Last updated: 2022-04-15
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Knit directory: Serreze-T1D_Workflow/
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Unstaged changes:
Modified: analysis/4.1.1_qtl.analysis_binary_ici-early.vs.pbs_5.batches.Rmd
Modified: analysis/4.1.1_qtl.analysis_binary_ici-early.vs.pbs_5.batches_mis.Rmd
Modified: analysis/4.1.1_qtl.analysis_binary_ici-early.vs.pbs_snpsqc_5.batches.Rmd
Modified: analysis/4.1.1_qtl.analysis_binary_ici-early.vs.pbs_snpsqc_5.batches_mis.Rmd
Modified: analysis/4.1.1_qtl.analysis_binary_ici-early.vs.pbs_snpsqc_dis_no-x_updated_5.batches.Rmd
Modified: analysis/4.1.1_qtl.analysis_binary_ici-early.vs.pbs_snpsqc_dis_no-x_updated_5.batches_mis.Rmd
Modified: analysis/4.1.1_qtl.analysis_binary_ici.vs.eoi_snpsqc_dis_no-x_updated.Rmd
Modified: analysis/4.1.1_qtl.analysis_binary_ici.vs.pbs_snpsqc_dis_no-x_updated.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_age_ici-early.vs.pbs_pheno.corrected.cleaned_5.batches.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_age_ici-early.vs.pbs_pheno.corrected.cleaned_5.batches_mis.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_age_ici-early.vs.pbs_snpsqc_pheno.corrected.cleaned_5.batches.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_age_ici-early.vs.pbs_snpsqc_pheno.corrected.cleaned_5.batches_mis.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_age_ici-early.vs.pbs_snpsqc_pheno.corrected.cleaned_dis_no-xk_5.batches.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_age_ici-early.vs.pbs_snpsqc_pheno.corrected.cleaned_dis_no-xk_5.batches_mis.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_age_ici.vs.eoi_pheno.corrected.cleaned_5.batches.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_age_ici.vs.eoi_pheno.corrected.cleaned_5.batches_mis.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_age_ici.vs.eoi_snpsqc_pheno.corrected.cleaned_5.batches.Rmd
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Modified: analysis/4.1.2_qtl.analysis_cont_age_ici.vs.eoi_snpsqc_pheno.corrected.cleaned_dis_no-xk_5.batches.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_age_ici.vs.eoi_snpsqc_pheno.corrected.cleaned_dis_no-xk_5.batches_mis.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_age_ici.vs.pbs_pheno.corrected.cleaned_5.batches.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_age_ici.vs.pbs_pheno.corrected.cleaned_5.batches_mis.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_age_ici.vs.pbs_snpsqc_pheno.corrected.cleaned_5.batches.Rmd
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Modified: analysis/4.1.2_qtl.analysis_cont_age_ici.vs.pbs_snpsqc_pheno.corrected.cleaned_dis_no-xk_5.batches_mis.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_rz.age_ici-early.vs.pbs_pheno.corrected.cleaned_5.batches.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_rz.age_ici-early.vs.pbs_pheno.corrected.cleaned_5.batches_mis.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_rz.age_ici-early.vs.pbs_snpsqc_pheno.corrected.cleaned_5.batches.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_rz.age_ici-early.vs.pbs_snpsqc_pheno.corrected.cleaned_5.batches_mis.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_rz.age_ici-early.vs.pbs_snpsqc_pheno.corrected.cleaned_dis_no-xk_5.batches.