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Add user specified reads to fastq to validate analysis method?
Hi,
I am analyzing mtDNA and am looking for indels, especially I am hoping to catch some large deletions.
I have performed 150bp PE on MiSeq using NexteraXT library prep.
Using different tools, I am not able to pick up the large deletions I was hoping, however, I am seeing a lot of small indels and substitution mutations, which I also was expecting.
To test my analysis methods, I would like to add some "in silico" generated reads to my fastq files. I am hoping to make 'reads' that cross a large deletions (i.e. the first 75bp of read1 at position 1-75 of mtDNA and the last 75bp and position 1001-1075 of mtDNA, read2 maybe something like position 1275-1201 [i.e. not split up at different genomic position]).
How would I go about manipulating my data in such a way?
I hope my question in clear...
Thanks!
I am analyzing mtDNA and am looking for indels, especially I am hoping to catch some large deletions.
I have performed 150bp PE on MiSeq using NexteraXT library prep.
Using different tools, I am not able to pick up the large deletions I was hoping, however, I am seeing a lot of small indels and substitution mutations, which I also was expecting.
To test my analysis methods, I would like to add some "in silico" generated reads to my fastq files. I am hoping to make 'reads' that cross a large deletions (i.e. the first 75bp of read1 at position 1-75 of mtDNA and the last 75bp and position 1001-1075 of mtDNA, read2 maybe something like position 1275-1201 [i.e. not split up at different genomic position]).
How would I go about manipulating my data in such a way?
I hope my question in clear...
Thanks!
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