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This is the command TrimmomaticSE that can be run in the OnWorks free hosting provider using one of our multiple free online workstations such as Ubuntu Online, Fedora Online, Windows online emulator or MAC OS online emulator

PROGRAM:

NAME


TrimmomaticPE - flexible read trimming tool for Illumina NGS data

SYNOPSIS


Paired End Mode:

TrimmomaticPE [-threads threads] [-phred33 | -phred64] [-trimlog logFile] paired output
1 unpaired output 1 paired output 2 unpaired output 2 step 1 ...

Single End Mode:

TrimmomaticSE [-threads threads] [-phred33 | -phred64] [-trimlog logFile] output step 1
...

DESCRIPTION


Trimmomatic performs a variety of useful trimming tasks for illumina paired-end and single
ended data.The selection of trimming steps and their associated parameters are supplied on
the command line.

OPTIONS


-phred
If no quality score is specified, phred-64 is the default.

-trimlog
Specifying a trimlog file creates a log of all read trimmings, indicating the
following details:

· the read name

· the surviving sequence length

· the location of the first surviving base, aka. the amount trimmed from the start

· the location of the last surviving base in the original read

· the amount trimmed from the end

Multiple steps can be specified as required, by using additional arguments at the end.

Most steps take one or more settings, delimited by ´:´ (a colon)

Step options:

ILLUMINACLIP:<fastaWithAdaptersEtc>:<seed mismatches>:<palindrome clip threshold>:<simple clip threshold>
fastaWithAdaptersEtc: specifies the path to a fasta file containing all the adapters, PCR sequences etc.
The naming of the various sequences within this file determines how they are used. See below.
seedMismatches: specifies the maximum mismatch count which will still allow a full match to be performed
palindromeClipThreshold: specifies how accurate the match between the two ´adapter ligated´ reads must be for PE palindrome read alignment.
simpleClipThreshold: specifies how accurate the match between any adapter etc. sequence must be against a read.
.
The adapters are installed on the Debian system at /usr/share/trimmomatic/.

SLIDINGWINDOW:<windowSize>:<requiredQuality>
windowSize: specifies the number of bases to average across
requiredQuality: specifies the average quality required.

LEADING:<quality>
quality: Specifies the minimum quality required to keep a base.

TRAILING:<quality>
quality: Specifies the minimum quality required to keep a base.

CROP:<length>
length: The number of bases to keep, from the start of the read.

HEADCROP:<length>
length: The number of bases to remove from the start of the read.

MINLENGTH:<length>
length: Specifies the minimum length of reads to be kept.

Trimming Order

Trimming occurs in the order which the steps are specified on the command line. It is
recommended in most cases that adapter clipping, if required, is done as early as
possible.

EXAMPLES


Paired End:

TrimmomaticPE s_1_1_sequence.txt.gz s_1_2_sequence.txt.gz lane1_forward_paired.fq.gz
lane1_forward_unpaired.fq.gz lane1_reverse_paired.fq.gz lane1_reverse_unpaired.fq.gz
ILLUMINACLIP:/usr/share/trimmomatic/illuminaClipping.fa:2:40:15 LEADING:3 TRAILING:3
SLIDINGWINDOW:4:15 MINLEN:36

This will perform the following:

Remove adapters
Remove leading low quality or N bases (below quality 3)
Remove trailing low quality or N bases (below quality 3)
Scan the read with a 4-base wide sliding window, cutting when the average quality per base drops below 15
Drop reads below the 36 bases long

The equivalent for single-ended reads is:

TrimmomaticSE s_1_1_sequence.txt.gz lane1_forward.fq.gz
ILLUMINACLIP:/usr/share/trimmomatic/illuminaClipping.fa:2:40:15 LEADING:3 TRAILING:3
SLIDINGWINDOW:4:15 MINLEN:36

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