Hiya folks,
I've got a two part question for you today. I'm attempting to create multi-species alignments for use in a scan for selection. I've one well-sequenced reference and several related species that have been sequenced using 454.
One technique would be to take each gene in the reference genome as a target and use Newbler (or something else) to map the 454 reads to the genes. But I'd rather something more elegant, like an over.chain file (http://genome.ucsc.edu/goldenPath/help/chain.html) that allows me to pull out specific orthologous regions from a whole-genome alignment.
Here are my issues:
1) I can use Newbler to align the 454 reads to the reference genome, but the resulting file formats don't help very much. Does anyone know an elegant way to transform ace (or other Newbler files) into SAM or GTF or PSL? Or is the most "elegant" way through AMOS as suggested in older threads?
2) For a couple of species, I have .gtf files that have already been generated for me. Yay. Does anyone know of an existing program that would allow me to use these .gtf files to get pull down all 454 reads (or at least names) that map to a given region of the reference? Or a way to reverse to .gtf so that the map is REFERENCE-->454 Reads rather than the current 454 Reads --> REFERENCE?
Many thanks, and happy sequencing.
--David
I've got a two part question for you today. I'm attempting to create multi-species alignments for use in a scan for selection. I've one well-sequenced reference and several related species that have been sequenced using 454.
One technique would be to take each gene in the reference genome as a target and use Newbler (or something else) to map the 454 reads to the genes. But I'd rather something more elegant, like an over.chain file (http://genome.ucsc.edu/goldenPath/help/chain.html) that allows me to pull out specific orthologous regions from a whole-genome alignment.
Here are my issues:
1) I can use Newbler to align the 454 reads to the reference genome, but the resulting file formats don't help very much. Does anyone know an elegant way to transform ace (or other Newbler files) into SAM or GTF or PSL? Or is the most "elegant" way through AMOS as suggested in older threads?
2) For a couple of species, I have .gtf files that have already been generated for me. Yay. Does anyone know of an existing program that would allow me to use these .gtf files to get pull down all 454 reads (or at least names) that map to a given region of the reference? Or a way to reverse to .gtf so that the map is REFERENCE-->454 Reads rather than the current 454 Reads --> REFERENCE?
Many thanks, and happy sequencing.
--David
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