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I have a script that performs BLAST queries (bl2seq)

The script works like this:

  1. Get sequence a, sequence b
  2. write sequence a to filea
  3. write sequence b to fileb
  4. run command 'bl2seq -i filea -j fileb -n blastn'
  5. get output from STDOUT, parse
  6. repeat 20 million times

The program bl2seq does not support piping. Is there any way to do this and avoid writing/reading to the harddrive?

I'm using Python BTW.

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+1 @Austin, this is a good question. I was looking for something similar (15 million queries to balstall - a command from Blast2 as well) and got here by Google'ing. Please consider re-asking on biostars.org –  Aleksandr Levchuk Apr 23 '11 at 0:27

5 Answers 5

up vote 1 down vote accepted

How do you know bl2seq does not support piping.? By the way, pipes is an OS feature, not the program. If your bl2seq program outputs something, whether to STDOUT or to a file, you should be able to parse the output. Check the help file of bl2seq for options to output to file as well, eg -o option. Then you can parse the file.

Also, since you are using Python, an alternative you can use is BioPython module.

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It's certainly up to the program whether it reads anything from standard input. Just because you can pipe something to STDIN doesn't mean the program will do anything with it. –  cjm Feb 12 '10 at 1:47
    
who says anything about STDIN. I am asking OP about STDOUT. –  ghostdog74 Feb 12 '10 at 1:51
    
I can parse the output just fine as it's going to STDOUT. @cjn - How would I pipe to two arguments? bl2seq -i <pipe1> -j <pipe2> –  Austin Feb 12 '10 at 3:15
    
@ghostdog75 you deserve credit for answering this. I didn't really understand what you meant at the time. –  Austin May 6 '10 at 20:00

Depending on what OS you're running on, you may be able to use something like bash's process substitution. I'm not sure how you'd set that up in Python, but you're basically using a named pipe (or named file descriptor). That won't work if bl2seq tries to seek within the files, but it should work if it just reads them sequentially.

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Hey, that worked! You're rad bl2seq -i<(echo sequence1) -j(echo sequence2) -p blastn –  Austin Feb 12 '10 at 3:26

Is this the bl2seq program from BioPerl? If so, it doesn't look like you can do piping to it. You can, however, code your own hack using Bio::Tools::Run::AnalysisFactory::Pise, which is the recommended way of going about it. You'd have to do it in Perl, though.

If this is a different bl2seq, then disregard the message. In any case, you should probably provide some more detail.

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It's the bl2seq program that comes with NCBI's Blast+. The BioPerl bl2seq is a wrapper of some sort. –  Austin Feb 12 '10 at 3:13

Wow. I have it figured out.

The answer is to use python's subprocess module and pipes!

EDIT: forgot to mention that I'm using blast2 which does support piping.

(this is part of a class)

def _query(self):
    from subprocess import Popen, PIPE, STDOUT
    pipe = Popen([BLAST,
    '-p', 'blastn',
    '-d', self.database,
    '-m', '8'],
    stdin=PIPE,
    stdout=PIPE)
    pipe.stdin.write('%s\n' % self.sequence)
    print pipe.communicate()[0]

where self.database is a string containing the database filename, ie 'nt.fa' self.sequence is a string containing the query sequence

This prints the output to the screen but you can easily just parse it. No slow disk I/O. No slow XML parsing. I'm going to write a module for this and put it on github.

Also, I haven't gotten this far yet but I think you can do multiple queries so that the blast database does not need to be read and loaded into RAM for each query.

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I call blast2 using R script:

....
system("mkfifo seq1")
system("mkfifo seq2")
system("echo  sequence1 > seq1"), wait = FALSE)
system("echo  sequence2 > seq2"), wait = FALSE)
system("blast2 -p blastp -i seq1 -j seq2 -m 8", intern = TRUE)
....

This is 2 times slower(!) vs. writing and reading from hard drive!

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Ha! I appreciate your anti-answer. –  Austin Jul 2 '10 at 1:55

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