Peak coverage along Gene examples
Briana Mittleman
11/12/2018
Last updated: 2018-11-13
workflowr checks: (Click a bullet for more information)-
✔ R Markdown file: up-to-date
Great! Since the R Markdown file has been committed to the Git repository, you know the exact version of the code that produced these results.
-
✔ Environment: empty
Great job! The global environment was empty. Objects defined in the global environment can affect the analysis in your R Markdown file in unknown ways. For reproduciblity it’s best to always run the code in an empty environment.
-
✔ Seed:
set.seed(12345)The command
set.seed(12345)was run prior to running the code in the R Markdown file. Setting a seed ensures that any results that rely on randomness, e.g. subsampling or permutations, are reproducible. -
✔ Session information: recorded
Great job! Recording the operating system, R version, and package versions is critical for reproducibility.
-
Great! You are using Git for version control. Tracking code development and connecting the code version to the results is critical for reproducibility. The version displayed above was the version of the Git repository at the time these results were generated.✔ Repository version: f8d8c94
Note that you need to be careful to ensure that all relevant files for the analysis have been committed to Git prior to generating the results (you can usewflow_publishorwflow_git_commit). workflowr only checks the R Markdown file, but you know if there are other scripts or data files that it depends on. Below is the status of the Git repository when the results were generated:
Note that any generated files, e.g. HTML, png, CSS, etc., are not included in this status report because it is ok for generated content to have uncommitted changes.Ignored files: Ignored: .DS_Store Ignored: .Rhistory Ignored: .Rproj.user/ Ignored: data/.DS_Store Ignored: output/.DS_Store Untracked files: Untracked: KalistoAbundance18486.txt Untracked: analysis/ncbiRefSeq_sm.sort.mRNA.bed Untracked: analysis/snake.config.notes.Rmd Untracked: analysis/verifyBAM.Rmd Untracked: data/18486.genecov.txt Untracked: data/APApeaksYL.total.inbrain.bed Untracked: data/ChromHmmOverlap/ Untracked: data/GM12878.chromHMM.bed Untracked: data/GM12878.chromHMM.txt Untracked: data/NuclearApaQTLs.txt Untracked: data/PeaksUsed/ Untracked: data/RNAkalisto/ Untracked: data/TotalApaQTLs.txt Untracked: data/Totalpeaks_filtered_clean.bed Untracked: data/YL-SP-18486-T-combined-genecov.txt Untracked: data/YL-SP-18486-T_S9_R1_001-genecov.txt Untracked: data/apaExamp/ Untracked: data/bedgraph_peaks/ Untracked: data/bin200.5.T.nuccov.bed Untracked: data/bin200.Anuccov.bed Untracked: data/bin200.nuccov.bed Untracked: data/clean_peaks/ Untracked: data/comb_map_stats.csv Untracked: data/comb_map_stats.xlsx Untracked: data/comb_map_stats_39ind.csv Untracked: data/combined_reads_mapped_three_prime_seq.csv Untracked: data/diff_iso_trans/ Untracked: data/ensemble_to_genename.txt Untracked: data/example_gene_peakQuant/ Untracked: data/filtered_APApeaks_merged_allchrom_refseqTrans.closest2End.bed Untracked: data/filtered_APApeaks_merged_allchrom_refseqTrans.closest2End.noties.bed