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Hi all,
I manage to select some reads from my metagenome illumina analyses. From my blastn analyses I am sure they are from a specific virus but when I try to map those against the reference genome neither tophat2 or bowtie2 allow me to have an alignment... I think is because of big variation between the reads. So... my question is ... is there any other program or way I can map my reads against a reference genome? The goal is to identify what part of the virus is present... so other times I just used Illumina and then samtools and IGV but this time I might need something different and I can't figure out what program will suits better.
If anyone could help it will be great.
Thanks
F.
I manage to select some reads from my metagenome illumina analyses. From my blastn analyses I am sure they are from a specific virus but when I try to map those against the reference genome neither tophat2 or bowtie2 allow me to have an alignment... I think is because of big variation between the reads. So... my question is ... is there any other program or way I can map my reads against a reference genome? The goal is to identify what part of the virus is present... so other times I just used Illumina and then samtools and IGV but this time I might need something different and I can't figure out what program will suits better.
If anyone could help it will be great.
Thanks
F.
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