Last updated: 2019-02-26
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Knit directory: threeprimeseq/analysis/
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Unstaged changes:
Modified: analysis/28ind.peak.explore.Rmd
Modified: analysis/CompareLianoglouData.Rmd
Modified: analysis/NewPeakPostMP.Rmd
Modified: analysis/apaQTLoverlapGWAS.Rmd
Modified: analysis/cleanupdtseq.internalpriming.Rmd
Modified: analysis/coloc_apaQTLs_protQTLs.Rmd
Modified: analysis/dif.iso.usage.leafcutter.Rmd
Modified: analysis/diffIsoAnalysisNewMapping.Rmd
Modified: analysis/diff_iso_pipeline.Rmd
Modified: analysis/explainpQTLs.Rmd
Modified: analysis/explore.filters.Rmd
Modified: analysis/flash2mash.Rmd
Modified: analysis/mispriming_approach.Rmd
Modified: analysis/overlapMolQTL.Rmd
Modified: analysis/overlapMolQTL.opposite.Rmd
Modified: analysis/overlap_qtls.Rmd
Modified: analysis/peakOverlap_oppstrand.Rmd
Modified: analysis/peakQCPPlots.Rmd
Modified: analysis/pheno.leaf.comb.Rmd
Modified: analysis/pipeline_55Ind.Rmd
Modified: analysis/swarmPlots_QTLs.Rmd
Modified: analysis/test.max2.Rmd
Modified: analysis/test.smash.Rmd
Modified: analysis/understandPeaks.Rmd
Modified: analysis/unexplainedeQTL_analysis.Rmd
Modified: code/Snakefile
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File | Version | Author | Date | Message |
---|---|---|---|---|
Rmd | 8f85cd2 | Briana Mittleman | 2019-02-26 | save plot |
html | 879be33 | Briana Mittleman | 2019-02-16 | Build site. |
Rmd | f8c76ea | Briana Mittleman | 2019-02-16 | move peak QC plots |
html | 486ff69 | Briana Mittleman | 2019-02-16 | Build site. |
Rmd | b3d5773 | Briana Mittleman | 2019-02-16 | add n sig genes |
html | ab3722b | Briana Mittleman | 2019-02-15 | Build site. |
Rmd | a38fd8c | Briana Mittleman | 2019-02-15 | add QTL analysis |
html | 4f17cca | Briana Mittleman | 2019-02-15 | Build site. |
Rmd | 606e562 | Briana Mittleman | 2019-02-15 | repub |
html | 03c4f95 | Briana Mittleman | 2019-02-14 | Build site. |
Rmd | 41a2537 | Briana Mittleman | 2019-02-14 | add map stat plots |
html | b8cfd6f | Briana Mittleman | 2019-02-07 | Build site. |
Rmd | 3fea644 | Briana Mittleman | 2019-02-07 | add accountmapbias |
library(tidyverse)
── Attaching packages ────────────────────────────────────────────────────────────────────────────────── tidyverse 1.2.1 ──
✔ ggplot2 3.0.0 ✔ purrr 0.2.5
✔ tibble 1.4.2 ✔ dplyr 0.7.6
✔ tidyr 0.8.1 ✔ stringr 1.4.0
✔ readr 1.1.1 ✔ forcats 0.3.0
Warning: package 'stringr' was built under R version 3.5.2
── Conflicts ───────────────────────────────────────────────────────────────────────────────────── tidyverse_conflicts() ──
✖ dplyr::filter() masks stats::filter()
✖ dplyr::lag() masks stats::lag()
library(cowplot)
Attaching package: 'cowplot'
The following object is masked from 'package:ggplot2':
ggsave
We are worried there amy be false positives in the QTL analysis if the QTL is in the read and the snp leads to a mapping bias for the data. I can account for this using WASP.
