Hi, Everybody is looking for their target reads in a fastq file, and I am just sitting here and can not find a good program to identify the remaining (junk) reads. I am working on ancient DNA (currently horse) illumina reads, and I want to identify the exact organisms (possibly pathogens, human or other contamination, etc) of the remaining reads besides the horse sequences (approx 20-30% of the data contains horse DNA actually). So, can anyone recommend a good program for this task? Thanks in advance :)

First you need to align your reads to the expected reference that it may be contaminated with using FastQ Screen Or DeconSeq, then below post to remove it

http://seqanswers.com/forums/showpost.php?p=109308&postcount=6

This would seem like a good use case for something like Kraken: https://ccb.jhu.edu/software/kraken/

But your ability to assign every read in your experiment to an organism of origin will depend entirely on the completeness of your database.

This might be worth trying: https://github.com/smangul1/rop, see paper: http://biorxiv.org/content/early/2016/05/13/053041

There are some suggestions in these previous threads:

• How would you discover the source of contaminant DNA ?
• Faster BLAST alternative