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_rz.age_ici-early.vs.pbs_snpsqc_pheno.corrected.cleaned_dis_no-xk_5.batches_mis.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_rz.age_ici.vs.eoi_pheno.corrected.cleaned_5.batches.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_rz.age_ici.vs.eoi_pheno.corrected.cleaned_5.batches_mis.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_rz.age_ici.vs.eoi_snpsqc_pheno.corrected.cleaned_5.batches.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_rz.age_ici.vs.eoi_snpsqc_pheno.corrected.cleaned_5.batches_mis.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_rz.age_ici.vs.eoi_snpsqc_pheno.corrected.cleaned_dis_no-xk_5.batches.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_rz.age_ici.vs.eoi_snpsqc_pheno.corrected.cleaned_dis_no-xk_5.batches_mis.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_rz.age_ici.vs.pbs_pheno.corrected.cleaned_5.batches.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_rz.age_ici.vs.pbs_pheno.corrected.cleaned_5.batches_mis.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_rz.age_ici.vs.pbs_snpsqc_pheno.corrected.cleaned_5.batches.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_rz.age_ici.vs.pbs_snpsqc_pheno.corrected.cleaned_5.batches_mis.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_rz.age_ici.vs.pbs_snpsqc_pheno.corrected.cleaned_dis_no-xk_5.batches.Rmd
Modified: analysis/4.1.2_qtl.analysis_cont_rz.age_ici.vs.pbs_snpsqc_pheno.corrected.cleaned_dis_no-xk_5.batches_mis.Rmd
Modified: analysis/index_5.batches.Rmd
Modified: analysis/index_5.batches_additional.Rmd
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Rmd | a8c2d1a | Belinda Cornes | 2022-04-13 | additonal analysis - peaks and continuous variables |
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We will load the data and subset indivials out that are in the groups of interest. We will create a binary phenotype from this (PBS ==0, ICI-Early == 1).
load("data/gm_allqc_5.batches.RData")
#gm_allqc
gm=gm_allqc
gm
Object of class cross2 (crosstype "bc")
Total individuals 308
No. genotyped individuals 308
No. phenotyped individuals 308
No. with both geno & pheno 308
No. phenotypes 1
No. covariates 6
No. phenotype covariates 0
No. chromosomes 20
Total markers 34537
No. markers by chr:
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16
2643 2629 1857 1890 1774 1941 1672 1627 1878 1176 1871 1300 1549 1578 1257 935
17 18 19 X
501 913 1014 4532
#removing ici-late
table(gm$covar$group)
(A2 Parental) (DQ8 Parental) B6.g7 Parental EOI F1
2 2 1 164 1
ICI PBS
104 34
ici.late_ids <- gm$covar[gm$covar$"diabetic status" == "T1D>17",]$id
length(ici.late_ids)
[1] 17
ici.late_ids
[1] "NG00198-ICI-LATE" "NG00329-ICI-LATE" "NG00343-ICI-LATE" "NG00386-ICI-LATE"
[5] "NG00442-ICI-LATE" "NG00443-ICI-LATE" "NG00526-ICI-LATE" "NG00522-ICI-LATE"
[9] "NG00790-ICI-LATE" "NG00874-ICI-LATE" "NG00929-ICI-LATE" "NG01225-ICI-LATE"
[13] "NG01303-ICI-LATE" "NG01020-ICI-LATE" "NG01397-ICI-LATE" "NG01389-ICI-LATE"
[17] "NG01548-ICI-LATE"
gm <- gm[paste0("-",as.character(ici.late_ids)),]
##extracting animals with ici-early and pbs group status
miceinfo <- gm$covar[gm$covar$group == "PBS" | gm$covar$group == "ICI",]
table(miceinfo$group)
ICI PBS
87 34
mice.ids <- rownames(miceinfo)
gm <- gm[mice.ids]
gm
Object of class cross2 (crosstype "bc")
Total individuals 121
No. genotyped individuals 121
