Add 2ul 10x First Strand Buffer, 4ul 5mM dNTP, 1ul RNase Inhibitor, 1ul ArrayScript to reaction. Incubate for 2h at 42C. Add 63ul water, 10ul 10x Second Starnd Buffer, 4ul 5mM dNTP Mix, 2ul DNA polymerase, 1ul RNaseH. Incubate for 2h at 16C. Purify the cNDA using column by adding 250ul cDNA Binding Buffer, spin at 10000g for 1min. Add 500ul Washing Buffer to column followed by spin at 10000g for 1 min. Spin dry the column. Add 12ul 50C water for disolving cDNA for 2min. Spin at 10000g for 1.5min. Repeat the elute step once. For labelling, add 12ul Biotin-NTP Mix, 4ul 10x T7 Reaction Buffer, 4ul 10x T7 Enzyme Mix to reaction. Incubate for 14h at 37C. Recover cRNA by columns. Add 60ul water and 350ul cRNA Binding Buffer to reaction. Transfer to column, spin and add 250ul 100% Ethanol and spin again. Add 650ul Washing Buffer, spin. Then spin dry the column. Add 100ul 50C water to disolve the cRNA.
 
Hybridization protocol Fragment 10ug labeled cRNA in 20ul by adding 5ul 5x Fragmentation Buffer and incubate for 20C at 94C. Add 78ul BufferA, 130ul BufferB 27ul water and incubate for 5min at 90C to denature cRNA. Load reaction to bioarray chamber. Incubate for 22h at 37C on a 300rmp rotating platform. Wash slides using 0.75x TNT for 1hr at 46C. Stain slides using 2ug/ml Alexa Fluor 647-streptavidin in TNB buffer at room temprature for 30 min in dark. Then wash the slides 4 times using 1x TNT for 5min each time. Wasing slides using 0.1x SSC/ 0.05% Tw20 for 30sec. Dry slides at 2000rpm for 3min.
Scan protocol Axon Genepix Pro 4100B scanner and GenePixPro 3.0 software, using wavelength 635nm, PTM 600V, 100% laser power, 5um pixel size, focus at 0um.
Description Monocyte_HVL_014
Data processing Discovery spots were loess normalized in R/BioConductor, then imported into GeneSpring GX 7.3.1 and normalized to 50th percentile per chip and median per gene, less than 0.01 set to 0.01.
 
Submission date Jan 16, 2009
Last update date Oct 08, 2009
Contact name Bing Sun
E-mail(s) [email protected]
Organization name San Francisco VA Medical Center
Street address B1, R103, 4150 Clement St
City San Francisco
State/province CA
ZIP/Postal code 94121
Country USA
 
Platform ID GPL2895
Series (1)
GSE18464 IFN-a-induced monocyte phenotype in chronic unsuppressed HIV infection

Data table header descriptions
ID_REF
FLAG
SIGNAL_RAW
BKD_RAW
EXPRESSION
VALUE Loess normalized intensity

Data table
ID_REF FLAG SIGNAL_RAW BKD_RAW EXPRESSION VALUE
1002 G 2473.87646 52 2421.87646 1345.91353572851
1003 L 60.64 61 -0.359999999999999 0.015694218989053
1004 L 64.46667 56 8.46667 7.41930890132592
1005 L 63.363636 48 15.363636 13.0372659435383
1006 L 69.01538 54 15.01538 12.6259541018481
1007 L 71.89474 58 13.89474 11.3653131812498
1009 G 232.4507 55 177.4507 104.921899043576
1010 G 1047.36621 63 984.36621 546.52902301392
1011 G 141.846161 63 78.846161 52.7153089430928
1012 G 152.672409 65 87.672409 56.2887426633177
1013 M 69.0344849 62 7.0344849 6.43271211267798
1014 M 86.046875 56 30.046875 23.5345927029097
1016 G 102.375 55 47.375 34.3165145798291
1017 L 73.14286 52 21.14286 17.7390513172716
1018 L 65.37079 57 8.37079 7.55972524289911
1019 L 68.98245 60 8.98245 8.01712887105954
1020 L 73.02778 59 14.02778 12.0617293593113
1021 G 1451.70374 56 1395.70374 775.059067753464
1023 G 1339.66284 54 1285.66284 712.745073064375
1024 L 61.02353 57 4.02353 4.01877701851516

Total number of rows: 53423

Table truncated, full table size 2512 Kbytes.




Supplementary file Size Download File type/resource
GSM361187.txt.gz 1.1 Mb (ftp)(http) TXT
Processed data included within Sample table

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