I have an example script from Yang:
/project2/yangili1/yangili/TCGA_pipe/script_process.sh
STAR2.6 --genomeDir /project2/yangili1/RNAseq_pipeline/index/GRCh37/STAR_hg19 --readFilesIn $inFile\_1.fastq $inFile\_2.fastq --outSAMstrandField intronMotif --outFileNamePrefix $outFile. --outSAMtype BAM Unsorted --varVCFfile $vcfFile --waspOutputMode SAMtag --outSAMattributes vA vG
First I need to find my star indexed genome:
*/project2/gilad/briana/genome_anotation_data/star_genome
Next I need my VCF file:
runStarwWASP.sh
#!/bin/bash
#SBATCH --job-name=runStarwWASP
#SBATCH --account=pi-yangili1
#SBATCH --time=24:00:00
#SBATCH --output=runStarwWASP.out
#SBATCH --error=runStarwWASP.err
#SBATCH --partition=bigmem2
#SBATCH --mem=100G
#SBATCH --mail-type=END
module load Anaconda3
source activate three-prime-env
in=$1
out=$2
STAR --runThreadN 4 --genomeDir /project2/gilad/briana/genome_anotation_data/star_genome --readFilesIn $1 --outSAMstrandField intronMotif --outFileNamePrefix /project2/gilad/briana/threeprimeseq/data/STAR_bam_WASP/$2.combined.STARwWASP.bam --outSAMtype BAM Unsorted --varVCFfile /project2/gilad/briana/YRI_geno_hg19/allChrom.dose.filt.vcf --waspOutputMode SAMtag --outSAMattributes vA vG
test_runStartwWASP.sh
#!/bin/bash
#SBATCH --job-name=test_runStarwWASP
#SBATCH --account=pi-yangili1
#SBATCH --time=24:00:00
#SBATCH --output=test_runStarwWASP.out
#SBATCH --error=test_runStarwWASP.err
#SBATCH --partition=broadwl
#SBATCH --mem=12G
#SBATCH --mail-type=END
module load Anaconda3
source activate three-prime-env
i=/project2/gilad/briana/threeprimeseq/data/fastq/YL-SP-19239-T-combined.fastq
describer=$(echo ${i} | sed -e 's/.*YL-SP-//' | sed -e "s/combined.fastq//")
sbatch runStarwWASP.sh $i $describer
Wraper:
wrap_runStarwWASP.sh
#!/bin/bash
#SBATCH --job-name=wrap_runStarwWASP
#SBATCH --account=pi-yangili1
#SBATCH --time=24:00:00
#SBATCH --output=wrap_runStarwWASP.out
#SBATCH --error=wrap_runStarwWASP.err
#SBATCH --partition=broadwl
#SBATCH --mem=12G
#SBATCH --mail-type=END
module load Anaconda3
source activate three-prime-env
for i in $(ls /project2/gilad/briana/threeprimeseq/data/fastq/*);do
describer=$(echo ${i} | sed -e 's/.*YL-SP-//' | sed -e "s/combined.fastq//")
sbatch runStarwWASP.sh $i $describer
done
Quota reached at 19193N for jobs- create a wrap2
wrap_runStarwWASP2.sh
#!/bin/bash
#SBATCH --job-name=wrap_runStarwWASP2
#SBATCH --account=pi-yangili1
#SBATCH --time=24:00:00
#SBATCH --output=wrap_runStarwWASP2.out
#SBATCH --error=wrap_runStarwWASP2.err
#SBATCH --partition=broadwl
#SBATCH --mem=12G
#SBATCH --mail-type=END
module load Anaconda3
source activate three-prime-env
for i in $(ls /project2/gilad/briana/threeprimeseq/data/fastq/YL-SP-192*); do
describer=$(echo ${i} | sed -e 's/.*YL-SP-//' | sed -e "s/combined.fastq//")
sbatch runStarwWASP.sh $i $describer
done
Sort and index these files.
SortIndexStarwWASP.sh
#!/bin/bash
#SBATCH --job-name=SortIndexStarwWASP
#SBATCH --account=pi-yangili1
#SBATCH --time=24:00:00
#SBATCH --output=SortIndexStarwWASP.out
#SBATCH --error=SortIndexStarwWASP.err
#SBATCH --partition=broadwl
#SBATCH --mem=36G
#SBATCH --mail-type=END
module load Anaconda3
source activate three-prime-env
describer=$1
samtools sort /project2/gilad/briana/threeprimeseq/data/STAR_bam_WASP/${describer}combined.STARwWASP.bamAligned.out.bam > /project2/gilad/briana/threeprimeseq/data/STAR_bam_WASP_sort/${describer}combined.STARwWASP.bamAligned.sort.bam
samtools index /project2/gilad/briana/threeprimeseq/data/STAR_bam_WASP_sort/${describer}combined.STARwWASP.bamAligned.sort.bam
wrap_SortIndexStarwWASP.sh
#!/bin/bash
#SBATCH --job-name=wrap_SortIndexStarwWASP
#SBATCH --account=pi-yangili1
#SBATCH --time=24:00:00
#SBATCH --output=wrap_SortIndexStarwWASP.out
#SBATCH --error=wrap_SortIndexStarwWASP.err
#SBATCH --partition=broadwl
#SBATCH --mem=36G
#SBATCH --mail-type=END
module load Anaconda3
source activate three-prime-env
for i in $(ls /project2/gilad/briana/threeprimeseq/data/STAR_bam_WASP/*STARwWASP.bamAligned.out.bam)
do
describer=$(echo ${i} | sed -e 's/.*STAR_bam_WASP\///' | sed -e "s/combined.STARwWASP.bamAligned.out.bam//")
sbatch SortIndexStarwWASP.sh $describer
done
Now I want to filter out reads with mapping problems at place we see a variant. I want to keep reads with the vW:i:1 tag. ( I will resort and index these files after this step)
I can use pysam to do this. Then I can move the final sorted duplicate files.
