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Hi,
I see that CLAP is designed to run on eukaryote genomes.
How to adapt it to run on bacteria?
I changed make_annotation.sh by adding species escherichia_coli_k_12 and adjusted ftp site and PATH accordingly. It retrieves annotation and sequence and performs all operations without error message. There are some cosmetic things like Chromosome is converted to "chrChromosome"
and some scripts assume 3 command line arguments one of which is "MT" but it doesn't seem to hurt. Is there anything else I should take into account or have to change/modify?
Cheers,
Tonu
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