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Hi all,
I have the n-th problem with blast. This time it's blastn that is destroying my days..
I use the blast+ (ncbi-blast-2.2.27+).
I simply have downloaded an RFAM db and used makeblastd on it:
with this command:
../ncbi-blast-2.2.27+/bin/makeblastdb -in rRNA.fa -dbtype 'nucl'
and this output:
Building a new DB, current time: 10/03/2012 11:30:22
New DB name: rRNA.fa
New DB title: rRNA.fa
Sequence type: Nucleotide
Keep Linkouts: T
Keep MBits: T
Maximum file size: 1000000000B
Ignoring sequence 'lcl|149850' as it has no sequence data
Adding sequences from FASTA; added 153329 sequences in 12.7754 seconds.
So I created a nucleotide database for use with my fasta file. Queries are ATGC type.
Then I run the blastn command on a file with 100 sequences:
../ncbi-blast-2.2.27+/bin/blastn -query longTestSeq.fasta -db data/rRNA.fa -out outBlastn100s
And this is part of the outputfile:
BLASTN 2.2.27+
Reference: Zheng Zhang, Scott Schwartz, Lukas Wagner, and Webb
Miller (2000), "A greedy algorithm for aligning DNA sequences", J
Comput Biol 2000; 7(1-2):203-14.
Database: rRNA.fa
153,329 sequences; 77,423,059 total letters
Query= comp173253_c0_seq1
Length=1717
***** No hits found *****
Lambda K H
1.33 0.621 1.12
Gapped
Lambda K H
1.28 0.460 0.850
Effective search space used: 123848567440
Query= comp174620_c0_seq1
Length=1566
***** No hits found *****
Lambda K H
1.33 0.621 1.12
Gapped
Lambda K H
1.28 0.460 0.850
Effective search space used: 113092217700
............and a lot of other NO HITS FOUND.
Why this happens?
I'm almost sure to have used the correct nucleotide database and queries. If you want I can cut and paste some of the sequences for each of them.
Please help me!
Thanks
I have the n-th problem with blast. This time it's blastn that is destroying my days..
I use the blast+ (ncbi-blast-2.2.27+).
I simply have downloaded an RFAM db and used makeblastd on it:
with this command:
../ncbi-blast-2.2.27+/bin/makeblastdb -in rRNA.fa -dbtype 'nucl'
and this output:
Building a new DB, current time: 10/03/2012 11:30:22
New DB name: rRNA.fa
New DB title: rRNA.fa
Sequence type: Nucleotide
Keep Linkouts: T
Keep MBits: T
Maximum file size: 1000000000B
Ignoring sequence 'lcl|149850' as it has no sequence data
Adding sequences from FASTA; added 153329 sequences in 12.7754 seconds.
So I created a nucleotide database for use with my fasta file. Queries are ATGC type.
Then I run the blastn command on a file with 100 sequences:
../ncbi-blast-2.2.27+/bin/blastn -query longTestSeq.fasta -db data/rRNA.fa -out outBlastn100s
And this is part of the outputfile:
BLASTN 2.2.27+
Reference: Zheng Zhang, Scott Schwartz, Lukas Wagner, and Webb
Miller (2000), "A greedy algorithm for aligning DNA sequences", J
Comput Biol 2000; 7(1-2):203-14.
Database: rRNA.fa
153,329 sequences; 77,423,059 total letters
Query= comp173253_c0_seq1
Length=1717
***** No hits found *****
Lambda K H
1.33 0.621 1.12
Gapped
Lambda K H
1.28 0.460 0.850
Effective search space used: 123848567440
Query= comp174620_c0_seq1
Length=1566
***** No hits found *****
Lambda K H
1.33 0.621 1.12
Gapped
Lambda K H
1.28 0.460 0.850
Effective search space used: 113092217700
............and a lot of other NO HITS FOUND.
Why this happens?
I'm almost sure to have used the correct nucleotide database and queries. If you want I can cut and paste some of the sequences for each of them.
Please help me!
Thanks
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