filterBamBasedonWasp.py
def main(Bamin, out):
okRead={}
#pysam to read in bam allignments
bamfile = pysam.AlignmentFile(Bamin, "rb")
finalBam = pysam.AlignmentFile(out, "wb", template=bamfile)
n=0
k=0
#read name is the first col in each bam file
for read in bamfile.fetch():
#last piece is always the right piece
#vw=read.split(\t)[-1]
if read.has_tag('vW'):
x= read.get_tag('vW')
print(x)
if x == 1:
k+=1
finalBam.write(read)
else:
n+=1
continue
else:
finalBam.write(read)
print("with wv" + n)
print("pass filter" + k)
bamfile.close()
finalBam.close()
if __name__ == "__main__":
import sys, pysam
describer = sys.argv[1]
inBam="/project2/gilad/briana/threeprimeseq/data/STAR_bam_WASP_sort/" + describer + "combined.STARwWASP.bamAligned.sort.bam"
outBam="/project2/gilad/briana/threeprimeseq/data/STAR_bam_WASP_filtered/" + describer + "combined.STARwWASP.bamAligned.filtered.out.bam"
main(inBam, outBam)
Run this on all individuals:
run_filterBamBasedonWasp.sh
#!/bin/bash
#SBATCH --job-name=run_filterBamBasedonWasp
#SBATCH --account=pi-yangili1
#SBATCH --time=24:00:00
#SBATCH --output=run_filterBamBasedonWasp.out
#SBATCH --error=run_filterBamBasedonWasp.err
#SBATCH --partition=broadwl
#SBATCH --mem=36G
#SBATCH --mail-type=END
module load Anaconda3
source activate three-prime-env
for i in $(ls /project2/gilad/briana/threeprimeseq/data/STAR_bam_WASP_sort/*.bam)
do
describer=$(echo ${i} | sed -e 's/.*STAR_bam_WASP_sort\///' | sed -e "s/combined.STARwWASP.bamAligned.sort.bam//")
python filterBamBasedonWasp.py $describer
done
Sort and index these:
SortIndexStarwWASP_filtered.sh
#!/bin/bash
#SBATCH --job-name=SortIndexStarwWASP_filtered
#SBATCH --account=pi-yangili1
#SBATCH --time=24:00:00
#SBATCH --output=SortIndexStarwWASP_filtered.out
#SBATCH --error=SortIndexStarwWASP_filtered.err
#SBATCH --partition=broadwl
#SBATCH --mem=36G
#SBATCH --mail-type=END
module load Anaconda3
source activate three-prime-env
describer=$1
samtools sort /project2/gilad/briana/threeprimeseq/data/STAR_bam_WASP_filtered/${describer}combined.STARwWASP.bamAligned.filtered.out.bam > /project2/gilad/briana/threeprimeseq/data/STAR_bam_WASP_filtered_sort/${describer}combined.STARwWASP.bamAligned.filtered.sort.bam
samtools index /project2/gilad/briana/threeprimeseq/data/STAR_bam_WASP_filtered_sort/${describer}combined.STARwWASP.bamAligned.filtered.sort.bam
wrap_SortIndexStarwWASP_filtered.sh
#!/bin/bash
#SBATCH --job-name=wrap_SortIndexStarwWASP_filtered
#SBATCH --account=pi-yangili1
#SBATCH --time=24:00:00
#SBATCH --output=wrap_SortIndexStarwWASP_filtered.out
#SBATCH --error=wrap_SortIndexStarwWASP_filtered.err
#SBATCH --partition=broadwl
#SBATCH --mem=36G
#SBATCH --mail-type=END
module load Anaconda3
source activate three-prime-env
for i in $(ls /project2/gilad/briana/threeprimeseq/data/STAR_bam_WASP_filtered/*STARwWASP.bamAligned.filtered.out.bam)
do
describer=$(echo ${i} | sed -e 's/.*STAR_bam_WASP_filtered\///' | sed -e "s/combined.STARwWASP.bamAligned.filtered.out.bam//")
sbatch SortIndexStarwWASP_filtered.sh $describer
done
Now I need to make these into a bed format. I also will move the old files and but these in the sort/ bed/ dirs. This way I can use the same pipeline from the Pipeline for 55 indivduals analysis.