Untracked: data/first50lines_closest.txt Untracked: data/gencov.test.csv Untracked: data/gencov.test.txt Untracked: data/gencov_zero.test.csv Untracked: data/gencov_zero.test.txt Untracked: data/gene_cov/ Untracked: data/joined Untracked: data/leafcutter/ Untracked: data/merged_combined_YL-SP-threeprimeseq.bg Untracked: data/mol_overlap/ Untracked: data/mol_pheno/ Untracked: data/nom_QTL/ Untracked: data/nom_QTL_opp/ Untracked: data/nom_QTL_trans/ Untracked: data/nuc6up/ Untracked: data/other_qtls/ Untracked: data/peakPerRefSeqGene/ Untracked: data/perm_QTL/ Untracked: data/perm_QTL_opp/ Untracked: data/perm_QTL_trans/ Untracked: data/reads_mapped_three_prime_seq.csv Untracked: data/smash.cov.results.bed Untracked: data/smash.cov.results.csv Untracked: data/smash.cov.results.txt Untracked: data/smash_testregion/ Untracked: data/ssFC200.cov.bed Untracked: data/temp.file1 Untracked: data/temp.file2 Untracked: data/temp.gencov.test.txt Untracked: data/temp.gencov_zero.test.txt Untracked: output/picard/ Untracked: output/plots/ Untracked: output/qual.fig2.pdf Unstaged changes: Modified: analysis/28ind.peak.explore.Rmd Modified: analysis/39indQC.Rmd Modified: analysis/cleanupdtseq.internalpriming.Rmd Modified: analysis/coloc_apaQTLs_protQTLs.Rmd Modified: analysis/dif.iso.usage.leafcutter.Rmd Modified: analysis/diff_iso_pipeline.Rmd Modified: analysis/explore.filters.Rmd Modified: analysis/flash2mash.Rmd Modified: analysis/overlapMolQTL.Rmd Modified: analysis/overlap_qtls.Rmd Modified: analysis/peakOverlap_oppstrand.Rmd Modified: analysis/pheno.leaf.comb.Rmd Modified: analysis/swarmPlots_QTLs.Rmd Modified: analysis/test.max2.Rmd Modified: code/Snakefile
Expand here to see past versions:
The quantified peak files are:
- /project2/gilad/briana/threeprimeseq/data/filtPeakOppstrand_cov/filtered_APApeaks_merged_allchrom_refseqGenes.Transcript_sm_quant.Nuclear_fixed.fc
- /project2/gilad/briana/threeprimeseq/data/filtPeakOppstrand_cov/filtered_APApeaks_merged_allchrom_refseqGenes.Transcript_sm_quant.Total_fixed.fc
I want to grep specific genes and look at the read distribution for peaks along a gene. In these files the peakIDs stil have the peak locations. Before I ran the QTL analysis I changed the final coverage (ex /project2/gilad/briana/threeprimeseq/data/phenotypes_filtPeakTranscript/filtered_APApeaks_merged_allchrom_refseqGenes.Transcript_sm_quant.Nuclear.pheno_fixed.txt.gz.qqnorm_chr$i.gz) to have the TSS as the ID.
Librarys
library(workflowr)This is workflowr version 1.1.1
Run ?workflowr for help getting startedlibrary(reshape2)
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 1.3.1
✔ readr 1.1.1 ✔ forcats 0.3.0── Conflicts ────────────────────────────────────────────────────────────────────────────── tidyverse_conflicts() ──
✖ dplyr::filter() masks stats::filter()
✖ dplyr::lag() masks stats::lag()library(VennDiagram)Loading required package: gridLoading required package: futile.loggerlibrary(data.table)
Attaching package: 'data.table'The following objects are masked from 'package:dplyr':
between, first, lastThe following object is masked from 'package:purrr':
