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Tested in the brain vasculome. Human plasma proteins determined by proteomics from 4 different studies were used [199,200,201,202,203,204]. A core set of human plasma proteins was build with proteins detected in all of these 4 studies, consisting of 387 individual proteins. It is worthwhile to notice that GWAS and plasma protein databases evolve and grow over the time, correlations with our brain vasculome will have to be continually re-assessed in future studies.Transcriptional Profiling with MicroarrayThree RNA samples for each organ were individually hybridized to Affymetrix GeneChip Mouse Genome 430 2.0 microarrays, after checking the RNA quantity and quality. RNA concentration was measured by Nanodrop, and the integrity of RNA was tested with RNA integrity number (RIN) score on Agilent Bioanalyzer 2010. All samples were used only when RIN scores were verified to be larger than 7.0. Microarray hybridization and scanning was performed after amplification with the NuGEN Ovation WTA Pico kit and fragmentation and labeling with Encore Biotin Module. Raw expression data for each chip was summarized and SR 3029 web normalized using RMA algorithm, to allow direct comparison of results obtained among different chips. The quality of each chip was determined by manually checking mean values, variances and paired scatter plots as well as Principal Component Analysis (PCA) plots. All chips passed the quality check. Among the large amount of probes/genes, we only focused on genes whose maximal expression values across all microarrays were great than 200, while the probes with intensity less than 200 were eliminated for further analysis.Statistical MethodsAll statistical analyses were performed with the statistics software R (Version 2.6.2; available from http://www.r-project. org) and R packages developed by the BioConductor project (available from http://www.bioconductor.org). Overall, raw expression data for each chip was summarized and normalized using RMA algorithm, genes with maximum expression levels across all microarrays great than 200 were considered for further analysis. Organ specifically expressed genes were identified using SAM algorithm; Fisher’s exact test was used to identify the enriched pathways from these organ specific genes. Only genes with 24195657 p,0.01 and fold change .4 were considered as specifically expressed. The combination of p value and fold change threshold serves to eliminate most false positives, as validated by a large microarray study led by FDA [208]. Fisher’s exact test was also used to test the enrichment of GWAS genes for each disease in the vasculome of mouse brain.Identification of Organ Specifically Expressed GenesThe specific genes between two groups were identified based on both 15826876 statistical significances, which were determined using SAM GSK -3203591 site algorithm (a variant of t-test and specifically designed for microarray data), and fold change. To minimize false positives,Mapping the Brain VasculomeSupporting InformationFigure S(XLSX)Table S3 Full list of plasma proteins expressed in brain vasculome. (XLSX)Purity of isolation protocols for brain, heart and kidney glomerular endothelial cells. The expression of different cell type specific genes were tested by RT-PCR, and compared between endothelial cells and corresponding whole tissue samples. (PDF)AcknowledgmentsThanks to Francis Luscinskas and Veronica Azcutia Criado (Brigham and Women’s Hospital and Harvard Medical School, Boston, MA) for helpful discussions about the isolation of.Tested in the brain vasculome. Human plasma proteins determined by proteomics from 4 different studies were used [199,200,201,202,203,204]. A core set of human plasma proteins was build with proteins detected in all of these 4 studies, consisting of 387 individual proteins. It is worthwhile to notice that GWAS and plasma protein databases evolve and grow over the time, correlations with our brain vasculome will have to be continually re-assessed in future studies.Transcriptional Profiling with MicroarrayThree RNA samples for each organ were individually hybridized to Affymetrix GeneChip Mouse Genome 430 2.0 microarrays, after checking the RNA quantity and quality. RNA concentration was measured by Nanodrop, and the integrity of RNA was tested with RNA integrity number (RIN) score on Agilent Bioanalyzer 2010. All samples were used only when RIN scores were verified to be larger than 7.0. Microarray hybridization and scanning was performed after amplification with the NuGEN Ovation WTA Pico kit and fragmentation and labeling with Encore Biotin Module. Raw expression data for each chip was summarized and normalized using RMA algorithm, to allow direct comparison of results obtained among different chips. The quality of each chip was determined by manually checking mean values, variances and paired scatter plots as well as Principal Component Analysis (PCA) plots. All chips passed the quality check. Among the large amount of probes/genes, we only focused on genes whose maximal expression values across all microarrays were great than 200, while the probes with intensity less than 200 were eliminated for further analysis.Statistical MethodsAll statistical analyses were performed with the statistics software R (Version 2.6.2; available from http://www.r-project. org) and R packages developed by the BioConductor project (available from http://www.bioconductor.org). Overall, raw expression data for each chip was summarized and normalized using RMA algorithm, genes with maximum expression levels across all microarrays great than 200 were considered for further analysis. Organ specifically expressed genes were identified using SAM algorithm; Fisher’s exact test was used to identify the enriched pathways from these organ specific genes. Only genes with 24195657 p,0.01 and fold change .4 were considered as specifically expressed. The combination of p value and fold change threshold serves to eliminate most false positives, as validated by a large microarray study led by FDA [208]. Fisher’s exact test was also used to test the enrichment of GWAS genes for each disease in the vasculome of mouse brain.Identification of Organ Specifically Expressed GenesThe specific genes between two groups were identified based on both 15826876 statistical significances, which were determined using SAM algorithm (a variant of t-test and specifically designed for microarray data), and fold change. To minimize false positives,Mapping the Brain VasculomeSupporting InformationFigure S(XLSX)Table S3 Full list of plasma proteins expressed in brain vasculome. (XLSX)Purity of isolation protocols for brain, heart and kidney glomerular endothelial cells. The expression of different cell type specific genes were tested by RT-PCR, and compared between endothelial cells and corresponding whole tissue samples. (PDF)AcknowledgmentsThanks to Francis Luscinskas and Veronica Azcutia Criado (Brigham and Women’s Hospital and Harvard Medical School, Boston, MA) for helpful discussions about the isolation of.

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Author: Ubiquitin Ligase- ubiquitin-ligase