At this point I will move the old bam and bed files to different directories
/project2/gilad/briana/threeprimeseq/data/sort_oldmapp/
/project2/gilad/briana/threeprimeseq/data/bed_sort_oldMap
/project2/gilad/briana/threeprimeseq/data/bed_oldMap
Run bam to bed:
bam2BedandSort.waspmap.sh
#!/bin/bash
#SBATCH --job-name=bam2BedandSort.waspmap
#SBATCH --account=pi-yangili1
#SBATCH --time=24:00:00
#SBATCH --output=bam2BedandSort.waspmap.out
#SBATCH --error=bam2BedandSort.waspmap.err
#SBATCH --partition=broadwl
#SBATCH --mem=36G
#SBATCH --mail-type=END
module load Anaconda3
source activate three-prime-env
for i in $(ls /project2/gilad/briana/threeprimeseq/data/STAR_bam_WASP_filtered_sort/*.bam)
do
describer=$(echo ${i} | sed -e 's/.*STAR_bam_WASP_filtered_sort\///' | sed -e "s/.STARwWASP.bamAligned.filtered.sort.bam//")
bedtools bamtobed -i $i > /project2/gilad/briana/threeprimeseq/data/bed/YL-SP-$describer.combined.bed
sort -k1,1 -k2,2n /project2/gilad/briana/threeprimeseq/data/bed/YL-SP-$describer.combined.bed > /project2/gilad/briana/threeprimeseq/data/bed_sort/YL-SP-$describer.combined.sort.bed
done
Move duplicate files and rename:
problem: these are called combined.combined (fix this)
for i in $(ls /project2/gilad/briana/threeprimeseq/data/bed_10up)
do
describer=$(echo ${i} | sed -e 's/.*YL-SP-//' | sed -e "s/.combined.sort10up.bed//")
mv $i /project2/gilad/briana/threeprimeseq/data/bed_10up/YL-SP-$describer-sort10up.bed
done
Also move the bam files to the sort dir from /project2/gilad/briana/threeprimeseq/data/STAR_bam_WASP_filtered_sort/
for i in $(ls /project2/gilad/briana/threeprimeseq/data/STAR_bam_WASP_filtered_sort/*.bam)
do
describer=$(echo ${i} | sed -e 's/.*STAR_bam_WASP_filtered_sort\///' | sed -e "s/.STARwWASP.bamAligned.filtered.sort.bam//")
mv $i /project2/gilad/briana/threeprimeseq/data/sort/YL-SP-$describer-sort.bam
done
Index all of these files:
reIndex.sh
#!/bin/bash
#SBATCH --job-name=reIndex
#SBATCH --account=pi-yangili1
#SBATCH --time=24:00:00
#SBATCH --output=reIndex.out
#SBATCH --error=reIndex.err
#SBATCH --partition=broadwl
#SBATCH --mem=36G
#SBATCH --mail-type=END
module load Anaconda3
source activate three-prime-env
for i in $(ls /project2/gilad/briana/threeprimeseq/data/sort/)
samtools index /project2/gilad/briana/threeprimeseq/data/sort/$i
done
Get 10 basepairs upstream: wrap_Upstream10Bases.sh
Find sequence for these regions: Nuc10BasesUp.sh
Fixed names (ok now)
for i in $(ls /project2/gilad/briana/threeprimeseq/data/bed_sort/)
do
describer=$(echo ${i} | sed -e 's/.*YL-SP-//' | sed -e "s/.combined.sort.bed//")
cp $i /project2/gilad/briana/threeprimeseq/data/bed_sort/YL-SP-$describer-sort.bed
done
filter bam files wrap_filterBamforMP.pysam2.sh
sort and index merged SortIndexMergedBam_noMP.sh and SortIndex_mergeBamFiles_byfrac_noMP.sh
name peaks
170824 = wc -l /project2/gilad/briana/threeprimeseq/data/mergedPeaks_noMP_filtered/Filtered_APApeaks_merged_allchrom_noMP.bed
seq 1 170824 > peak.num.txt