No. phenotyped individuals 121
No. with both geno & pheno 121
No. phenotypes 1
No. covariates 6
No. phenotype covariates 0
No. chromosomes 20
Total markers 34537
No. markers by chr:
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16
2643 2629 1857 1890 1774 1941 1672 1627 1878 1176 1871 1300 1549 1578 1257 935
17 18 19 X
501 913 1014 4532
#pr.qc <- pr
#for (i in 1:20){pr.qc[[i]] = pr.qc[[i]][mice.ids,,]}
#bin_pheno <- NULL
#bin_pheno$PBS <- ifelse(gm$covar$group == "PBS", 1, 0)
#bin_pheno$ICI-Early <- ifelse(gm$covar$group == "ICI-Early", 1, 0)
#bin_pheno <- as.data.frame(bin_pheno)
#rownames(bin_pheno) <- rownames(gm$covar)
gm$covar$ICI_Early.vs.PBS <- ifelse(gm$covar$group == "PBS", 0, 1)
gm.full <- gm
##removing problmetic marker
gm <- drop_markers(gm, "UNCHS013106")
markers <- marker_names(gm)
gmapdf <- read.csv("/Users/corneb/Documents/MyJax/CS/Projects/Serreze/haplotype.reconstruction/output_5.batches/genetic_map.csv")
pmapdf <- read.csv("/Users/corneb/Documents/MyJax/CS/Projects/Serreze/haplotype.reconstruction/output_5.batches/physical_map.csv")
#mapdf <- merge(gmapdf,pmapdf, by=c("marker","chr"), all=T)
#rownames(mapdf) <- mapdf$marker
#mapdf <- mapdf[markers,]
#names(mapdf) <- c('marker','chr','gmapdf','pmapdf')
#mapdfnd <- mapdf[!duplicated(mapdf[c(2:3)]),]
pr.qc <- calc_genoprob(gm)
gm
Object of class cross2 (crosstype "bc")
Total individuals 121
No. genotyped individuals 121
No. phenotyped individuals 121
No. with both geno & pheno 121
No. phenotypes 1
No. covariates 7
No. phenotype covariates 0
No. chromosomes 20
Total markers 34537
No. markers by chr:
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16
2643 2629 1857 1890 1774 1941 1672 1627 1878 1176 1871 1300 1549 1578 1257 935
17 18 19 X
501 913 1014 4532
For each of the phenotype analyzed, permutations were used for each model to obtain genome-wide LOD significance threshold for p < 0.01, p < 0.05, p < 0.10, respectively, separately for X and automsomes (A).
The table shows the estimated significance thresholds from permutation test.
We also looked at the kinship to see how correlated each sample is. Kinship values between pairs of samples range between 0 (no relationship) and 1.0 (completely identical). The darker the colour the more indentical the pairs are.
Xcovar <- get_x_covar(gm)
#addcovar = model.matrix(~Sex, data = covars)[,-1]
#K <- calc_kinship(pr.qc, type = "loco")
#heatmap(K[[1]])
#K.overall <- calc_kinship(pr.qc, type = "overall")
#heatmap(K.overall)
kinship <- calc_kinship(pr.qc)
heatmap(kinship)
#operm <- scan1perm(pr.qc, gm$covar$phenos, Xcovar=Xcovar, n_perm=2000)
#operm <- scan1perm(pr.qc, gm$covar$phenos, addcovar = addcovar, n_perm=2000)
#operm <- scan1perm(pr.qc, gm$covar$phenos, n_perm=2000)
operm <- scan1perm(pr.qc, gm$covar["ICI_Early.vs.PBS"], model="binary", n_perm=10, perm_Xsp=TRUE, chr_lengths=chr_lengths(gm$gmap))
summary_table<-data.frame(unclass(summary(operm, alpha=c(0.01, 0.05, 0.1))))
names(summary_table) <- c("autosomes","X")
summary_table$significance.level <- rownames(summary_table)
rownames(summary_table) <- NULL
summary_table[c(3,1:2)] %>%
kable(escape = F,align = c("ccc")) %>%
kable_styling("striped", full_width = T) %>%
column_spec(1, bold=TRUE)
significance.level | autosomes | X |
---|---|---|
0.01 | 3.139211 | 3.482196 |
0.05 | 2.903903 | 3.464086 |
0.1 | 2.609035 | 3.440403 |
