I have some txt files that look like this (they contain DNA sequences and sample codes):


I would like to remove the first 15 characters of every other line in the file. This would remove the string GACTACACGTAGTAT from the second, fourth, sixth, eighth lines (etc).

For instance the cut command can remove the first 15characters of every line:

cut -c 1-15 /path/to/file.txt

I'd like to apply to to only every other line, starting with the second.

  • 2
    Please post the code for what you have tried, and what happens when you run your code. – Greg Hewgill May 13 '15 at 22:15
  • use Biopython or Bioperl or Biojava or BioETC for parse the falta, it 's two line of code ......... – Jose Ricardo Bustos M. May 13 '15 at 22:19
  • @JoseRicardoBustosM. i'd rather find a solution that doess not involve installing one of these packages as there is probably a solution using the base terminal commands. – colin May 13 '15 at 22:23
  • you need truncate, both fasta and qual files – Jose Ricardo Bustos M. May 13 '15 at 22:23
  • 1
    @colin, will you please address the comment made by Jose Ricardo Bustos M. re: "in the FASTA format , it isn't always one line of header and then one line of sequence ..." and is this applicable to your situation? Because if it's so than any solution that's coded to explicitly skip every other line can fail! – user3439894 May 14 '15 at 13:58
up vote 5 down vote accepted

If you don't mind using sedand assuming other line starts with > then the following will remove the first 15 contiguous uppercase characters "A-Z" of the other lines:

sed 's/^[A-Z]\{15\}//' file > new_file

Or, in place edit (GNU sed) use -i:

sed -i 's/^[A-Z]\{15\}//' file

Or, in place edit (BSD sed) use -i '':

sed -i '' 's/^[A-Z]\{15\}//' file

Or, back it up:

sed -i.bak 's/^[A-Z]\{15\}//' file


$ cat file
$ sed 's/^[A-Z]\{15\}//' file
  • is there a way to do this so that I don't have to actually enter the sequence being removed, and instead it just removes the first 15 characters, regardless of what they are? Often what needs to be removed is the first 15 characters, but not necessarily GACTACACGTAGTAT – colin May 13 '15 at 23:17
  • @colin Are all the lines starting with > always less then 15 characters? If they are you can use the following: sed 's/^.\{15\}//' file – user3439894 May 13 '15 at 23:28
  • unfortunately the lines with the > at the beginning can get up at 17+ characters. – colin May 13 '15 at 23:35
  • 1
    @colin Assuming every other line starts with > then the following will remove the first 15 uppercase characters "A-Z" of the other lines: sed 's/^[A-Z]\{15\}//' file – user3439894 May 13 '15 at 23:47
  • 1
    @colin try: sed 's/^[A-Z]\{3\}//' file – user3439894 May 14 '15 at 16:18

You can try

sed '0~2s/^.\{15\}//g' filename

0~2 takes every 2nd line


looks for the first 15 characters

The sed command replaces them with nothing!

  • This generates the following error: sed: 1: "0~2s/^.\{15\}//g": invalid command code ~ – colin May 14 '15 at 16:13
  • Which flavour of unix are you using? More over it could be a copy paste eror. Try using the Tilde symbol while writing the code! It worked perfectly fine for me! – Dipak May 14 '15 at 17:35
  • I'm using terminal on mac osx- just entered the code by hand into terminal, i still get the same error: sed: 1: "0~2/^.\{15\}//g": invalid command code ~, which is a bummer because your code seems like it would generalize to the most situations! – colin May 14 '15 at 17:44
  • 1
    @colin, OS X uses BSD sed and it doesn't support the ~ in the 0~2s portion of the sed instruction presented by Dipak although the GNU sed does. The sed command I provided you does not need to use that paradigm and will not touch the header lines as they have numeric characters in them and the sed instruction I've provided can only remove the first 15 contiguous uppercase alpha characters from lines starting with an uppercase alpha character, so there is no need to instruct sed to skip lines. – user3439894 May 14 '15 at 19:49
  • Again, consider checking how to format your answer. Use the {} button to print code. – fedorqui May 15 '15 at 12:26

The following script might help you, it takes two arguments: 1. Original file (from which to make a conversion) 2. File where to save results.

# call this script and pass two arguments:
# ./script FROM_FILE TO_FILE

while IFS=$'\n' read line; do
    # skip 2,4,6, ..., nth lines 
    [ $((i % 2)) -eq 0 ] && (echo -n $line >> $TO; continue);
    echo ${line:15} >> $TO
done < $FROM
  • While it does remove the first 15 characters of every other line in the file it also removes the entire every other line starting with the first line too! – user3439894 May 13 '15 at 22:59
  • Now it outputs nothing! Test your code before you post it! – user3439894 May 13 '15 at 23:02
  • You're absolutely right - my fault. Try again, dear. – Haodemon May 13 '15 at 23:04
  • 1
    I strongly suggest you reread what colin wants... "I would like to remove the first 15 characters of every other line in the file. This would remove the string GACTACACGTAGTAT from the second, fourth, sixth, eighth lines (etc)." – user3439894 May 13 '15 at 23:05
  • The solution you proposed would only work if colin has file filled with the same strings. He could have very well used a simple text editor to fix that ;) And yet, I find your solution elegant and smart. – Haodemon May 13 '15 at 23:18