transposeThe following objects are masked from 'package:reshape2':
dcast, meltlibrary(ggpubr)Loading required package: magrittr
Attaching package: 'magrittr'The following object is masked from 'package:purrr':
set_namesThe following object is masked from 'package:tidyr':
extract
Attaching package: 'ggpubr'The following object is masked from 'package:VennDiagram':
rotatelibrary(cowplot)
Attaching package: 'cowplot'The following object is masked from 'package:ggpubr':
get_legendThe following object is masked from 'package:ggplot2':
ggsavenuc_names=c('Geneid', 'Chr', 'Start', 'End', 'Strand', 'Length', '18486_N' ,'18497_N', '18500_N' ,'18505_N', '18508_N' ,'18511_N', '18519_N', '18520_N', '18853_N' ,'18858_N', '18861_N', '18870_N' ,'18909_N' ,'18912_N' ,'18916_N', '19092_N' ,'19093_N', '19119_N', '19128_N' ,'19130_N', '19131_N' ,'19137_N', '19140_N', '19141_N' ,'19144_N', '19152_N' ,'19153_N', '19160_N' ,'19171_N', '19193_N' ,'19200_N', '19207_N', '19209_N', '19210_N', '19223_N' ,'19225_N', '19238_N' ,'19239_N', '19257_N')
tot_names=c('Geneid', 'Chr' ,'Start', 'End', 'Strand', 'Length', '18486_T', '18497_T' ,'18500_T','18505_T', '18508_T' ,'18511_T', '18519_T', '18520_T', '18853_T', '18858_T', '18861_T', '18870_T', '18909_T' ,'18912_T', '18916_T', '19092_T' ,'19093_T', '19119_T', '19128_T', '19130_T', '19131_T' ,'19137_T', '19140_T' ,'19141_T', '19144_T', '19152_T' ,'19153_T', '19160_T' ,'19171_T', '19193_T', '19200_T', '19207_T' ,'19209_T' ,'19210_T', '19223_T', '19225_T', '19238_T', '19239_T', '19257_T')NuclearAPA=read.table("../data/perm_QTL_trans/filtered_APApeaks_merged_allchrom_refseqGenes_pheno_Nuclear_transcript_permResBH.txt", stringsAsFactors = F, header=T) %>% mutate(sig=ifelse(-log10(bh)>=1, 1,0 )) %>% separate(pid, sep = ":", into=c("chr", "start", "end", "id")) %>% separate(id, sep = "_", into=c("gene", "strand", "peak")) %>% filter(sig==1)
totalAPA=read.table("../data/perm_QTL_trans/filtered_APApeaks_merged_allchrom_refseqGenes_pheno_Total_transcript_permResBH.txt", stringsAsFactors = F, header=T) %>% mutate(sig=ifelse(-log10(bh)>=1, 1,0 )) %>% separate(pid, sep = ":", into=c("chr", "start", "end", "id")) %>% separate(id, sep = "_", into=c("gene", "strand", "peak")) %>% filter(sig==1)examples to look at Nuclear: IRF5, HSF1, NOL9,DCAF16,
Total: NBEAL2, SACM1L, COX7A2L
#nuclear
grep IRF5 /project2/gilad/briana/threeprimeseq/data/filtPeakOppstrand_cov/filtered_APApeaks_merged_allchrom_refseqGenes.Transcript_sm_quant.Nuclear_fixed.fc > /project2/gilad/briana/threeprimeseq/data/example_gene_peakQuant/IRF5_NuclearCov_peaks.txt
grep HSF1 /project2/gilad/briana/threeprimeseq/data/filtPeakOppstrand_cov/filtered_APApeaks_merged_allchrom_refseqGenes.Transcript_sm_quant.Nuclear_fixed.fc > /project2/gilad/briana/threeprimeseq/data/example_gene_peakQuant/HSF1_NuclearCov_peaks.txt
grep NOL9 /project2/gilad/briana/threeprimeseq/data/filtPeakOppstrand_cov/filtered_APApeaks_merged_allchrom_refseqGenes.Transcript_sm_quant.Nuclear_fixed.fc > /project2/gilad/briana/threeprimeseq/data/example_gene_peakQuant/NOL9_NuclearCov_peaks.txt
