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I'm new to this so I'm hoping this is a basic question and that someone can suggest a good reference to guide me.
I have 6 lanes of Illumina 100mer paired-end data representing 6 BACs from a plant chromosome (no reference sequence). 5 0f the 6 BACs should overlap.
I have assembled the 6 BACs separately using velvet.
I was then hoping to assemble the velvet contigs.fasta of the BACs using a tool like the Staden package or PHRAP/Consed but have just realized that I'm not sure how to do this and keep the scaffolding and quality scores. What is the most common strategy for assembling a set of BACs?
1)Should I have assembled all 6 BACs (or the 5 overlapping BACs) together?
2)Should I have used the velvetg -amos_file option and then used the AMOS suit?(just starting to read about AMOS)
Thanks,
Bill
I have 6 lanes of Illumina 100mer paired-end data representing 6 BACs from a plant chromosome (no reference sequence). 5 0f the 6 BACs should overlap.
I have assembled the 6 BACs separately using velvet.
I was then hoping to assemble the velvet contigs.fasta of the BACs using a tool like the Staden package or PHRAP/Consed but have just realized that I'm not sure how to do this and keep the scaffolding and quality scores. What is the most common strategy for assembling a set of BACs?
1)Should I have assembled all 6 BACs (or the 5 overlapping BACs) together?
2)Should I have used the velvetg -amos_file option and then used the AMOS suit?(just starting to read about AMOS)
Thanks,
Bill
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