sort -k1,1 -k2,2n Filtered_APApeaks_merged_allchrom_noMP.bed > Filtered_APApeaks_merged_allchrom_noMP.sort.bed
paste /project2/gilad/briana/threeprimeseq/data/mergedPeaks_noMP_filtered/Filtered_APApeaks_merged_allchrom_noMP.sort.bed peak.num.txt | column -s $'\t' -t > temp
awk '{print $1 "\t" $2 "\t" $3 "\t" $7 "\t" $4 "\t" $5 "\t" $6}' temp > /project2/gilad/briana/threeprimeseq/data/mergedPeaks_noMP_filtered/Filtered_APApeaks_merged_allchrom_noMP.sort.named.bed
#cut the chr
sed 's/^chr//' /project2/gilad/briana/threeprimeseq/data/mergedPeaks_noMP_filtered/Filtered_APApeaks_merged_allchrom_noMP.sort.named.bed > /project2/gilad/briana/threeprimeseq/data/mergedPeaks_noMP_filtered/Filtered_APApeaks_merged_allchrom_noMP.sort.named.noCHR.bed
Gene assignments mapnoMPPeaks2GenomeLoc.sh
filterPheno_bothFraction_GeneLocAnno_5perc.py
In /project2/gilad/briana/threeprimeseq/data/phenotypes_filtPeakTranscript_noMP_GeneLocAnno_5percUs/
#zip file
gzip filtered_APApeaks_merged_allchrom_refseqGenes.GeneLocAnno_NoMP_sm_quant.Nuclear.fixed.pheno_5perc.fc
gzip filtered_APApeaks_merged_allchrom_refseqGenes.GeneLocAnno_NoMP_sm_quant.Total.fixed.pheno_5perc.fc
module load python
#leafcutter script
python /project2/gilad/briana/threeprimeseq/code/prepare_phenotype_table.py filtered_APApeaks_merged_allchrom_refseqGenes.GeneLocAnno_NoMP_sm_quant.Nuclear.fixed.pheno_5perc.fc.gz
python /project2/gilad/briana/threeprimeseq/code/prepare_phenotype_table.py filtered_APApeaks_merged_allchrom_refseqGenes.GeneLocAnno_NoMP_sm_quant.Total.fixed.pheno_5perc.fc.gz
#source activate three-prime-env
sh filtered_APApeaks_merged_allchrom_refseqGenes.GeneLocAnno_NoMP_sm_quant.Nuclear.fixed.pheno_5perc.fc.gz_prepare.sh
sh filtered_APApeaks_merged_allchrom_refseqGenes.GeneLocAnno_NoMP_sm_quant.Total.fixed.pheno_5perc.fc.gz_prepare.sh
#keep only 2 PCs
head -n 3 filtered_APApeaks_merged_allchrom_refseqGenes.GeneLocAnno_NoMP_sm_quant.Nuclear.fixed.pheno_5perc.fc.gz.PCs > filtered_APApeaks_merged_allchrom_refseqGenes.GeneLocAnno_NoMP_sm_quant.Nuclear.fixed.pheno_5perc.fc.gz.2PCs
head -n 3 filtered_APApeaks_merged_allchrom_refseqGenes.GeneLocAnno_NoMP_sm_quant.Total.fixed.pheno_5perc.fc.gz.PCs > filtered_APApeaks_merged_allchrom_refseqGenes.GeneLocAnno_NoMP_sm_quant.Total.fixed.pheno_5perc.fc.gz.2PCs
makeSampleList_newGeneAnno.py
APAqtl_nominal_GeneLocAnno_noMP_5percUsage.sh
APAqtl_perm_GeneLocAnno_noMP_5percUsage.sh
run_APAqtlpermCorrectQQplot_GeneLocAnno_noMP_5perUs.sh
totQTLs=read.table("../data/perm_QTL_GeneLocAnno_noMP_5percov/filtered_APApeaks_merged_allchrom_refseqGenes.GeneLocAnno.NoMP_sm_quant.Total.fixed.pheno_5perc_permResBH.txt", stringsAsFactors = F, header=T)
Sig_TotQTLs= totQTLs %>% filter(-log10(bh)>=1)
nrow(Sig_TotQTLs)
[1] 291
How many genes are tested:
totQTLs %>% separate(pid, into=c("chr", "start", "end", "id"), sep=":") %>% separate(id, into=c("gene", "strand", "peak"), sep="_") %>% group_by(gene) %>% select(gene) %>% tally() %>% nrow()
Warning: Expected 3 pieces. Additional pieces discarded in 3 rows [886,
887, 888].
