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Looks like in some circumstances the output is not sorted by read name. Technically speaking I think this is fine (the output is still valid .sam as far as I can tell), but read-name sorting is required for some downstream tools, like PCR-duplicate marking methods.
Not really sure if this is a bug or just a nice-to-have feature request, but I think it would smooth adoption if output was more similar to other aligners.
The text was updated successfully, but these errors were encountered:
We are currently working on a switch which preserves order of sequences from input FASTQ files (it will affect time and memory requirements, thus we want to provide it as an optional mode).
Looks like in some circumstances the output is not sorted by read name. Technically speaking I think this is fine (the output is still valid .sam as far as I can tell), but read-name sorting is required for some downstream tools, like PCR-duplicate marking methods.
Not really sure if this is a bug or just a nice-to-have feature request, but I think it would smooth adoption if output was more similar to other aligners.
The text was updated successfully, but these errors were encountered: