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Sample GSM1079463 Query DataSets for GSM1079463
Status Public on Feb 07, 2013
Title G5_33V0
Sample type RNA
 
Source name CAMR/TGP (C4d+/DSA+)
Organism Homo sapiens
Characteristics tissue: renal biopsy
Treatment protocol One biopsy core was collected into a vial containing 1ml of RNALater® (Ambion, Catalog Number AM7023), stored at -20°C for 24 hours, and then transferred to -70°C until RNA isolation. Renal tissue content in all cores was verified using a dissecting microscope and any non-renal tissue was removed. Total RNA was isolated using the QIAGEN Rneasy Mini Kit (Catalog Number 74104, Qiagen, USA) and was quantified using the NanoDrop 2000 (Thermo Scientific, Wilmington, Delaware). To further assess RNA quality, samples were assessed by the Agilent 2100 Bioanalyzer (Agilent Technology, Santa Clara, CA,) and samples with an RNA Integrity Number score cut off >7 were deemed suitable for Gene Chip Microarray Hybridization. The complete protocol for converting total RNA into biotin-labeled RNA by Affymetrix Human Gene 1.0 ST Array hybridization containing 28,869 gene probe sets can be found in the manufacturer¹s protocol for the Ambion Whole Transcript Expression Kit (Catalog Number 4425209, Ambion, Austin, TX) and Affymetix Gene chip Whole Transcript Terminal Labeling Kit (Catalog Number 900671, Affymetrix, Santa Clara, CA).
Extracted molecule total RNA
Extraction protocol Total RNA was isolated using the QIAGEN RNeasy Mini Kit (Catalog Number 74104, Qiagen, USA) and was quantified using the NanoDrop 2000 (Thermo Scientific, Wilmington, Delaware). To further assess RNA quality, samples were assessed by the Agilent 2100 Bioanalyzer (Agilent Technology, Santa Clara, CA,) and samples with an RNA Integrity Number score cut off >7 were deemed suitable for Gene Chip Microarray Hybridization.
Label biotin
Label protocol Follow protocols of Ambion Whole Transcript Expression Kit (Catalog Number 4425209, Ambion, Austin, TX) and Affymetix Genechip Whole Transcript Terminal Labeling Kit (Catalog Number 900671, Affymetrix, Santa Clara, CA)
 
Hybridization protocol Total RNA samples hybridized to the Affymetrix Hugene 1.0 st chip according to the protocols provided by the manufacturer.
Scan protocol Affymetrix Gene Chip 3000 7G scanner, software AGCC v2.0
Data processing The gene expression profiles of the biopsy specimens were compared according to the following groups:
Group 1: Normal transplant kidney biopsies (n=12)
Group 2: Non-specific IFTA (N=17)
Group 3: TGP DSA-/C4d- (g+ptc > 1) (N=8)
Group 4: TGP DSA+/C4d- (N=9)
Group 5: CAMR/TGP (C4d+/DSA+) (N=14)
Probe intensities were extracted from Affymetrix CEL files, normalized and summarized at the transcript cluster level using the Robust Multiarray Average method from the R/Bioconductor (http://bioconductor.org) oligo package. Array quality control was performed to remove arrays that significantly differed in initial overall probe intensity. Expression values were analyzed on the log base 2 scale. Significance testing was performed by fitting gene-wise linear models using the limma Bioconductor package, and genes were ranked for differential expression using Benjamini & Hochberg adjusted p-values and log-posterior odds of differential expression (log probability of differential expression versus probability of no differential expression). In order to obtain the Benjamini and Hochberg adjusted p-value, the false discovery rate (FDR) was set at <0.01. Gene set analysis was performed using the limma romer (Rotation Gene Set Enrichment Analysis) method. This analysis generates a p-value for enrichment of three categories of gene expression for each gene set: probability of enrichment of up-regulated and down-regulated genes, and enrichment of genes with expression level changes (P-value was set at < 0.05). Gene Set libraries were taken from the Molecular Signatures Database (MSigDB) and new libraries were generated by mapping HUGO gene identifiers to the University of Alberta, Edmonton, Pathogenesis Based Transcripts (PBT; http://transplants.med.ualberta.ca/Nephlab/data/gene_lists.html) gene sets. The following core PBT were analyzed:
* KT: Kidney specific transcripts (n=63) * IRIT: Injury and repair induced transcripts (n=228) * GRIT: Gamma-IFN and rejection induced transcripts (n=50) * QCAT: Quantitative cytotoxic T cell--associated transcripts (n=25) * CMAT: Quantitative constitutive macrophage-associated transcripts (n=72) * BAT: B cell associated transcripts (n=50) * NKAT: Natural killer cell-associated transcripts (n=244) * ENDAT: Endothelial cell associated transcripts (n=114) * DSAST: Donor Specific Antibody Selective Transcripts (n= 25) Analysis for changes in gene expression of Gene Ontology (GO) categories was performed using the GOstats Bioconductor package to calculate Hypergeomtric p-values for over or under-representation of each GO term.
 
Submission date Feb 06, 2013
Last update date Feb 07, 2013
Contact name Bin Ye
E-mail(s) bin.ye@einstein.yu.edu
Phone 718-678-1147
Organization name Albert Einstein College of Medicine
Department Genetics
Street address 1301 Morris Park Ave
City New York
State/province NY
ZIP/Postal code 10461
Country USA
 
Platform ID GPL6244
Series (1)
GSE44131 The clinical and genomic significance of donor-specific antibody (DSA) positive/C4d negative and DSA negative/C4d negative transplant glomerulopathy

Data table header descriptions
ID_REF
VALUE RMA normalized and log2 transformed intensity values

Data table
ID_REF VALUE
7896736 6.89983621232471
7896738 4.44990800229155
7896740 5.3954094579841
7896742 8.07739721230335
7896744 6.7850738564704
7896746 9.64200346891524
7896748 10.6473037997309
7896750 4.86707799731356
7896752 9.51630283118167
7896754 7.27876818910934
7896756 5.22287930359315
7896759 6.90590149657999
7896761 7.07593256985035
7896779 7.07195473332613
7896798 7.39589649101237
7896817 7.09445313342564
7896822 8.60828844650416
7896859 6.2775308732071
7896861 4.62645450504125
7896863 6.21983297005146

Total number of rows: 29096

Table truncated, full table size 707 Kbytes.




Supplementary file Size Download File type/resource
GSM1079463_EA1-HuGene-1_0-ST-9521.CEL.gz 4.2 Mb (ftp)(http) CEL
Processed data included within Sample table

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