Last updated: 2019-06-13

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Knit directory: apaQTL/analysis/

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Unstaged changes:
    Modified:   analysis/DiffIsoAnalysis.Rmd
    Modified:   analysis/Readdistagainstfeatures.Rmd
    Modified:   analysis/choosePCs.Rmd
    Modified:   analysis/index.Rmd
    Modified:   analysis/motifDisruption.Rmd
    Modified:   analysis/nascenttranscription.Rmd
    Modified:   analysis/nucintronicanalysis.Rmd
    Modified:   analysis/overlapapaqtlsandeqtls.Rmd
    Modified:   analysis/rna_netseq_h3k12ac.Rmd
    Modified:   code/BothFracDTPlotGeneRegions.sh
    Modified:   code/Snakefile
    Deleted:    code/Upstream10Bases_general.py
    Modified:   code/apaQTLCorrectPvalMakeQQ.R
    Modified:   code/apaQTL_Nominal.sh
    Modified:   code/apaQTL_permuted.sh
    Modified:   code/apaQTLsnake.err
    Modified:   code/bam2bw.sh
    Modified:   code/bed2saf.py
    Modified:   code/cluster.json
    Modified:   code/clusterfiltPAS.json
    Modified:   code/config.yaml
    Modified:   code/environment.yaml
    Modified:   code/makePheno.py
    Deleted:    code/test.txt

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These are the previous versions of the R Markdown and HTML files. If you’ve configured a remote Git repository (see ?wflow_git_remote), click on the hyperlinks in the table below to view them.

File Version Author Date Message
Rmd b7c8ed1 brimittleman 2019-06-13 fix big bugg
html 71146f1 brimittleman 2019-04-29 Build site.
Rmd 3c5e041 brimittleman 2019-04-29 add write out for qtls
html 9490b23 brimittleman 2019-04-29 Build site.
Rmd b18b96c brimittleman 2019-04-29 fix distance
html 2d33728 brimittleman 2019-04-28 Build site.
Rmd 7416404 brimittleman 2019-04-28 add res
html ed97e35 brimittleman 2019-04-21 Build site.
Rmd be90ded brimittleman 2019-04-21 fix to 5perc phenp
html 28bd046 brimittleman 2019-04-18 Build site.
Rmd 017f5c0 brimittleman 2019-04-18 add map apa qtl pipeline

library(tidyverse)
── Attaching packages ─────────────────────────────────────────────────────────────── tidyverse 1.2.1 ──
✔ ggplot2 3.1.1       ✔ purrr   0.3.2  
✔ tibble  2.1.1       ✔ dplyr   0.8.0.1
✔ tidyr   0.8.3       ✔ stringr 1.3.1  
✔ readr   1.3.1       ✔ forcats 0.3.0  
── Conflicts ────────────────────────────────────────────────────────────────── tidyverse_conflicts() ──
✖ dplyr::filter() masks stats::filter()
✖ dplyr::lag()    masks stats::lag()
library(reshape2)

Attaching package: 'reshape2'
The following object is masked from 'package:tidyr':

    smiths
library(workflowr)
This is workflowr version 1.3.0
Run ?workflowr for help getting started
library(cowplot)

Attaching package: 'cowplot'
The following object is masked from 'package:ggplot2':

    ggsave

In this analysis I will call apaQTls in both fractions. I will start with the phenotype files and normalized the counts using the leafcutter package in order to run the fastq QTL mapper.

Prepare phenotypes for QTL- phenotype dir

It is best to run this analysis in the data/phenotype_5perc directory. I have copied the leafcutter prepare_phenotype_table.py to the code directroy to use here.