[1] 11183
sigQTLTGenes=Sig_TotQTLs %>% separate(pid, into=c("chr", "start", "end", "id"), sep=":") %>% separate(id, into=c("gene", "strand", "peak"), sep="_") %>% group_by(gene) %>% tally() %>% nrow()
sigQTLTGenes
[1] 235
nucQTLs=read.table("../data/perm_QTL_GeneLocAnno_noMP_5percov/filtered_APApeaks_merged_allchrom_refseqGenes.GeneLocAnno.NoMP_sm_quant.Nuclear.fixed.pheno_5perc_permResBH.txt", stringsAsFactors = F, header=T)
Sig_NucQTLs= nucQTLs %>% filter(-log10(bh)>=1)
nrow(Sig_NucQTLs)
[1] 615
How many genes:
nucQTLs %>% separate(pid, into=c("chr", "start", "end", "id"), sep=":") %>% separate(id, into=c("gene", "strand", "peak"), sep="_") %>% group_by(gene) %>% select(gene) %>% tally() %>% nrow()
Warning: Expected 3 pieces. Additional pieces discarded in 3 rows [1056,
1057, 1058].
[1] 11499
sigQTLNGenes=Sig_NucQTLs %>% separate(pid, into=c("chr", "start", "end", "id"), sep=":") %>% separate(id, into=c("gene", "strand", "peak"), sep="_") %>% group_by(gene) %>% tally() %>% nrow()
sigQTLNGenes
[1] 496
Write QTLs to get locations:
totQTLs_sig=read.table("../data/perm_QTL_GeneLocAnno_noMP_5percov/filtered_APApeaks_merged_allchrom_refseqGenes.GeneLocAnno.NoMP_sm_quant.Total.fixed.pheno_5perc_permResBH.txt", stringsAsFactors = F, header=T)%>% filter(-log10(bh)>=1)
write.table(totQTLs_sig,"../data/ApaQTLs/TotalapaQTLs.GeneLocAnno.noMP.5perc.10FDR.txt", row.names = F, col.names = F, quote = F)
nucQTLs_sig=read.table("../data/perm_QTL_GeneLocAnno_noMP_5percov/filtered_APApeaks_merged_allchrom_refseqGenes.GeneLocAnno.NoMP_sm_quant.Nuclear.fixed.pheno_5perc_permResBH.txt", stringsAsFactors = F, header=T)%>% filter(-log10(bh)>=1)
write.table(nucQTLs_sig,"../data/ApaQTLs/NuclearapaQTLs.GeneLocAnno.noMP.5perc.10FDR.txt", row.names = F, col.names = F, quote = F)
getDistPeakEnd2QTL.py
TotDist=read.table("../data/ApaQTLs/Distance2EndPeak.Total.apaQTLs.txt", header=T) %>% mutate(Fraction="Total") %>% select(Fraction, Distance)
NucDist=read.table("../data/ApaQTLs/Distance2EndPeak.Nuclear.apaQTLs.txt", header=T)%>% mutate(Fraction="Nuclear") %>% select(Fraction, Distance)
BothDist=data.frame(rbind(TotDist, NucDist))
distplot=ggplot(BothDist, aes(x=Distance, by=Fraction, fill=Fraction))+geom_histogram(bins=70, alpha=.5) + scale_fill_manual(values=c("deepskyblue3","darkviolet")) + labs(title="Distance From apaQTL to End of Peak" )
distplot
Version | Author | Date |
---|---|---|
ab3722b | Briana Mittleman | 2019-02-15 |
ggsave(distplot, file="../output/plots/QTLDist2EndofPeak.png")
Saving 7 x 5 in image
Where are the QTLs:
QTLfile2Bed.py “Total” QTLfile2Bed.py “Nuclear”
I will need to sort the output
sort -k1,1 -k2,2n /project2/gilad/briana/threeprimeseq/data/ApaQTLs/Total.apaQTLs.bed > /project2/gilad/briana/threeprimeseq/data/ApaQTLs/Total.apaQTLs.sort.bed
sort -k1,1 -k2,2n /project2/gilad/briana/threeprimeseq/data/ApaQTLs/Nuclear.apaQTLs.bed > /project2/gilad/briana/threeprimeseq/data/ApaQTLs/Nuclear.apaQTLs.sort.bed
mapQTLs2GenomeLoc.sh
Look at number of reads lost due to WASP filter
getWASPfiltStats.py
def main(Bamin,out,desc):
okRead={}
#pysam to read in bam allignments
outF=open(out, "w")
bamfile = pysam.AlignmentFile(Bamin, "rb")
n=0
k=0
#read name is the first col in each bam file
for read in bamfile.fetch():
#last piece is always the right piece
#vw=read.split(\t)[-1]
if read.has_tag('vW'):
x= read.get_tag('vW')
