I am working with transcriptomes of two species, neither of which have a reference. The reads are 100 bp PE. My strategy has been to make a reference de novo from each library using abyss-pe. Mapping the reads was done in bwa. I map each library to its own reference and that of the other species for SNP identification (i.e. library 1 mapped to reference 1, library 2 mapped to reference 1, etc.).

This strategy has worked great, and some SNPs have been validated empirically. However, I have recently noticed a small but significant number of SNPs in each library that are mapped library 1 to library 1, and yet the variant allele is at like 98%. Given that this is the same library that generated the reference, shouldn't this not happen?

Does anyone know why this happens?