extract options:¶

-s|-sample <dir> specifies sample directory

-f|-reads specifies alternative dir for FAST5 files (default fast5)

Can be absolute (beginning with /) or relative e.g. -f reads/downloads if replicating Metrichor file structure

-a|-fasta specifies FASTA file extraction (default)

-q|-fastq specifies FASTQ file extraction

-basecallindex specifies the index of the analysis (default: latest)

-mergereads to generate merged FASTA files in addition to single read files

-minquality <value> to set the minimum quality for a 'pass' read

align options:¶

-s|-sample <dir> specifies sample directory

-r|-reference <path> specifies path to reference database

-aligner <name> specifies the aligner (default last)

-alignerparams <params> specifies parameters to the aligner

-showaligns echoes aligner commands to screen

analyse options:¶

-s|-sample <dir> specifies sample directory

-r|-reference <path> specifies path to reference database

-aligner <name> specifies the aligner (default last)

-coveragebin <int> specifies coverage bin size (default 100)

-bitmaps to output bitmap PNG graphs instead of PDF

compare options:¶

-l|-samplelist <file> specifies a sample list file

-o|-outputdir <directory> specifies an output directory

-type <2d|template|complement> specifies an output directory

process options:¶

-process <file> specifies a process file

Read type options:¶

-passonly to analyse only pass reads

-failonly to analyse only fail reads

-2donly to analyse only 2D reads

-templateonly to analyse just Template reads

-complementonly to analyse just Complement reads

Other options:¶

-t|-numthreads <number> specifies the number of threads to use (default 1)

-log <filename> enables debug logging to file

-force to force NanoOK to ignore warnings

-timeout to set the number of seconds before giving up waiting for new reads (default 2)

Valid aligners: last, bwa, blasr, marginalign, graphmap