#print(x)
if x == 1:
k+=1
#finalBam.write(read)
else:
n+=1
continue
else:
continue
#finalBam.write(read)
outF.write("%s\t%d\n"%(desc, n))
bamfile.close()
outF.clos()
if __name__ == "__main__":
import sys, pysam
describer = sys.argv[1]
describer2=describer[:-1]
inBam="/project2/gilad/briana/threeprimeseq/data/STAR_bam_WASP_sort/" + describer + "combined.STARwWASP.bamAligned.sort.bam"
outFile="/project2/gilad/briana/threeprimeseq/data/WASP_filt_stat/WASPFilt" + describer2 + ".txt"
main(inBam,outFile, describer2)
run_getWASPfiltStats.sh
#!/bin/bash
#SBATCH --job-name=run_getWASPfiltStats
#SBATCH --account=pi-yangili1
#SBATCH --time=24:00:00
#SBATCH --output=run_getWASPfiltStats.out
#SBATCH --error=run_getWASPfiltStats.err
#SBATCH --partition=broadwl
#SBATCH --mem=36G
#SBATCH --mail-type=END
module load Anaconda3
source activate three-prime-env
for i in $(ls /project2/gilad/briana/threeprimeseq/data/STAR_bam_WASP_sort/*.bam)
do
describer=$(echo ${i} | sed -e 's/.*STAR_bam_WASP_sort\///' | sed -e "s/combined.STARwWASP.bamAligned.sort.bam//")
python getWASPfiltStats.py $describer
done
Cat all of the files together and move the duplicates to replicate folder
waspStat=read.table("../data/WASP_STAT/WASP_Filt_AllLineStats.txt",stringsAsFactors = F, col.names = c("Sample", "FilteredReads")) %>% separate(Sample, into=c("Line", "Fraction"), sep="-")
Plot
ggplot(waspStat, aes(x=Line, fill=Fraction, y=FilteredReads, by=Fraction)) + geom_bar(stat="identity", position="dodge")
make boxplot
ggplot(waspStat, aes(x=Fraction, y=log10(FilteredReads), fill=Fraction)) + geom_boxplot()
Version | Author | Date |
---|---|---|
879be33 | Briana Mittleman | 2019-02-16 |
Plto barplots by fractions with error bar
waspStat_sem= waspStat %>% group_by(Fraction) %>% summarise(mean=mean(FilteredReads), sd=sd(FilteredReads))
ggplot(waspStat_sem, aes(x=Fraction, y=mean, fill=Fraction)) + geom_bar(stat='identity') + geom_errorbar(aes(ymin=mean-sd, ymax=mean+sd), width=.2,) + labs(title="Reads filtered out due to WASP filter", y='Reads') +scale_fill_manual(values=c("deepskyblue3","darkviolet"))
Version | Author | Date |
---|---|---|
879be33 | Briana Mittleman | 2019-02-16 |
Map stat plots:
mapStats_wasp=read.table("../data/threePrimeSeqMetaData55Ind_noDup_WASPMAP.txt", stringsAsFactors = F, header = T)
Plot mappeded reads no MP by fractions:
mapStats_wasp_noMP=mapStats_wasp %>% group_by(fraction) %>% summarise(mean=mean(Mapped_noMP), sd=sd(Mapped_noMP))
mapreads_plot=ggplot(mapStats_wasp_noMP, aes(x=fraction, y=mean, fill=fraction)) + geom_bar(stat='identity')+ geom_errorbar(aes(ymin=mean-sd, ymax=mean+sd), width=.2)+ scale_fill_manual(values=c("deepskyblue3","darkviolet")) + labs(title="Number of reads\n mapping and passing missprime filter", y="Number of sequence reads")
mapStats_wasp_propnoMP=mapStats_wasp %>% group_by(fraction) %>% summarise(mean=mean(prop_MappedwithoutMP), sd=sd(prop_MappedwithoutMP))
propmap_plot=ggplot(mapStats_wasp_propnoMP, aes(x=fraction, y=mean, fill=fraction)) + geom_bar(stat='identity')+ geom_errorbar(aes(ymin=mean-sd, ymax=mean+sd), width=.2)+ scale_fill_manual(values=c("deepskyblue3","darkviolet"))+ labs(title="Proportion of reads\n mapping and passing missprime filter", y="Proportion of sequence reads")
mapStats_wasp_reads=mapStats_wasp %>% group_by(fraction) %>% summarise(mean=mean(reads), sd=sd(reads))
