diff --git a/alignment/bamqc.sh b/alignment/bamqc.sh
index 7c2b403bcc6b6c9105637e372165d75a72959e65..c08dcbe41e98a8964ede472573c5e90c16efb73d 100644
--- a/alignment/bamqc.sh
+++ b/alignment/bamqc.sh
@@ -8,14 +8,14 @@ usage() {
echo "-n --NucType"
echo "-p --Prefix for output file name"
echo "-c --Capture Bedfile"
- echo "Example: bash hisat.sh -p prefix -r GRCh38 -a hisat -x SRR1551047_1.fastq.gz -y SRR1551047_2.fastq.gz"
+ echo "Example: bash bamqc.sh -p prefix -r /project/shared/bicf_workflow_ref/GRCh38 -b SRR1551047.bam -y dna -c target.bed"
exit 1
}
OPTIND=1 # Reset OPTIND
while getopts :r:b:n:p:h opt
do
case $opt in
- r) refgeno=$OPTARG;;
+ r) index_path=$OPTARG;;
b) sbam=$OPTARG;;
c) bed=$OPTARG;;
y) nuctype=$OPTARG;;
@@ -31,12 +31,6 @@ if [[ -z $pair_id ]] || [[ -z $fq1 ]]; then
usage
fi
-if [ $refgeno == 'GRCh38' ] || [ $refgeno == 'GRCm38' ]; then
- index_path=/project/shared/bicf_workflow_ref/${refgeno}
-else
- usage
-fi
-
module load samtools/1.6 fastqc/0.11.5
samtools flagstat ${sbam} > ${pair_id}.flagstat.txt
fastqc -f bam ${sbam}
diff --git a/alignment/dnaseqalign.sh b/alignment/dnaseqalign.sh
index 98972fef62e8671e10260d7c155e0cef82171338..0e1962388c69848a3fbb226e9add3e42dcf6e751 100644
--- a/alignment/dnaseqalign.sh
+++ b/alignment/dnaseqalign.sh
@@ -7,14 +7,14 @@ usage() {
echo "-x --FastQ R1"
echo "-y --FastQ R2"
echo "-p --Prefix for output file name"
- echo "Example: bash hisat.sh -p prefix -r GRCh38 -x SRR1551047_1.fastq.gz -y SRR1551047_2.fastq.gz"
+ echo "Example: bash dnaseqalign.sh -p prefix -r /project/shared/bicf_workflow_ref/GRCh38 -x SRR1551047_1.fastq.gz -y SRR1551047_2.fastq.gz"
exit 1
}
OPTIND=1 # Reset OPTIND
while getopts :r:a:x:y:p:h opt
do
case $opt in
- r) refgeno=$OPTARG;;
+ r) index_path=$OPTARG;;
x) fq1=$OPTARG;;
y) fq2=$OPTARG;;
a) algo=$OPTARG;;
@@ -30,12 +30,6 @@ if [[ -z $pair_id ]] || [[ -z $fq1 ]]; then
usage
fi
-if [ $refgeno == 'GRCh38' ] || [ $refgeno == 'GRCm38' ] || [ $refgeno == 'GRCh37' ]; then
- index_path=/project/shared/bicf_workflow_ref/${refgeno}
-else
- usage
-fi
-
if [[ -z $SLURM_CPUS_ON_NODE ]]
then
SLURM_CPUS_ON_NODE=1
@@ -48,7 +42,7 @@ then
else
bwa mem -M -t $SLURM_CPUS_ON_NODE -R "@RG\tID:${pair_id}\tLB:tx\tPL:illumina\tPU:barcode\tSM:${pair_id}" ${index_path}/genome.fa ${fq1} ${fq2} > out.sam
fi
-if [ $refgeno == 'GRCh38' ]
+if [[ $index_path == '/project/shared/bicf_workflow_ref/GRCh38' ]]
then
cat out.sam | k8 /cm/shared/apps/bwakit/0.7.15/bwa-postalt.js -p ${pair_id}.hla ${index_path}/genome.fa.alt | samtools view -1 - > output.unsort.bam
run-HLA ${pair_id}.hla > ${pair_id}.hla.top 2> ${pair_id}.log.hla
@@ -59,7 +53,7 @@ else
fi
samtools sort --threads $SLURM_CPUS_ON_NODE -o output.dups.bam output.unsort.bam
samtools view -h output.unsort.bam | samblaster -M -a --excludeDups --addMateTags --maxSplitCount 2 --minNonOverlap 20 -d discordants.sam -s splitters.sam > temp.sam
-gawk '{ if (\$0~"^@") { print; next } else { \$10="*"; \$11="*"; print } }' OFS="\\t" splitters.sam | samtools view -S -b - | samtools sort -o ${pair_id}.splitters.bam -
-gawk '{ if (\$0~"^@") { print; next } else { \$10="*"; \$11="*"; print } }' OFS="\\t" discordants.sam | samtools view -S -b - | samtools sort -o ${pair_id}.discordants.bam -
-java -Djava.io.tmpdir=./ -Xmx4g -jar \$PICARD/picard.jar FixMateInformation ASSUME_SORTED=TRUE SORT_ORDER=coordinate ADD_MATE_CIGAR=TRUE I=output.dups.bam O=${pair_id}.bam
+gawk '{ if ($0~"^@") { print; next } else { $10="*"; $11="*"; print } }' OFS="\t" splitters.sam | samtools view -S -b - | samtools sort -o ${pair_id}.splitters.bam -
+gawk '{ if ($0~"^@") { print; next } else { $10="*"; $11="*"; print } }' OFS="\t" discordants.sam | samtools view -S -b - | samtools sort -o ${pair_id}.discordants.bam -
+java -Djava.io.tmpdir=./ -Xmx4g -jar $PICARD/picard.jar FixMateInformation ASSUME_SORTED=TRUE SORT_ORDER=coordinate ADD_MATE_CIGAR=TRUE I=output.dups.bam O=${pair_id}.bam
samtools index -@ $SLURM_CPUS_ON_NODE ${pair_id}.bam