[code]#!/bin/bash ## Job Name #SBATCH...

#!/bin/bash
## Job Name
#SBATCH --job-name=re-duck
## Allocation Definition
#SBATCH --account=srlab
#SBATCH --partition=srlab
## Resources
## Nodes (We only get 1, so this is fixed)
#SBATCH --nodes=1
## Walltime (days-hours:minutes:seconds format)
#SBATCH --time=30-00:00:00
## Memory per node
#SBATCH --mem=100G
#SBATCH --mail-type=ALL
#SBATCH --mail-user=sr320@uw.edu
## Specify the working directory for this job
#SBATCH --chdir=/gscratch/scrubbed/sr320/1217/



# Directories and programs
bismark_dir="/gscratch/srlab/programs/Bismark-0.21.0"
bowtie2_dir="/gscratch/srlab/programs/bowtie2-2.3.4.1-linux-x86_64/"
samtools="/gscratch/srlab/programs/samtools-1.9/samtools"
reads_dir="/gscratch/srlab/strigg/data/Pgenr/FASTQS/"
genome_folder="/gscratch/srlab/sr320/data/geoduck/v01/"

source /gscratch/srlab/programs/scripts/paths.sh



${bismark_dir}/bismark_genome_preparation \
--verbose \
--parallel 28 \
--path_to_aligner ${bowtie2_dir} \
${genome_folder}


find ${reads_dir}*_R1_001_val_1.fq.gz \
| xargs basename -s _R1_001_val_1.fq.gz | xargs -I{} ${bismark_dir}/bismark \
--path_to_bowtie ${bowtie2_dir} \
-genome /gscratch/srlab/sr320/data/geoduck/v01 \
-p 4 \
-score_min L,0,-0.6 \
-1 /gscratch/srlab/strigg/data/Pgenr/FASTQS/{}_R1_001_val_1.fq.gz \
-2 /gscratch/srlab/strigg/data/Pgenr/FASTQS/{}_R2_001_val_2.fq.gz \




find *.bam | \
xargs basename -s .bam | \
xargs -I{} ${bismark_dir}/deduplicate_bismark \
--bam \
--paired \
{}.bam



${bismark_dir}/bismark_methylation_extractor \
--bedGraph --counts --scaffolds \
--multicore 14 \
--buffer_size 75% \
*deduplicated.bam



# Bismark processing report

${bismark_dir}/bismark2report

#Bismark summary report

${bismark_dir}/bismark2summary



# Sort files for methylkit and IGV

find *deduplicated.bam | \
xargs basename -s .bam | \
xargs -I{} ${samtools} \
sort --threads 28 {}.bam \
-o {}.sorted.bam

# Index sorted files for IGV
# The "-@ 16" below specifies number of CPU threads to use.

find *.sorted.bam | \
xargs basename -s .sorted.bam | \
xargs -I{} ${samtools} \
index -@ 28 {}.sorted.bam





find *deduplicated.bismark.cov.gz \
| xargs basename -s _R1_001_val_1_bismark_bt2_pe.deduplicated.bismark.cov.gz \
| xargs -I{} ${bismark_dir}/coverage2cytosine \
--genome_folder ${genome_folder} \
-o {} \
--merge_CpG \
--zero_based \
{}_R1_001_val_1_bismark_bt2_pe.deduplicated.bismark.cov.gz


#bismark, #sbatch