Provided by: nanofilt_2.6.0-4_all 
NAME
NanoFilt - filtering and trimming of long read sequencing data
DESCRIPTION
usage: NanoFilt [-h] [-v] [--logfile LOGFILE] [-l LENGTH]
[--maxlength MAXLENGTH] [-q QUALITY] [--minGC MINGC] [--maxGC MAXGC] [--headcrop
HEADCROP] [--tailcrop TAILCROP] [-s SUMMARY] [--readtype {1D,2D,1D2}] [input]
Perform quality and/or length and/or GC filtering of (long read) fastq data.
Reads on stdin.
General options:
-h, --help
show the help and exit
-v, --version
Print version and exit.
--logfile LOGFILE
Specify the path and filename for the log file.
input input, uncompressed fastq file
Options for filtering reads on.:
-l LENGTH, --length LENGTH
Filter on a minimum read length
--maxlength MAXLENGTH
Filter on a maximum read length
-q QUALITY, --quality QUALITY
Filter on a minimum average read quality score
--minGC MINGC
Sequences must have GC content >= to this. Float between 0.0 and 1.0. Ignored if
using summary file.
--maxGC MAXGC
Sequences must have GC content <= to this. Float between 0.0 and 1.0. Ignored if
using summary file.
Options for trimming reads.:
--headcrop HEADCROP
Trim n nucleotides from start of read
--tailcrop TAILCROP
Trim n nucleotides from end of read
Input options.:
-s SUMMARY, --summary SUMMARY
Use albacore or guppy summary file for quality scores
--readtype {1D,2D,1D2}
Which read type to extract information about from summary. Options are 1D, 2D or
1D2
EXAMPLES:
gunzip -c reads.fastq.gz | NanoFilt -q 10 -l 500 --headcrop 50 | minimap2 genome.fa
- | samtools sort -O BAM -@24 -o alignment.bam - gunzip -c reads.fastq.gz |
NanoFilt -q 12 --headcrop 75 | gzip > trimmed-reads.fastq.gz gunzip -c
reads.fastq.gz | NanoFilt -q 10 | gzip > highQuality-reads.fastq.gz
SEE ALSO
The full documentation for NanoFilt is maintained as a Texinfo manual. If the info and
NanoFilt programs are properly installed at your site, the command
info NanoFilt
should give you access to the complete manual.