#!/bin/bash
module load python

gzip APApeak_Phenotype_GeneLocAnno.Total.5perc.fc
gzip APApeak_Phenotype_GeneLocAnno.Nuclear.5perc.fc

python ../../code/prepare_phenotype_table.py APApeak_Phenotype_GeneLocAnno.Total.5perc.fc.gz
python ../../code/prepare_phenotype_table.py APApeak_Phenotype_GeneLocAnno.Nuclear.5perc.fc.gz

This will output bash scripts to run.

module load Anaconda3
source activate three-prime-env

sh APApeak_Phenotype_GeneLocAnno.Nuclear.5perc.fc.gz_prepare.sh
sh APApeak_Phenotype_GeneLocAnno.Total.5perc.fc.gz_prepare.sh

Subset the PCs to use the first 2 in the qtl calling:

module load Anaconda3
source activate three-prime-env

head -n 3 APApeak_Phenotype_GeneLocAnno.Nuclear.5perc.fc.gz.PCs > APApeak_Phenotype_GeneLocAnno.Nuclear.5perc.fc.gz.2PCs
head -n 3 APApeak_Phenotype_GeneLocAnno.Total.5perc.fc.gz.PCs > APApeak_Phenotype_GeneLocAnno.Total.5perc.fc.gz.2PCs

Call QTLs- code dir

Next I will need to make a sample list. From the code directory:

python makeSampleList.py

remove 19092

Prepare directroy

mkdir ../data/apaQTLNominal
mkdir ../data/apaQTLPermuted

Run the code to call QTLs within 1mb of each PAS peak. I run both a nominal pass and a permuted pas. The permulted pas chosses the best snp for each peak gene pair.

sbatch apaQTL_Nominal.sh
sbatch apaQTL_permuted.sh

Concatinate all of the results in the permuted set. I do this so I can account for multiple testing with the benjamini hochberg test.

Concatinate results in permuted directory:

cat APApeak_Phenotype_GeneLocAnno.Total.5perc.fc.gz.qqnorm_chr* > APApeak_Phenotype_GeneLocAnno.Total_permRes.txt

cat APApeak_Phenotype_GeneLocAnno.Nuclear.5perc.fc.gz.qqnorm_chr* > APApeak_Phenotype_GeneLocAnno.Nuclear_permRes.txt
 

Run correction script

Rscript apaQTLCorrectPvalMakeQQ.R  

Evaluation results

totRes=read.table("../data/apaQTLPermuted/APApeak_Phenotype_GeneLocAnno.Total_permResBH.txt", stringsAsFactors = F, header = T) %>% separate(pid, into=c("Chr", "Start", "End", "PeakID"), sep=":") %>% separate(PeakID, into=c("Gene", "Loc", "Strand","Peak"), sep="_")

Total Apa QTLs

TotQTLs= totRes %>% filter(-log10(bh)>=1)
nrow(TotQTLs)
[1] 382

apaQTL genes:

TotQTLs_gene=TotQTLs %>% group_by(Gene)  %>% summarise(nQTL=n())

summary(TotQTLs_gene$nQTL)
   Min. 1st Qu.  Median    Mean 3rd Qu.    Max. 
  1.000   1.000   1.000   1.224   1.000   3.000 
hist(TotQTLs_gene$nQTL)

Version Author Date
9490b23 brimittleman 2019-04-29
2d33728 brimittleman 2019-04-28

Location distribution for peaks:

TotQTLs_loc= TotQTLs %>% group_by(Loc) %>% summarise(nLoc=n()) %>% mutate(PropLoc=nLoc/nrow(TotQTLs))


totQTLloc=ggplot(TotQTLs_loc, aes(x=Loc, y=PropLoc, fill=Loc)) + geom_bar(stat = "Identity") + labs(x="Location of Significant Peak", y="Proportion of QTLs", title="Total QTL peak distribution")+ theme(axis.text.x = element_text(angle = 90, hjust = 1))
nucRes=read.table("../data/apaQTLPermuted/APApeak_Phenotype_GeneLocAnno.Nuclear_permResBH.txt", stringsAsFactors = F, header = T) %>% separate(pid, into=c("Chr", "Start", "End", "PeakID"), sep=":") %>% separate(PeakID, into=c("Gene", "Loc", "Strand","Peak"), sep="_")

Nuclear Apa QTLs

NucQTLs= nucRes %>% filter(-log10(bh)>=1)
nrow(NucQTLs)
[1] 702

apaQTL genes:

NucQTLs_gene= NucQTLs %>% group_by(Gene)  %>% summarise(nQTL=n())

summary(NucQTLs_gene$nQTL)
   Min. 1st Qu.  Median    Mean 3rd Qu.    Max. 
  1.000   1.000   1.000   1.249   1.000   4.000 
hist(NucQTLs_gene$nQTL)

Version Author Date
9490b23 brimittleman 2019-04-29
2d33728 brimittleman 2019-04-28

Location distribution for peaks:

NucQTLs_loc= NucQTLs %>% group_by(Loc) %>% summarise(nLoc=n()) %>% mutate(PropLoc=nLoc/nrow(NucQTLs))


nucQTLloc=ggplot(NucQTLs_loc, aes(x=Loc, y=PropLoc, fill=Loc)) + geom_bar(stat = "Identity") + labs(x="Location of Significant Peak", y="Proportion of QTLs", title="Nuclear QTL peak distribution")+theme(axis.text.x = element_text(angle = 90, hjust = 1))
plot_grid(totQTLloc, nucQTLloc)

Version Author Date
9490b23 brimittleman 2019-04-29
2d33728 brimittleman 2019-04-28
write.table(TotQTLs, file="../data/apaQTLs/Total_apaQTLs_5fdr.txt", col.names = T, row.names = F, quote=F)

write.table(NucQTLs, file="../data/apaQTLs/Nuclear_apaQTLs_5fdr.txt", col.names = T, row.names = F, quote=F)

sessionInfo()
R version 3.5.1 (2018-07-02)
Platform: x86_64-pc-linux-gnu (64-bit)
Running under: Scientific Linux 7.4 (Nitrogen)

Matrix products: default
BLAS/LAPACK: /software/openblas-0.2.19-el7-x86_64/lib/libopenblas_haswellp-r0.2.19.so

locale:
 [1] LC_CTYPE=en_US.UTF-8       LC_NUMERIC=C              
 [3] LC_TIME=en_US.UTF-8        LC_COLLATE=en_US.UTF-8    
 [5] LC_MONETARY=en_US.UTF-8    LC_MESSAGES=en_US.UTF-8   
 [7] LC_PAPER=en_US.UTF-8       LC_NAME=C                 
 [9] LC_ADDRESS=C               LC_TELEPHONE=C            
[11] LC_MEASUREMENT=en_US.UTF-8 LC_IDENTIFICATION=C       

attached base packages:
[1] stats     graphics  grDevices utils     datasets  methods   base     

other attached packages:
 [1] cowplot_0.9.4   workflowr_1.3.0 reshape2_1.4.3  forcats_0.3.0  
 [5] stringr_1.3.1   dplyr_0.8.0.1   purrr_0.3.2     readr_1.3.1    
 [9] tidyr_0.8.3     tibble_2.1.1    ggplot2_3.1.1   tidyverse_1.2.1

loaded via a namespace (and not attached):
 [1] Rcpp_1.0.0       cellranger_1.1.0 pillar_1.3.1     compiler_3.5.1  
 [5] git2r_0.25.2     plyr_1.8.4       tools_3.5.1      digest_0.6.18   
 [9] lubridate_1.7.4  jsonlite_1.6     evaluate_0.12    nlme_3.1-137    
[13] gtable_0.2.0     lattice_0.20-38  pkgconfig_2.0.2  rlang_0.3.1     
[17] cli_1.0.1        rstudioapi_0.10  yaml_2.2.0       haven_1.1.2     
[21] withr_2.1.2      xml2_1.2.0       httr_1.3.1       knitr_1.20      
[25] hms_0.4.2        generics_0.0.2   fs_1.2.6         rprojroot_1.3-2 
[29] grid_3.5.1       tidyselect_0.2.5 glue_1.3.0       R6_2.3.0        
[33] readxl_1.1.0     rmarkdown_1.10   modelr_0.1.2     magrittr_1.5    
[37] whisker_0.3-2    backports_1.1.2  scales_1.0.0     htmltools_0.3.6 
[41] rvest_0.3.2      assertthat_0.2.0 colorspace_1.3-2 labeling_0.3    
[45] stringi_1.2.4    lazyeval_0.2.1   munsell_0.5.0    broom_0.5.1     
[49] crayon_1.3.4