Hi, I have trimmomatic 0.39-1 installed via bioconda and I have read the manual. I am confused about giving input files for "paired-end" mode in trimmomatic command lines. I followed up the script and revised it.
java -jar /opt/anaconda3/pkgs/trimmomatic-0.39-1/share/trimmomatic-0.39-1/trimmomatic.jar -threads 16 -phred33 ${SRR}_1.fastq.gz ${SRR}_2.fastq.gz ${SRR}_1_paired.fastq.gz ${SRR}_1_unpaired.fastq.gz ${SRR}_2_paired.fastq.gz ${SRR}_2_unpaired.fastq.gz ILLUMINACLIP:/opt/anaconda3/pkgs/trimmomatic-0.39-1/share/trimmomatic-0.39-1/adapters/TruSeq3-PE-2.fa:2:30:10 LEADING:3 TRAILING:3 SLIDINGWINDOW:4:15 MINLEN:36
so for example, if I would like to put raw read data 00_fastq.text, I change ${SRR}_1.fastq.gz into /Users/maysonlin/Downloads/PhormiaMaleFemaleTranscriptome_Stranded/Phormia raw data/00_fastq/00_1.fastq.qz, do I follow the right track?
I tried to revise the directory and file names, it gives this
Usage: PE [-version] [-threads <threads>] [-phred33|-phred64] [-trimlog <trimLogFile>] [-summary <statsSummaryFile>] [-quiet] [-validatePairs] [-basein <inputBase> | <inputFile1> <inputFile2>] [-baseout <outputBase> | <outputFile1P> <outputFile1U> <outputFile2P> <outputFile2U>] <trimmer1>... or: SE [-version] [-threads <threads>] [-phred33|-phred64] [-trimlog <trimLogFile>] [-summary <statsSummaryFile>] [-quiet] <inputFile> <outputFile> <trimmer1>... or: -version
which exact command have you tried running? did it throw any error? what you propose seems correct, instead of
${SRR}_1.fastq.gz, you just need to locate you own file. You also have to specify the reverse reads, and 4 output files (forward paired, forward unpaired, reverse paired, reverse unpaired)