Entering edit mode
10.5 years ago
hoangtv
▴
30
Hi, Could anyone please help me to solve the problem with making an ExonCountSet? I am new to R, so I am struggling now. I counted the 6 SAM files from GSNAP output using dexseq_count.py by following DEXSeq manual, then I made sample table. Here is what I did:
>sampleTable <- data.frame(row.names = c( "E1", "E2", "E3","F1", "F2", "F3" ), countFile = c( "E1.count", "E2.count", "E3.count", "F1.counts","F2.count", "F3.count" ), condition = c( "E", "E", "E", "F", "F", "F" ))
>sampleTable
countFile condition
E1 E1.count E
E2 E2.count E
E3 E3.count E
F1 F1.counts F
F2 F2.count F
F3 F3.count F
>ecs <-read.HTSeqCounts(sampleTable$countFile,sampleTable,"protein_coding_flattened.gff")
Error in read.table(x, header = FALSE, stringsAsFactors = FALSE) :
'file' must be a character string or connection*
Thank you very much Thanh
If you type
list.files(), do E1.count and the other files show up? Also, I suspect thatF1.countsshould beF1.count.Hi dpryan79, Thank you very much for your quick reply. The F1.counts is just the typo in previous message, sorry about that. Just note that I installed HTseq , flattened the annotation gtf file and did the counting in a different machine and then move data over to another one to process in R. I typed list.files(). All files seem to show up:
What is the output of
class(sampleTable$countFile)? The common cause of this is that it's not a character vector.Just to keep everyone in the loop, Alejandro Reyes (one of the DEXSeq authors) saw this same thread over on seqanswers. The
read.HTSeqCounts()function (and vignette) will get tweaked to avoid this error in the future. It's always a good sign with the authors of tools follow these sites and respond when there are issues!