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I have set of EST sequences in fasta file. Here, how to subset based on sequence ID or name?

>gi|296783888|gb|GW992815.1|GW992815 UAS-Mi10 Complementary DNA of mulberry (Morus indica) Morus indica cDNA 5' similar to Putative phosphoribosyltransferase/phosphoribosylanthranilate-like gene from Morus indica, mRNA sequence

>gi|296783887|gb|GW992814.1|GW992814 UAS-Mi9 Complementary DNA of mulberry (Morus indica) Morus indica cDNA 5' similar to Dehydration-responsive protein RD22, Similar to BURP domain-containing protein like gene from Morus indica, mRNA sequence

Like using header line >gi|296783888|gb|GW992815.1|GW992815 UAS-Mi10 Complementary DNA of mulberry (Morus indica) Morus indica cDNA 5' similar to Putative phosphoribosyltransferase/phosphoribosylanthranilate-like gene from Morus indica, mRNA sequence or using only >gi|296783888
How to do this in R?

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Does strsplit(text, ">gi") work? –  Scott Chamberlain Apr 19 '14 at 17:42
@ScottChamberlain: Actaully i used read.fasta function in seqinr package to read input file. As you mentioned i tried but the error is Error in strsplit(p, ">gi|296783888") : non-character argument –  ramesh Apr 19 '14 at 17:51

1 Answer 1

up vote 3 down vote accepted

For a slightly more heavy-weight solution, if this fits in to the Bioconductor work flow,


to install the Biostrings and Rsamtools package, then

indexFa("foo.fasta")   # create an index of file 'foo.fasta'
fa = FaFile("foo.fasta")  # reference the fasta file and it's index

You can discover the coordinates (names and start / end) of each sequence with

gr = as(seqinfo(fa), "GRanges")

and query for arbitrary sequences and ranges within sequences by choosing appropriate subsets, e.g., the second sequence and then first sequence in your example

getSeq(fa, gr[2:1])

or by looking up the coordinates by partial match to the names

idx = pmatch("gi|296783888", names(gr))  ## NA's if duplicates or not unique
seq = getSeq(fa, gr[idx])

"seq" is a DNAStringSet, and can be manipulated in many ways; see the vignettes available in the package


especially the Quick Overview. To save the object to a fasta file 'file.fa' in a directory 'some' relative to the current working directory, use

writeXStringSet(seq, "some/file.fa")
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Thanks a lot, your answer helped me lot.... –  ramesh Apr 19 '14 at 18:06
I tried your suggestions, it worked for my sample files, when i moved to larger files, I got the following error Warning messages: 1: In doTryCatch(return(expr), name, parentenv, handler) : [fai_build_core] different line length in sequence 'LA11031.CleanEST.seq.Contig60'. 2: In doTryCatch(return(expr), name, parentenv, handler) : [fai_load] fail to open FASTA index. Error in indexFa(open(FaFile(file))) : error in evaluating the argument 'file' in selecting a method for function 'indexFa': Error in value[[3L]](cond) : 'open' index failed file: mulberry.fasta. –  ramesh Apr 21 '14 at 6:19
I found out, when extra empty line is added after sequences, I am getting this warning. How to format and remove these empty lines automatically in multi-fasta file? –  ramesh Apr 21 '14 at 6:26
Maybe an easy way to correctly format the input is to read the entire file dna = Biostrings::readDNAStringSet("tmp.fa") then write it out again Biostrings::writeXStringSet(dna, "tmp1.fa"); "tmp1.fa" is then correctly formatted for indexing. –  Martin Morgan Apr 21 '14 at 6:41
@gunzapper Yes, add the argument as="AAStringSet" to getSeq(). Also use Biostrings::readAAStringSet(). –  Martin Morgan Dec 11 '14 at 13:13

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