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Sample GSM832212 Query DataSets for GSM832212
Status Public on Aug 13, 2013
Title Low2, HP4
Sample type RNA
 
Source name Liver Hepatic Parenchyma
Organism Homo sapiens
Characteristics ishak fibrosis: 0
gender: Female
race: Black
age: 39
Treatment protocol H&E and trichrome stained sections were then graded and staged (Ishak fibrosis and Metavir) by a hepatopathologist who was blinded to all clinical information.
Growth protocol Tissues were divided into two at the time of biopsy. One piece was immediately placed in OCT and snap-frozen in liquid nitrogen.
Extracted molecule total RNA
Extraction protocol RNA was extracted and isolated from each sample separately using the Agencourt® RNAdvance Cell v2 system (Beckman Coulter Genomics, Danvers, MA); this extraction platform relies on paramagnetic bead purification of nucleic acids. It was linearly amplified using the NuGEN Ovation Pico WTA (linear amplification) System® (NuGEN Technologies, Inc., San Carlos, CA)
Label biotin
Label protocol One ug total RNA was combined with 2 ul T7 oligo(dT) primer and 2 ul Poly-A controls and brought to a volume of 12 ul. The samples were incubated at 70ºC for 10 minutes. A master mix of 4 ul first strand buffer, 2 ul DTT and 1 ul 10 mM dNTPs was added to the samples, followed by a two minute incubation at 42ºC. One ul Superscript II (Invitrogen, Carlsbad, CA) was added to each sample and the samples were incubated at 42ºC for one hour for first strand cDNA synthesis. A master mix of 91 ul water, 30 ul 5X second strand buffer, 3 ul 10 mM dNTPs, 4 ul DNA polymerase I, 1 ul E.coli DNA ligase, and 1 ul RNase H was added to each sample and the samples were incubated for two hours at 16ºC for second strand cDNA synthesis. Two ul of T4 DNA polymerase was added followed by a five minute incubation at 16ºC. Ten ul, 0.5 M EDTA was added to stop the reaction. cDNA clean-up was performed with the Affymetrix GeneChip Sample Clean-up Module, as per manufacturer’s instructions. The cDNA was eluted in 14 ul elution buffer. The final elution volume (~12ul) was combined with 28 ul of IVT mix master mix (4 ul 10X IVT labeling buffer, 12 ul Labeling NTP mix, 4 ul labeling enzyme mix, and 8 ul RNAse-free water) for the in vitro transcription cRNA synthesis reaction. The samples were incubated overnight for 16 hours at 37ºC followed by a hold at 4ºC. Clean-up was performed as per the manufacturer’s protocol using the Affymetrix GeneChip Sample Clean-up Module. The final elution volume was ~19ul. Concentration was checked via a nanodrop spectrophotometer. Six ul 5X fragmentation buffer was then combined with 15 ug cRNA and incubated at 95ºC for 35 minutes to fragment the cRN
 
Hybridization protocol The samples were ice quenched and combined with the hybridization cocktail (5 ul oligonucleotide B2 control, 15 ul 20X eukaryotic hybridization controls, 150 ul 2X hybridization buffer, 30 ul 100% DMSO and 70 ul water). After 10 minutes of pre-hybridizing Human U133 Plus 2.0 Genome array at 45ºC, 60 rpm, 200 ul of cocktail was loaded onto each array and the arrays were hybridized for 16 hours at 45ºC, 60 rpm. The cocktail was removed and the arrays were stained and washed using the Affymetrix GeneChip Fluidics Station 450 and FS450_001 fluidics script.
Scan protocol All arrays were scanned in the Affymetrix GeneChip Scanner 3000 and the raw analysis was performed with Affymetrix GeneChip Operating System (GCOS) 1.4.
Data processing Results from microarray hybridization were analyzed using the Bioconductor package in R. Data were normalized with the “rma” procedure using a custom HGU133Plus2 annotation, to avoid known problems associated with the affymetrix annotation -. The normalized data was then analyzed using the “affy” -and “limma” -packages in Bioconductor.
 
Submission date Nov 12, 2011
Last update date Aug 13, 2013
Contact name Supriya Munshaw
E-mail(s) smunsha1@jhmi.edu
Organization name Johns Hopkins University
Department Medicine
Lab Viral Hepatitis Center
Street address 855 N. Wolfe St, Suite 530
City Baltimore
ZIP/Postal code 21205
Country USA
 
Platform ID GPL14877
Series (1)
GSE33650 Gene Expression differences in Hepatic Parenchyma and Portal Tracts in Hepatitis C Virus Infected Subjects with High and Low Fibrosis

Data table header descriptions
ID_REF
VALUE RMA

Data table
ID_REF VALUE
100009676_at 4.714112371
10000_at 3.933618113
10001_at 4.118236048
10002_at 4.975402065
10003_at 3.546394599
100048912_at 4.891111452
100049716_at 4.244731412
10004_at 4.665444819
10005_at 4.526293774
10006_at 8.768809897
10007_at 4.83213957
10008_at 4.346925474
100093630_at 6.370951179
10009_at 3.419181469
1000_at 6.736380673
100101938_at 5.073662469
10010_at 5.719053987
100113407_at 2.933320961
10011_at 7.543014254
100124700_at 3.511712392

Total number of rows: 18123

Table truncated, full table size 367 Kbytes.




Supplementary file Size Download File type/resource
GSM832212_Low2_6.CEL.gz 3.9 Mb (ftp)(http) CEL
Processed data included within Sample table
Processed data are available on Series record

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