Make A Custom Blast Library Using The Output Of Another Blast Result
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13.0 years ago
Zach Powers ▴ 340

Hi Biostar,

I am working on a microbial gene annotation project and I am interested in taking a large number of sequences (say 20,000) and blasting them against the NR database. However, even with a local copy of nr and a decent computer this will take forever (days, anyway). My sequences, however, are not random so I wanted to make a subset of NR that will allow me to perform a much faster BLAST query.

My sequences are 454 reads of PCR amplicons made with highly degenerate primers targeting a family of proteins so what I would like to do is as follows:

  1. Blast a set of known sequences against nr.
  2. Take the hits from this query and use the hits to make a new blastdb
  3. Blast thousands of sequences against this smaller dataset and enjoy the massive speed gains.

So before reinventing the wheel, I was wondering if there is a trivially easy way to do this that someone knows about, or has done. In the meantime I will try writing a biopython script to run the blast and to use the 'gi' and 'sseqids' of the hits to make a new fasta file.

thanks, zach cp

blast makeblastdb ncbi • 6.7k views
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In step 2 "take those sequences", you mean take the hits to those sequences? Otherwise the procedure doesn't make sense.

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@neilfws - yes thats what I mean. corrected. thanks

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13.0 years ago
Sujai Kumar ▴ 270

No need for a python script. The command line is your friend.

Assuming your initial sequences are in known_sequences.fa, first do the blastx against a local copy of nr (add your favourite blastx parameters) using the blast+ toolkit:

blastx -query known_sequences.fa -db nr -outfmt 6 >known_sequences.blastx.nr.hits.txt

Then, extract the GIs from the second column of the hits file:

cut -f2 known_sequences.blastx.nr.hits.txt | cut -f2 -d "|" >known_sequences.blastx.nr.gids.txt

Then make a blastdb using blastdb_aliastool:

blastdb_aliastool -dbtype prot -gilist known_sequences.blastx.nr.gids.txt -db nr -out nr_subset
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Sujai just a tip, to extract the GI's instead of using two cut commands you could simply use awk:

 "awk -F"|" '{print $2}' known_sequences.blastx.nr.hits.txt > known_sequences.blastx.nr.gids.txt

Learning just the basics about awk or sed can really save quite some time on the long run.

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nice Sujal, Thanks! I will ty this. One downside ( i will check) of using the GIs is that many of the blast queries hit back large sequences (whole genomes, ESTs) but I think the speed gains will still be awesome ---- time to give it a go.

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I think you should consider ALchEmiXt's broader suggestions though - a taxon restricted database is more general than just picking the ones your sequences hit.

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Agreed, I was just being lazy ;-)

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13.0 years ago
ALchEmiXt ★ 1.9k

If you are interested in just a specific taxon you could limit your BLAST searches by taxonid. Furthermore the blast+ utilities will allow you to generate a subset multiFasta or DB from a list of gi's. More specifically the BLASTDBCMD command.

So there are several ways to go with this;

  1. Limit blast to taxon-group
  2. after gi extraction make a blastDB subset using blastdbcmd command
  3. or usig your gi list retrieve all relevant sequences using Entrez online and use the multi-fasta as input DB in blast+ (it can do that) or convert it into a blastDB.
  4. probably some more ways. Also depends on how often you want to update the subsets.
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In a completely different application, I need to limit my BLAST results to a particular taxon---say, danio rerio. How do I do this from the command line for the c++ version of blastn?

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Oh, found it.

Search the Entrez Protein database (or Nucleotide, etc) with query: "txid7742[ORGN]" or "danio rerio[orgn]

Select "Send to File" and choose format "GI list"

Then, for blastn, us -gilist <file>.

I figured this out from the following thread.

http://www.biostars.org/post/show/6528/vertebrate-subset-nr-database-build-my-own/

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