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I have the following problem: I have 10 different FASTA files with thousand sequences inside each file. I would like to read from each fasta file all the sequence and then (with paste) create a one big file with all the sequences.

My question is the following: how can I read from different files in the same time?

I tried:

a<-list.files()

and then

for (x in a) { temp<-read.table(x) seq<-summary(temp) print (seq)

but it doesn't work properly. I tried also the command read.fasta but it gives to me a strange output (not all the sequence)

Thank you very much for your help, it will be very appreciate!

Fabio

PS. I started to work with R just one week ago...so please, be patient even if it is a stupid question!

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if you don't get help here, maybe try your question on the Bioconductor mailing list (pointing out that you are cross-posting from StackOverflow). –  Ben Bolker Feb 17 '12 at 13:36
    
Can you successfully import a single file? Why are there no ; or new lines between commands? –  Roman Luštrik Feb 17 '12 at 14:18

1 Answer 1

Bioconductor has many packages for working with DNA sequences. Install the ShortRead package with

source("http://bioconductor.org/biocLite.R")
biocLite("ShortRead")

Load the library and consult the help page for readFasta

library(ShortRead)
?readFasta

Figure out a pattern (like list.files) that matches the fasta files you want to read in, and read all fasta files matching the pattern into a single object

patt <- "fasta$"
fasta <- readFasta("/my/directory/containing/fasta/files", patt)

Then write the object out

writeFasta(fasta, "my_destination.fasta")

But actually R would not be the right tool for just concatenating files; likely you want to do more interesting things, some of which might be described in the vignettes for ShortRead, Biostrings, and GenomicRanges

browseVignettes("ShortRead")
browseVignettes("Biostrings")
browseVignettes("GenomicRanges")

The Bioconductor mailing list is the best place to get support for Bioconductor packages.

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Thank you very much. However instead of readFasta...I used the command apply (lapply(myseqs, function(x), read.fasta(x)). –  fabioln79 Feb 21 '12 at 13:02

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