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Hi
I was trying to create indices for the reference genome using bfast 0.6.3.c and also trying to convert the reads.
Convert the reference:
bfast-0.6.3c/bfast/bfast fasta2brg -f microbial.fa
The above command airs out with an error and the error file has the following few last lines as output:
[----
[-----53
[-----540,-
[-----542,----2000000]
[-----545,----2000000]
[-----546,----------0]Base:[X]
************************************************************
In function "RGBinaryRead": Fatal Error[OutOfRange]. Variable/Value: original.
Message: Not a valid base pair.
***** Exiting due to errors *****
************************************************************
Can someone point out as to what might be the problem, i guess it is complaining about an invalid base, X in the sequence. How can i workaround this?
Convert the reads
perl /code/orange/BFAST/bfast-0.6.3c/scripts/ill2fastq.pl
what command line options should I choose to convert a file with the name rna_qseq.txt ?
Thanks,
Nipun
I was trying to create indices for the reference genome using bfast 0.6.3.c and also trying to convert the reads.
Convert the reference:
bfast-0.6.3c/bfast/bfast fasta2brg -f microbial.fa
The above command airs out with an error and the error file has the following few last lines as output:
[----
[-----53
[-----540,-
[-----542,----2000000]
[-----545,----2000000]
[-----546,----------0]Base:[X]
************************************************************
In function "RGBinaryRead": Fatal Error[OutOfRange]. Variable/Value: original.
Message: Not a valid base pair.
***** Exiting due to errors *****
************************************************************
Can someone point out as to what might be the problem, i guess it is complaining about an invalid base, X in the sequence. How can i workaround this?
Convert the reads
perl /code/orange/BFAST/bfast-0.6.3c/scripts/ill2fastq.pl
what command line options should I choose to convert a file with the name rna_qseq.txt ?
Thanks,
Nipun
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