grep DCAF16 /project2/gilad/briana/threeprimeseq/data/filtPeakOppstrand_cov/filtered_APApeaks_merged_allchrom_refseqGenes.Transcript_sm_quant.Nuclear_fixed.fc > /project2/gilad/briana/threeprimeseq/data/example_gene_peakQuant/DCAF16_NuclearCov_peaks.txt
grep PPP4C /project2/gilad/briana/threeprimeseq/data/filtPeakOppstrand_cov/filtered_APApeaks_merged_allchrom_refseqGenes.Transcript_sm_quant.Nuclear_fixed.fc > /project2/gilad/briana/threeprimeseq/data/example_gene_peakQuant/PPP4C_NuclearCov_peaks.txt
#total
grep NBEAL2 /project2/gilad/briana/threeprimeseq/data/filtPeakOppstrand_cov/filtered_APApeaks_merged_allchrom_refseqGenes.Transcript_sm_quant.Total_fixed.fc > /project2/gilad/briana/threeprimeseq/data/example_gene_peakQuant/NBEAL2_TotalCov_peaks.txt
grep SACM1L /project2/gilad/briana/threeprimeseq/data/filtPeakOppstrand_cov/filtered_APApeaks_merged_allchrom_refseqGenes.Transcript_sm_quant.Total_fixed.fc > /project2/gilad/briana/threeprimeseq/data/example_gene_peakQuant/SACM1L_TotalCov_peaks.txt
grep TESK1 /project2/gilad/briana/threeprimeseq/data/filtPeakOppstrand_cov/filtered_APApeaks_merged_allchrom_refseqGenes.Transcript_sm_quant.Total_fixed.fc > /project2/gilad/briana/threeprimeseq/data/example_gene_peakQuant/TESK1_TotalCov_peaks.txt
grep DGCR14 /project2/gilad/briana/threeprimeseq/data/filtPeakOppstrand_cov/filtered_APApeaks_merged_allchrom_refseqGenes.Transcript_sm_quant.Total_fixed.fc > /project2/gilad/briana/threeprimeseq/data/example_gene_peakQuant/DGCR14_TotalCov_peaks.txt
Copy these to my computer so I can work with them here. I am going to want to make a function that makes the histogram reproducibly for anyfile. I will need to know how many bins to include in the histogram. First I will make the graph for one example then I will make it more general.
Files are in /Users/bmittleman1/Documents/Gilad_lab/threeprimeseq/data/example_gene_peakQuant
Start wit a small file.
pos=c(3,4,7:39)
PPP4c=read.table("../data/example_gene_peakQuant/PPP4C_NuclearCov_peaks.txt", stringsAsFactors = F, col.names = nuc_names) %>% select(pos)
PPP4c$peaks=seq(0, (nrow(PPP4c)-1))
PPP4c_melt=melt(PPP4c, id.vars=c('peaks','Start','End'))Plot:
ggplot(PPP4c_melt, aes(x=peaks, y=value, by=variable, fill=variable)) + geom_histogram(stat="identity")Warning: Ignoring unknown parameters: binwidth, bins, pad
Try with actual location as the center of the peak.
pos=c(3,4,7:39)
PPP4c_2=read.table("../data/example_gene_peakQuant/PPP4C_NuclearCov_peaks.txt", stringsAsFactors = F, col.names = tot_names) %>% select(pos)
PPP4c_2$peaks=seq(0, (nrow(PPP4c_2)-1))
PPP4c_2= PPP4c_2 %>% mutate(PeakCenter=(Start+ (End-Start)/2))
PPP4c2_melt=melt(PPP4c_2, id.vars=c('peaks','PeakCenter', "Start", "End"))
colnames(PPP4c2_melt)= c('peaks','PeakCenter', "Start", "End", "Individual", "ReadCount")Plot:
ggplot(PPP4c2_melt, aes(x=PeakCenter, y=ReadCount, by=Individual, fill=Individual)) + geom_histogram(stat="identity") + labs(title="Peak Coverage and Location PP4c")Warning: Ignoring unknown parameters: binwidth, bins, pad
Generalize this for more genes:
makePeakLocplot=function(file, geneName,fraction){
pos=c(3,4,7:39)
if (fraction=="Total"){
gene=read.table(file, stringsAsFactors = F, col.names = tot_names) %>% select(pos)
}
else{
