Mercurial > repos > daumsoft > star_icgc_alignment11
view ICGC_STAR_ALIGNMENT_PIPELINE/ICGC_pipeline.sh @ 0:be0f5f54462d draft default tip
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author | daumsoft |
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date | Mon, 10 Sep 2018 01:20:03 -0400 |
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#!/bin/bash if [ "$#" -ne 1 ]; then echo "[usage:] ICGC_pipeline.sh fastq_in_tar.gz" exit 1; fi #FASTQ_1=$1 #FASTQ_2=$2 #SAMPLE_ID=$3 #TAR_FILE=$SAMPLE_ID".tar" TAR_FILE=$1 export PATH=/storage/data/program/GDC_TGCA-Harmonized/RNA-Seq/bin/ICGC-STAR_ALIGNMENT_PIPELINE:$PATH #tar cvfh $TAR_FILE $FASTQ_2 $FASTQ_1 STAD_ALIGN=~/package/DAUMSOFT/RNA-seq/ICGC_STAR_ALIGNMENT_PIPELINE/star_align.py STAR_INDEX_PATH=~/refs/hg38/gdc/Index_Files/GDC.h38.d1.vd1_STAR2_Index_Files/star_genome_d1_vd1_gtfv22 WORK_DIR=./wrk OUTPUT_BAM=./out REFERENCE=~/refs/hg38/gdc/GRCh38.d1.vd1_Reference_Sequence/GRCh38.d1.vd1.fa RUN_THREAD_NUM=8 rm -rf $WORK_DIR rm -rf $OUTPUT_BAM mkdir $WORK_DIR mkdir $OUTPUT_BAM python $STAD_ALIGN \ --genomeDir $STAR_INDEX_PATH \ --tarFileIn $TAR_FILE \ --workDir $WORK_DIR \ --out $OUTPUT_BAM \ --genomeFastaFiles $REFERENCE \ --runThreadN $RUN_THREAD_NUM \ --outFilterMultimapScoreRange 1 \ --outFilterMultimapNmax 20 \ --outFilterMismatchNmax 10 \ --alignIntronMax 500000 \ --alignMatesGapMax 1000000 \ --sjdbScore 2 \ --limitBAMsortRAM 0 \ --alignSJDBoverhangMin 1 \ --genomeLoad NoSharedMemory \ --outFilterMatchNminOverLread 0.33 \ --outFilterScoreMinOverLread 0.33 \ --twopass1readsN -1 \ --sjdbOverhang 100 \ --outSAMstrandField intronMotif \ --outSAMunmapped Within