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Hi,
I would like to know if someone has experience in comparing a local de novo assembly to a reference assembly and measure which one is the best.
I have mapped genomic Illumina reads to a reference genome. Then, since I'm interested in a 1Mb region of one of the chromosomes, I used a de novo assembler to assemble the reads that mapped to that 1Mb region. So now I have about 6000 contigs ranging in size from 500bp to 30kb and I would like to:
1- visualize their position in relation to the original 1Mb region
2- Be able to say that the de novo local assembly is better (or worse) than just to map my reads to the reference assembly.
Many thanks
I would like to know if someone has experience in comparing a local de novo assembly to a reference assembly and measure which one is the best.
I have mapped genomic Illumina reads to a reference genome. Then, since I'm interested in a 1Mb region of one of the chromosomes, I used a de novo assembler to assemble the reads that mapped to that 1Mb region. So now I have about 6000 contigs ranging in size from 500bp to 30kb and I would like to:
1- visualize their position in relation to the original 1Mb region
2- Be able to say that the de novo local assembly is better (or worse) than just to map my reads to the reference assembly.
Many thanks
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