you need erase first bases of file fasta and qual for analysis, while i find a solution with QIIME, a solution using python and biopython:

from Bio import SeqIO

file_fasta = open("test.fasta")
file_qual = open("test.qual")

iterator_fasta = SeqIO.parse(file_fasta, "fasta")
iterator_qual = SeqIO.parse(file_qual, "qual")

size_trim = 15

output_fasta = open("trim.fasta","w")
for seq in iterator_fasta:
  if len(seq) <= size_trim:
    raise NameError('len seq less or equal than trim size')
  seq.seq = seq.seq[size_trim:]


output_qual = open("trim.qual","w")
for seq_qual in iterator_qual:
  if len(seq_qual.letter_annotations['phred_quality']) <= size_trim:
    raise NameError('len qual less or equal than trim size')
  seq_qual.letter_annotations['phred_quality'] = seq_qual.letter_annotations['phred_quality']


you get in trim.fasta



using qiime, I recommend to use split_libraries, it does the trim and check the quality .... truncate_fasta_qual_files.py only select first B bases, trim last base doing otherwise to expected.

  • you should remove ambiguities also – Jose Ricardo Bustos M. May 13 '15 at 23:55
  • @colin using qiime exist split_libraries, this script does the trim – Jose Ricardo Bustos M. May 14 '15 at 0:09
  • it does not trim the first n bases in split_libraries- it can only remove known sequences, like your barcodes for instance. I will look into truncate_fasta_qual_files.py. Please elaborate on what you mean by "you should remove ambiguities also". – colin May 14 '15 at 14:12
  • @colin deleted N's at the end – Jose Ricardo Bustos M. May 14 '15 at 14:18

A one-liner alternative to sed is awk.

Given an alternating-lined-element FASTA file called foo.fa, you can strip the first 15 characters of the sequence strings with substr():

$ awk '/^#/ {next} /^>/ { print $0 } /^[^>]/ { print substr($0, 16, length($0) - 15) }' foo.fa > foo.filtered.fa

As awk uses 1-based indexing, the start position argument in substr() is 16.

In addition to offering code to process alternating lines separately, another advantage of awk is that it can sometimes run faster than sed. Yet another advantage is portability, given differences in sed between common bioinformatics platforms.

So if you plan on doing this a lot or on "whole genome"-scale files, you might investigate this approach, as well.

  • Alex, could you please explain a bit, what your one-liner is doing? – user3439894 May 14 '15 at 21:46
  • The /^#/ {next} directive applies two different code blocks on the specified regular expression patterns ^> and ^[^>], which represent header and sequence lines in an alternating-line FASTA file, respectively. The ^> block simply prints the header line ($0), while the ^[^>] block prints the substring of the sequence line (again, $0) with a start parameter of 15 and a length parameter of the line length, minus 14. This effectively strips the first 15 characters, whatever they are. – Alex Reynolds May 14 '15 at 22:03
  • Sorry, I made an off-by-one error. The correct start index is 16, not 15. – Alex Reynolds May 14 '15 at 22:10

Use regular expressions and either perl or awk,

perl (write a script, and expand it to detect other regular expressions,

my $pattern=$ARGV[1]||"GACTACACGTAGT";
#provide any gene sequence prefix, and pattern removes that prefix
while (<>) {
    #explicit check for non-gene/header pattern
    if( $_ =~ /^[\>\;]/ ) {
        print $_;
    #check for the specific header pattern provided, for example
    elsif( $_ =~ /^SRR1502445/ ) {
        print $_;
    #check for the gene pattern given
    elsif( $_ =~ /^$pattern(.*)/ ) {
        print "$1\n";
    else {
        print $_;

perl -lane,

perl -lane 'if( $_ =~ /^GACTACACGTAGT(.*)/ ) {print "$1\n";} else {print $_; }'


/SRR1502445/ { print $0; }
/^GACTACACGTAGTAT/ { print substr($0,16); }

Works on any linux/unix box, and cygwin also.

The file format seems to be FASTA, which is described here FASTA Specification

  • 1
    You should see the first comment colin made on my answer. The first 15 characters will not always be "GACTACACGTAGTAT" so your answer is in the same boat my first was. – user3439894 May 13 '15 at 23:57
  • in the FASTA format , it isn't always one line of header and then one line of sequence , usually there are several lines of sequence, and OP needs only delete first 15 letter in several lines of sequence – Jose Ricardo Bustos M. May 14 '15 at 0:56
  • The OP Asked for a solution which would remove the first 15 characters from every other line - which from your comments suggests incomplete knowledge of the file format. However, the solution I have offered uses regular expressions, and will solve both the problem as stated, and the more general problem, of how to recognize the gene pattern versus the header pattern (at least for the perl script version). – ChuckCottrill May 15 '15 at 1:02
  • @ChuckCottrill, I think maybe you have misunderstood and or have not followed all the relevant comments. The header row can be different lengths and values and DNS sequences too that will not be the same 15 characters as in the sample. Also the perl script you posted has else if in it and isn't that supposed to be elsif? I ask because the script as written throws errors there. Additionally in the perl -lane line you have {print "$1\n";} and shouldn't that just be {print "$1";}? Otherwise it's inserting a blank like after every DNS sequence and that's not shown that way in the OP. – user3439894 May 15 '15 at 2:27

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