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mkatari-bioinformatics-august-2013-deseq [2015/06/17 08:19] mkatarimkatari-bioinformatics-august-2013-deseq [2015/08/21 14:13] (current) mkatari
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 Then we will load the experimental design. An example is provided [[https://docs.google.com/file/d/0B172nc4dAaaOaE5fTVVhUHJKazg/edit?usp=sharing|here]]: Then we will load the experimental design. An example is provided [[https://docs.google.com/file/d/0B172nc4dAaaOaE5fTVVhUHJKazg/edit?usp=sharing|here]]:
 <code> <code>
-expdesign = read.table(pathToExpDesign)+expdesign = read.table("expdesign.txt")
 </code> </code>
  
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 An important part of DESeq is to estimate dispersion. This is simply a form of variance for the genes. An important part of DESeq is to estimate dispersion. This is simply a form of variance for the genes.
 <code> <code>
 +# if you have replicates do the following:
 cds = estimateDispersions( cds ) cds = estimateDispersions( cds )
 +### HOWEVER, If you have NO replicates, then try this
 +cds = estimateDispersions( cds, method="blind" , sharingMode = "fit-only" )
 </code> </code>
  
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 #To get the genes that have FDR of 10% and save it in the output directory. #To get the genes that have FDR of 10% and save it in the output directory.
 <code> <code>
-resSig = res[ which(res$padj < 0.1), ]+resSigind = res[ which(res$padj < 0.1 & res$log2FoldChange > 1), ] 
 +resSigrep = res[ which(res$padj < 0.1 & res$log2FoldChange < -1), ]
  
-outfile = "Deseq.results.txt" +indoutfile = "Deseq.indresults.txt"  
 +repoutfile = "Deseq.represults.txt" 
  
-write.table(resSig,  +write.table(resSigind,  
-            outfile+            indoutfile,  
 +            sep="\t",  
 +            col.names=T,  
 +            row.names=F, 
 +            quote=F) 
 + 
 +write.table(resSigrep,  
 +            repoutfile
             sep="\t",              sep="\t", 
             col.names=T,              col.names=T, 
mkatari-bioinformatics-august-2013-deseq.1434529157.txt.gz · Last modified: 2015/06/17 08:19 by mkatari