What kind of data do you have so far ("raw" FASTQ or is it already processed?) and what exactly do you want to achieve?

jwfoley, the data's still being processed and I'll receive in FASTQ. I want to find mutation hot spots, nucleotide substituations and comparing the diversity of the genome at various times.

Hi vitor,

First, you need to trim your reads, to discard low quality bases. You could use Trimmomatic, fastx_toolkit, prinseq, etc. Then, you have to map your sequences to the reference genome. If you want to analyze substitutions, I think it is more suitable to chose a more sensitive mapper, as SMALT, but your reads should be short (75 bp) , because they were sequenced with HiSeq, in this case I think bowtie 1 is good enough, Once you have your reads mapped, you have to perform a SNP calling. I recommend you freebayes, because it allows to analyze haploid organisms. With your VCF file generated with freeBayes you can perform a functional analysis with SNPeff.

I hope it helps!