I'm trying to decide if our data shows that we require the depth of HiSeq or if we could do MiSeq.
What I have done is concatenated all the contigs into one fasta file which I used to create an index in Bowtie.
Then, I tried aligning the raw reads to this index using Bowtie.
Unfortunately, I found that only 75% of my "genome" was covered. Is there something I'm missing?
What I have done is concatenated all the contigs into one fasta file which I used to create an index in Bowtie.
Then, I tried aligning the raw reads to this index using Bowtie.
Unfortunately, I found that only 75% of my "genome" was covered. Is there something I'm missing?
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