Hello everyone! I am using a cluster to align my WGS data to indexed reference genome via BWA. I receive this error on samtools sort part of the task;

[main] CMD: bwa mem -t 40 /save/refs/bwa_refs/Homo_sapiens.GRCh38.dna.toplevel.fa.gz /work/fastqs/557-male_$
[main] Real time: 125431.829 sec; CPU: 4892515.629 sec
[bam_sort_core] merging from 1260 files and 35 in-memory blocks...
[E::hts_open_format] Failed to open file /work/rekren/aligned/aligned_to_human_M_sortedbam.bam.tmp.1016.bam
samtools sort: fail to open "/work/aligned/aligned_to_human_M_sortedbam.bam.tmp.1016.bam": Too many open files

I have read about -m and @ parameters of samtools sort from the manual but playing around with different combinations for those I received out-of memory error from the cluster. Maybe I am overlooking something. Can you suggest a solution for me please?

P.S.:

To submit this task to cluster I use SLURM and my script is below;

#!/bin/bash
#SBATCH -J bwa_task #job name
#SBATCH -e error.out #error file name
#SBATCH --mem=200G #memory reservation
#SBATCH --cpus-per-task=40 #ncpu on the same node
#SBATCH --mail-type=BEGIN,END,FAIL (name.surname@email.com)
#Purge any previous modules
module purge
#Load the application
module load bioinfo/bwa-0.7.17
module load bioinfo/samtools-1.9
# My command lines I want to run on the cluster
bwa mem -t 40 /save/refs/bwa_refs/Homo_sapiens.GRCh38.dna.toplevel.fa.gz /work/fastqs/557-male_ACGCACCT-CCTTCACC-BHNJYMDSXY_L004_R1.fastq.gz /work/fastqs/557-male_ACGCACCT-CCTTCACC-BHNJYMDSXY_L004_R2.fastq.gz | samtools sort -@ 35 -o /work/aligned/aligned_to_human_M_sortedbam.bam

First keeping the output as bam then sorting it via controlled usage of Picard worked in my case. It might help other people who are facing the same kind of issue.

#!/bin/bash
#SBATCH -J bwa_task #job name
#SBATCH -e error.out #error file name
#SBATCH --mem=200G #memory reservation
#SBATCH --cpus-per-task=50 #ncpu on the same node
#SBATCH --mail-type=BEGIN,END,FAIL (name.surname@email.com)
#Purge any previous modules
module purge
#Load the application
module load bioinfo/picard-2.20.7
bwa mem -t 50 /save/refs/bwa_refs/Homo_sapiens.GRCh38.dna.toplevel.fa.gz /work/fastqs/557-male_ACGCACCT-CCTTCACC-BHNJYMDSXY_L004_R1.fastq.gz /workn/fastqs/557-male_ACGCACCT-CCTTCACC-BHNJYMDSXY_L004_R2.fastq.gz | samtools view -F 0x4 -bh -o /work/aligned/aligned_to_human_M.bam
java -Xmx170g -jar ${PICARD} SortSam \
    INPUT=/work/aligned/aligned_to_human_M.bam \
    OUTPUT=/work/aligned/aligned_to_human_M_sorted.bam \
    SORT_ORDER=coordinate \
    MAX_RECORDS_IN_RAM=1000000 \

Look at the man page for samtools-sort. Increase the memory size (-m) and it'll use fewer files. It's easy to see the effect as it reports how many files it is merging with, so you can make a guess at the correct value looking at ulimit to see the maximum you are permitted. (Default mem is 768Mb per thread IIRC)

Just remember -m is per thread. I dislike that, but it's too late to change.