seqread_plot=ggplot(mapStats_wasp_reads, aes(x=fraction, y=mean, fill=fraction)) + geom_bar(stat='identity')+ geom_errorbar(aes(ymin=mean-sd, ymax=mean+sd), width=.2)+ scale_fill_manual(values=c("deepskyblue3","darkviolet"))+ labs(title="Sequenced Reads", y="Number of sequence reads")
All plots:
library(cowplot)
allmapstatplots=plot_grid(seqread_plot,mapreads_plot,propmap_plot,ncol = 3)
allmapstatplots
Version | Author | Date |
---|---|---|
879be33 | Briana Mittleman | 2019-02-16 |
ggsave(allmapstatplots, file="../output/plots/MapStatBarPlots.png",width=15)
Saving 15 x 5 in image
Boxplot:
seqread_plotbar=ggplot(mapStats_wasp, aes(x=fraction, y=log10(reads), fill=fraction)) + geom_boxplot()+scale_fill_manual(values=c("deepskyblue3","darkviolet"))+ labs(title="Sequenced Reads", y="log10(Number of sequence reads)")
seqread_plotbar
Version | Author | Date |
---|---|---|
879be33 | Briana Mittleman | 2019-02-16 |
mapreads_plotbar=ggplot(mapStats_wasp, aes(x=fraction, y=log10(Mapped_noMP), fill=fraction)) + geom_boxplot()+scale_fill_manual(values=c("deepskyblue3","darkviolet"))+ labs(title="Mapped Reads\n filtered for misspriming", y="log10(Mapped Reads)")
mapreads_plotbar
Version | Author | Date |
---|---|---|
879be33 | Briana Mittleman | 2019-02-16 |
maprop_plotbar=ggplot(mapStats_wasp, aes(x=fraction, y=prop_MappedwithoutMP, fill=fraction)) + geom_boxplot()+scale_fill_manual(values=c("deepskyblue3","darkviolet"))+ labs(title="Proportion Mapped Reads\n and filtered for misspriming", y="Proportion mapped post misspriming")
maprop_plotbar
Version | Author | Date |
---|---|---|
879be33 | Briana Mittleman | 2019-02-16 |
allmapstatboxplots=plot_grid(seqread_plotbar,mapreads_plotbar,maprop_plotbar,ncol = 3)
allmapstatboxplots
Version | Author | Date |
---|---|---|
879be33 | Briana Mittleman | 2019-02-16 |
ggsave(allmapstatboxplots, file="../output/plots/MapStatBoxPlots.png",width=15)
Saving 15 x 5 in image
sessionInfo()
R version 3.5.1 (2018-07-02)
Platform: x86_64-apple-darwin15.6.0 (64-bit)
Running under: macOS 10.14.1
Matrix products: default
BLAS: /Library/Frameworks/R.framework/Versions/3.5/Resources/lib/libRblas.0.dylib
LAPACK: /Library/Frameworks/R.framework/Versions/3.5/Resources/lib/libRlapack.dylib
locale:
[1] en_US.UTF-8/en_US.UTF-8/en_US.UTF-8/C/en_US.UTF-8/en_US.UTF-8
attached base packages:
[1] stats graphics grDevices utils datasets methods base
other attached packages:
[1] bindrcpp_0.2.2 cowplot_0.9.3 forcats_0.3.0 stringr_1.4.0
[5] dplyr_0.7.6 purrr_0.2.5 readr_1.1.1 tidyr_0.8.1
[9] tibble_1.4.2 ggplot2_3.0.0 tidyverse_1.2.1
loaded via a namespace (and not attached):
[1] Rcpp_0.12.19 cellranger_1.1.0 plyr_1.8.4 compiler_3.5.1
[5] pillar_1.3.0 git2r_0.24.0 workflowr_1.2.0 bindr_0.1.1
[9] tools_3.5.1 digest_0.6.17 lubridate_1.7.4 jsonlite_1.6
[13] evaluate_0.13 nlme_3.1-137 gtable_0.2.0 lattice_0.20-35
[17] pkgconfig_2.0.2 rlang_0.2.2 cli_1.0.1 rstudioapi_0.9.0
[21] yaml_2.2.0 haven_1.1.2 withr_2.1.2 xml2_1.2.0
[25] httr_1.3.1 knitr_1.20 hms_0.4.2 fs_1.2.6
[29] rprojroot_1.3-2 grid_3.5.1 tidyselect_0.2.4 glue_1.3.0
[33] R6_2.3.0 readxl_1.1.0 rmarkdown_1.11 modelr_0.1.2
[37] magrittr_1.5 whisker_0.3-2 backports_1.1.2 scales_1.0.0
[41] htmltools_0.3.6 rvest_0.3.2 assertthat_0.2.0 colorspace_1.3-2
[45] labeling_0.3 stringi_1.2.4 lazyeval_0.2.1 munsell_0.5.0
[49] broom_0.5.0 crayon_1.3.4