gene=read.table(file, stringsAsFactors = F, col.names = nuc_names) %>% select(pos)
}
gene$peaks=seq(0, (nrow(gene)-1))
gene= gene %>% mutate(PeakCenter=(Start+ (End-Start)/2))
gene_melt=melt(gene, id.vars=c('peaks','PeakCenter', "Start", "End"))
colnames(gene_melt)= c('peaks','PeakCenter', "Start", "End", "Individual", "ReadCount")
finalplot=ggplot(gene_melt, aes(x=PeakCenter, y=ReadCount, by=Individual, fill=Individual)) + geom_histogram(stat="identity", show.legend = FALSE) + labs(title=paste("Peak Coverage and Location", geneName, sep = " "))
return(finalplot)
}Try for another gene:
makePeakLocplot("../data/example_gene_peakQuant/PPP4C_NuclearCov_peaks.txt",'PPP4c',"Nuclear")Warning: Ignoring unknown parameters: binwidth, bins, pad
makePeakLocplot("../data/example_gene_peakQuant/DCAF16_NuclearCov_peaks.txt",'DCAF16',"Nuclear")Warning: Ignoring unknown parameters: binwidth, bins, pad
makePeakLocplot("../data/example_gene_peakQuant/DGCR14_TotalCov_peaks.txt",'DGCR14',"Total")Warning: Ignoring unknown parameters: binwidth, bins, pad
makePeakLocplot("../data/example_gene_peakQuant/IRF5_NuclearCov_peaks.txt",'IRF5',"Nuclear")Warning: Ignoring unknown parameters: binwidth, bins, pad
makePeakLocplot("../data/example_gene_peakQuant/HSF1_NuclearCov_peaks.txt",'HSF1',"Nuclear")Warning: Ignoring unknown parameters: binwidth, bins, pad
makePeakLocplot("../data/example_gene_peakQuant/NOL9_NuclearCov_peaks.txt",'NOL9',"Nuclear")Warning: Ignoring unknown parameters: binwidth, bins, pad
makePeakLocplot("../data/example_gene_peakQuant/SACM1L_TotalCov_peaks.txt",'SACM1L',"Total")Warning: Ignoring unknown parameters: binwidth, bins, pad
Make a function to do this by peak number (ignoring direction)
makePeakNumplot=function(file, geneName,fraction){
pos=c(7:39)
if (fraction=="Total"){
gene=read.table(file, stringsAsFactors = F, col.names = tot_names) %>% select(pos)
}
else{
gene=read.table(file, stringsAsFactors = F, col.names = nuc_names) %>% select(pos)
}
gene$peaks=seq(0, (nrow(gene)-1))
gene_melt=melt(gene, id.vars=c('peaks'))
colnames(gene_melt)= c('peaks',"Individual", "ReadCount")
finalplot=ggplot(gene_melt, aes(x=peaks, y=ReadCount, by=Individual, fill=Individual)) + geom_histogram(stat="identity", show.legend = FALSE) + labs(title=paste("Peak Coverage", geneName, sep = " "))
return(finalplot)
}I can plot them next to eachother using cowplot
ppp4c_loc=makePeakLocplot("../data/example_gene_peakQuant/PPP4C_NuclearCov_peaks.txt",'PPP4c',"Nuclear")Warning: Ignoring unknown parameters: binwidth, bins, padppp4c_num=makePeakNumplot("../data/example_gene_peakQuant/PPP4C_NuclearCov_peaks.txt",'PPP4c',"Nuclear")Warning: Ignoring unknown parameters: binwidth, bins, padplot_grid(ppp4c_loc,ppp4c_num)
dcaf16_loc=makePeakLocplot("../data/example_gene_peakQuant/DCAF16_NuclearCov_peaks.txt",'DCAF16',"Nuclear")Warning: Ignoring unknown parameters: binwidth, bins, paddcaf16_num=makePeakNumplot("../data/example_gene_peakQuant/DCAF16_NuclearCov_peaks.txt",'DCAF16',"Nuclear")Warning: Ignoring unknown parameters: binwidth, bins, padplot_grid(dcaf16_loc,dcaf16_num)
