Stack Overflow is a community of 4.7 million programmers, just like you, helping each other.

Join them; it only takes a minute:

Sign up
Join the Stack Overflow community to:
  1. Ask programming questions
  2. Answer and help your peers
  3. Get recognized for your expertise

I have a multi fasta file, from which I need to extract the bases ranging 100-200, including their corresponding headers. I know that 'cut -c 100-200' can do it without having their corresponding headers. Is there any way to do this in Perl or bash ??

Example file:

8YS68_00009_00025 GAGTTTGATCCTGGCTCAGAGCGAACGCTGGCGGCAGGCTTAACACATGCAAGTCGAGCGGGCGTAGCAATACGTCAGCGGCAGACGGGTGAGTAACGCGTGGGAACATACCTTTTGGTTCGGAACAACACAGGGAAACTTGTGCTAATACCGGATAAGCTACGGGAAGATT 8YS68_00009_00027 GAGTTTGATCATGGCTCAGAGCGAACGCTGGCGGCAGGCCTAACACATGCAAGTCGAGCGCCGTAGCAATACGGAGCGGCAGACGGGTGAGTAACGCGTGGGAACGTACCTTTCGGTTCGGAATAACTCAGGGAAACTTGAGCTAATACCGAATACGTCCGTAAGGAGAAAGATTTATCGCCGAAAGATCGGCCCGCGTAAGATTAGCTAGTTGGTGAGGTAAGGCTCACCAAGCGACGATCGTTAGCTTGTC 8YS68_00012_00035 GAGTTTGATCATGGCTCAGAACGAACGTTGGCGGCGTGGATTAGGCATGCAAGTCGAACGAATCCCATCTGGGTAACTGGGTGGGGGAAGTGGCGAAAGGGGCAGTAATGCGTGGGTAACCTACCTGGGGACCGGGATAGCCTCCTAACGGATGGGTAATACCGGATACGACCTTCGGAGGCATCTCCTGAAGG

Desired output: seq id ------ATCGATCGATCG-----

seq id ------ATCGATCGATCG-----

seq id ------ATCGATCGATCG-----

Which means, I want to exactly extract the bases between 100-200 of each sequences, along with their headers. If a sequence is shorter than 100 bp, then ignore it.

share|improve this question
    
Can you give a short input/desired output sample? – Adrian Frühwirth May 13 '13 at 12:32
    
That is not FASTA format. If your data is actually missing the ">" in front of the identifier then none of the approaches below will work. – SES May 14 '13 at 13:35

Using Bio::SeqIO, the following code will extract from 100 to 200 and print the headers.

#!/usr/bin/perl 
use strict; 
use warnings;
use Bio::SeqIO;

my $in_file = "fasta_dat.txt"; 

my $in = Bio::SeqIO->new (-file=> $in_file, -format=>'fasta');
my $out = Bio::SeqIO->new( -file   => '>test.fasta',
                           -format => 'fasta');


while(my $seq = $in->next_seq() ) {
    my $subseq = $seq->trunc(100, 200);
    $out->write_seq($subseq);
}

Update: or just adopt choroba's solution here

share|improve this answer

Maybe you can make use of the following python script :

    import sys,re
    i,list1 =0,[]
    for line in open(sys.argv[1]):
      if re.match(r'^[>|;]',line):  print line,
      else:
        for x in line:
          if x != "\n": i+=1
          if 100 < i < 200: list1.append(x)
    print "".join(list1)
share|improve this answer

If your desired output is another multi-fasta file, all you need is a little awk. Simply substring what you want.

awk '!/^>/ { print substr($0, 100, 100); next }1' file.fa

The 1 on the end returns true, enabling default printing of all lines in the file. The rest should be self explanatory. HTH.


A guess:

awk '/^>/ { h = $0; getline; print h RS substr($0, 100, 100) }' file.fa

or without getline:

awk '/^>/ { h = $0; next } h { print h RS substr($0, 100, 100); h = "" }' file.fa
share|improve this answer
    
Thanks Steve. Unfortunately, this gives the header of non-sequnces as well; the header is printed even if there are no corresponding sequences. How to tackle this ? – Ronn May 13 '13 at 13:20
    
I thought you said you had a multi-fasta file? You will need to define non-sequence. As per the comments above, please edit your question to include example data and expected output. – Steve May 13 '13 at 13:32
up vote 0 down vote accepted

After reviewing the suggestions and working for sometime with this problem, I found a solution in Perl. Here is the important "loop" which does the job in Perl, which I wrote.

my $seq  = '';
my $head ;

while (my $seq = <IN>) {
if ($seq =~ m/^>/){
    $head = $seq;
    }
    else{
    my $dna .=$seq;
    my $subseq = substr ($seq, 100, 100);
    my $size = length($subseq);
    if ($size > 99){
        print OUT "$head";
        print OUT "$subseq";
        } 
  }

}

Thank you all for the help and support.

share|improve this answer

Your Answer

 
discard

By posting your answer, you agree to the privacy policy and terms of service.

Not the answer you're looking for? Browse other questions tagged or ask your own question.