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Sample GSM1110208 Query DataSets for GSM1110208
Status Public on Mar 29, 2013
Title infected human aortic endothelial cell (HAEC)
Sample type RNA
 
Channel 1
Source name HAEC stably infected with rKSHV.219
Organisms Homo sapiens; Human herpesvirus 8 strain rKSHV.219
Characteristics infection: Human herpesvirus 8 strain rKSHV.219 (infection: stable)
Growth protocol Microvascular LEC and BEC were cultured in EGM2-MV media (Lonza). Macrovascular HUVEC and HAEC were cultured in EGM2 media (Lonza). Cells stably infected with rKSHV.219 were maintained in 0.25 ug/mL puromycin (Invivogen).
Extracted molecule total RNA
Extraction protocol All samples were harvested in RLT buffer and RNA was isolated using the RNeasy Mini Kit according to the manufacturer’s protocol (Qiagen).
Label Cy5
Label protocol The Quick Amp Labeling Kit (Agilent) was used according to the manufacturer’s protocol to generate Cy5/Cy3 labeled cRNA from 450 ng of total RNA, which contains mix of spike-in transcripts A + B (Agilent). An equal amount of the spike-in transcript mix were added to both Cy5 and Cy3 labeled samples. The spike-in transcripts were detected by E1A probes on the array and used for linear normalization subsequent to the LOWESS normalization performed by the Agilent feature extraction software.
 
Channel 2
Source name Common reference: mix of several different cell types (BJAB, BCBL, iSLK, iSLK.219), both latent and lytic.
Organisms Homo sapiens; Human gammaherpesvirus 8
Characteristics common reference composition: cell type: mix of several different cell types (BJAB, BCBL, iSLK, iSLK.219); virus: HHV8 Type M (in BCBL) or HHV8 Type P (in iSLK.219); infection status: uninfected (BJAB and iSLK) or stably infected (latent & lytic BCBL and iSLK.219)
Growth protocol Microvascular LEC and BEC were cultured in EGM2-MV media (Lonza). Macrovascular HUVEC and HAEC were cultured in EGM2 media (Lonza). Cells stably infected with rKSHV.219 were maintained in 0.25 ug/mL puromycin (Invivogen).
Extracted molecule total RNA
Extraction protocol All samples were harvested in RLT buffer and RNA was isolated using the RNeasy Mini Kit according to the manufacturer’s protocol (Qiagen).
Label Cy3
Label protocol The Quick Amp Labeling Kit (Agilent) was used according to the manufacturer’s protocol to generate Cy5/Cy3 labeled cRNA from 450 ng of total RNA, which contains mix of spike-in transcripts A + B (Agilent). An equal amount of the spike-in transcript mix were added to both Cy5 and Cy3 labeled samples. The spike-in transcripts were detected by E1A probes on the array and used for linear normalization subsequent to the LOWESS normalization performed by the Agilent feature extraction software.
 
 
Hybridization protocol Samples were hybridized to the custom tiling microarrays according the manufacturer’s protocol (Agilent). Hybridized microarrays were washed according to the manufacturer’s protocol (Agilent).
Scan protocol Microarrays were scanned on the GenePix 4000B scanner (Axon instruments) and all feature intensities collected using the GenePix Pro 6.0 software.
Description inf HAEC
Biological replicate 1 of 1. All samples in Experiment 2 were processed in parallel, visualized on the same microarray on the same day, and the resulting microarray data was analyzed as one collective data set.
Data processing TIFF images of scanned slides were analyzed using Feature Extraction Software version 9.5.3 (Agilent) using a custom grid file (017577_D_F_20070822). LOWESS normalized, background subtracted data were obtained from log2 of processed Red signal/processed Green signal. Agilent software was used. Data of identical probes were averaged. Data were subjected to a further linear normalization step by the average of the features detecting the spike-in transcripts. Only features that did not have any feature non-uniformity or population outlier flags contributed to the averages used for determining the normalization factor. Removed any data that failed any of the following spot quality filters: 1. gIsFound = 1 AND rIsFound = 1; 2. no PopnOL or NonUnifOL detected; 3. g OR r IsWellAboveBackground. Data of every probe was centered to the average of the corresponding control samples. Data for host genes were removed and probes against viral sequences were ordered by position in genome.
 
Submission date Mar 28, 2013
Last update date Mar 29, 2013
Contact name Henry H Chang
E-mail(s) [email protected]
Organization name Novartis Institutes for BioMedical Research
Department Infectious Diseases Group
Street address 4560 Horton Street
City Emeryville
State/province CA
ZIP/Postal code 94608
Country USA
 
Platform ID GPL16894
Series (2)
GSE45591 Mock and stably infected rKSHV.219 cells (LEC, BEC, HUVEC, and HAEC) [Expt2]
GSE45600 A unique herpesviral transcriptional program in KSHV-infected lymphatic endothelial cells leads to mTORC1 activation and rapamycin sensitivity

Data table header descriptions
ID_REF
VALUE Normalized (linear and LOWESS) log2 ratio (Cy5/Cy3) representing test/reference

Data table
ID_REF VALUE
CUST_1_PI425407708 -0.021822886
CUST_2_PI425407708 -1.606566863
CUST_3_PI425407708 -1.748161139
CUST_4_PI425407708 -3.05659353
CUST_5_PI425407708 -3.308324537
CUST_6_PI425407708 -3.084117447
CUST_7_PI425407708 -3.42532616
CUST_8_PI425407708 -2.889404864
CUST_9_PI425407708 -3.661767403
CUST_10_PI425407708 -2.761183261
CUST_11_PI425407708 -2.918789276
CUST_12_PI425407708 -4.489415673
CUST_13_PI425407708 -4.393747359
CUST_14_PI425407708 -3.103114832
CUST_15_PI425407708 -2.498330615
CUST_16_PI425407708 -3.135574738
CUST_17_PI425407708 -4.303525802
CUST_18_PI425407708 -3.82790669
CUST_19_PI425407708 -3.70043284
CUST_20_PI425407708 -4.387968997

Total number of rows: 13484

Table truncated, full table size 449 Kbytes.




Supplementary file Size Download File type/resource
GSM1110208_inf_HAEC_raw.txt.gz 13.8 Mb (ftp)(http) TXT
Processed data included within Sample table

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