dgcr14_loc=makePeakLocplot("../data/example_gene_peakQuant/DGCR14_TotalCov_peaks.txt",'DGCR14',"Total")Warning: Ignoring unknown parameters: binwidth, bins, paddgcr14_num=makePeakNumplot("../data/example_gene_peakQuant/DGCR14_TotalCov_peaks.txt",'DGCR14',"Total")Warning: Ignoring unknown parameters: binwidth, bins, padplot_grid(dgcr14_loc,dgcr14_num)
irf5_loc=makePeakLocplot("../data/example_gene_peakQuant/IRF5_NuclearCov_peaks.txt",'IRF5',"Nuclear")Warning: Ignoring unknown parameters: binwidth, bins, padirf5_num=makePeakNumplot("../data/example_gene_peakQuant/IRF5_NuclearCov_peaks.txt",'IRF5',"Nuclear")Warning: Ignoring unknown parameters: binwidth, bins, padplot_grid(irf5_loc,irf5_num)
HSF1_loc=makePeakLocplot("../data/example_gene_peakQuant/HSF1_NuclearCov_peaks.txt",'HSF1',"Nuclear")Warning: Ignoring unknown parameters: binwidth, bins, padHSF1_num=makePeakNumplot("../data/example_gene_peakQuant/HSF1_NuclearCov_peaks.txt",'HSF1',"Nuclear")Warning: Ignoring unknown parameters: binwidth, bins, padplot_grid(HSF1_loc,HSF1_num)
NOL9_loc=makePeakLocplot("../data/example_gene_peakQuant/NOL9_NuclearCov_peaks.txt",'NOL9',"Nuclear")Warning: Ignoring unknown parameters: binwidth, bins, padNOL9_num=makePeakNumplot("../data/example_gene_peakQuant/NOL9_NuclearCov_peaks.txt",'NOL9',"Nuclear")Warning: Ignoring unknown parameters: binwidth, bins, padplot_grid(NOL9_loc,NOL9_num)
SACM1L_loc=makePeakLocplot("../data/example_gene_peakQuant/SACM1L_TotalCov_peaks.txt",'SACM1L',"Total")Warning: Ignoring unknown parameters: binwidth, bins, padSACM1L_num=makePeakNumplot("../data/example_gene_peakQuant/SACM1L_TotalCov_peaks.txt",'SACM1L',"Total")Warning: Ignoring unknown parameters: binwidth, bins, padplot_grid(SACM1L_loc,SACM1L_num)
Session information
sessionInfo()R version 3.5.1 (2018-07-02)
Platform: x86_64-apple-darwin15.6.0 (64-bit)
Running under: macOS Sierra 10.12.6
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] grid stats graphics grDevices utils datasets methods
[8] base
other attached packages:
[1] bindrcpp_0.2.2 cowplot_0.9.3 ggpubr_0.1.8
[4] magrittr_1.5 data.table_1.11.8 VennDiagram_1.6.20
[7] futile.logger_1.4.3 forcats_0.3.0 stringr_1.3.1
[10] dplyr_0.7.6 purrr_0.2.5 readr_1.1.1
[13] tidyr_0.8.1 tibble_1.4.2 ggplot2_3.0.0
[16] tidyverse_1.2.1 reshape2_1.4.3 workflowr_1.1.1
loaded via a namespace (and not attached):
[1] tidyselect_0.2.4 haven_1.1.2 lattice_0.20-35
[4] colorspace_1.3-2 htmltools_0.3.6 yaml_2.2.0
[7] rlang_0.2.2 R.oo_1.22.0 pillar_1.3.0
[10] glue_1.3.0 withr_2.1.2 R.utils_2.7.0
[13] lambda.r_1.2.3 modelr_0.1.2 readxl_1.1.0
[16] bindr_0.1.1 plyr_1.8.4 munsell_0.5.0
[19] gtable_0.2.0 cellranger_1.1.0 rvest_0.3.2
[22] R.methodsS3_1.7.1 evaluate_0.11 labeling_0.3
[25] knitr_1.20 broom_0.5.0 Rcpp_0.12.19
[28] formatR_1.5 backports_1.1.2 scales_1.0.0
[31] jsonlite_1.5 hms_0.4.2 digest_0.6.17
[34] stringi_1.2.4 rprojroot_1.3-2 cli_1.0.1
[37] tools_3.5.1 lazyeval_0.2.1 futile.options_1.0.1
[40] crayon_1.3.4 whisker_0.3-2 pkgconfig_2.0.2
[43] xml2_1.2.0 lubridate_1.7.4 assertthat_0.2.0
[46] rmarkdown_1.10 httr_1.3.1 rstudioapi_0.8
[49] R6_2.3.0 nlme_3.1-137 git2r_0.23.0
[52] compiler_3.5.1
This reproducible R Markdown analysis was created with workflowr 1.1.1