The figures below show QTL maps for each phenotype
out <- scan1(pr.qc, gm$covar["ICI_Early.vs.PBS"], Xcovar=Xcovar, model="binary")
summary_table<-data.frame(unclass(summary(operm, alpha=c(0.01, 0.05, 0.1))))
plot_lod<-function(out,map){
for (i in 1:dim(out)[2]){
#png(filename=paste0("/Users/chenm/Documents/qtl/Jai/",colnames(out)[i], "_lod.png"))
ymx <- maxlod(out) # overall maximum LOD score
plot(out, map, lodcolumn=i, col="slateblue", ylim=c(0, ymx+0.5))
#legend("topright", lwd=2, colnames(out)[i], bg="gray90")
title(main = paste0(colnames(out)[i], " [positions in cM]"))
add_threshold(map, summary(operm,alpha=0.1), col = 'purple')
add_threshold(map, summary(operm, alpha=0.05), col = 'red')
add_threshold(map, summary(operm, alpha=0.01), col = 'blue')
#par(mar=c(5.1, 6.1, 1.1, 1.1))
ymx <- 11 # overall maximum LOD score
plot(out, map, lodcolumn=i, col="slateblue", ylim=c(0, ymx+0.5))
#legend("topright", lwd=2, colnames(out)[i], bg="gray90")
title(main = paste0(colnames(out)[i], " [positions in cM] \n(using same scale as eoi vs. ici for easier comparison)"))
add_threshold(map, summary(operm, alpha=0.1), col = 'purple')
add_threshold(map, summary(operm, alpha=0.05), col = 'red')
add_threshold(map, summary(operm, alpha=0.01), col = 'blue')
#for (j in 1: dim(summary_table)[1]){
# abline(h=summary_table[j, i],col="red")
# text(x=400, y =summary_table[j, i]+0.12, labels = paste("p=", row.names(summary_table)[j]))
#}
#dev.off()
}
}
plot_lod(out,gm$gmap)
The table below shows QTL peaks associated with the phenotype. We use the 95% threshold from the permutations to find peaks.
peaks <- find_peaks(out, gm$gmap, threshold=summary(operm,alpha=0.05)$A, thresholdX = summary(operm,alpha=0.05)$X, peakdrop=3, drop=1.5)
if(nrow(peaks) >0){
peaks$marker <- find_marker(gm$gmap, chr=peaks$chr,pos=peaks$pos)
names(peaks)[2] <- c("phenotype")
peaks <- peaks[-1]
rownames(peaks) <- NULL
print(kable(peaks, escape = F, align = c("cccccccc"), "html")
%>% kable_styling("striped", full_width = T)%>%
column_spec(1, bold=TRUE)
)
#plot only peak chromosomes
plot_lod_chr<-function(out,map,chrom){
for (i in 1:dim(out)[2]){
#png(filename=paste0("/Users/chenm/Documents/qtl/Jai/",colnames(out)[i], "_lod.png"))
#par(mar=c(5.1, 6.1, 1.1, 1.1))
ymx <- maxlod(out) # overall maximum LOD score
plot(out, map, chr = chrom, lodcolumn=i, col="slateblue", ylim=c(0, ymx+0.5))
#legend("topright", lwd=2, colnames(out)[i], bg="gray90")
title(main = paste0(colnames(out)[i], " - chr", chrom, " [positions in cM]"))
add_threshold(map, summary(operm,alpha=0.1), col = 'purple')
add_threshold(map, summary(operm, alpha=0.05), col = 'red')
add_threshold(map, summary(operm, alpha=0.01), col = 'blue')
#for (j in 1: dim(summary_table)[1]){
# abline(h=summary_table[j, i],col="red")
# text(x=400, y =summary_table[j, i]+0.12, labels = paste("p=", row.names(summary_table)[j]))
#}
#dev.off()
ymx <- 11
plot(out, map, chr = chrom, lodcolumn=i, col="slateblue", ylim=c(0, ymx+0.5))
#legend("topright", lwd=2, colnames(out)[i], bg="gray90")
title(main = paste0(colnames(out)[i], " - chr", chrom, " [positions in cM]\n(using same scale as eoi vs. ici for easier comparison)"))
add_threshold(map, summary(operm,alpha=0.1), col = 'purple')
add_threshold(map, summary(operm, alpha=0.05), col = 'red')
add_threshold(map, summary(operm, alpha=0.01), col = 'blue')
}
}
for(i in unique(peaks$chr)){
#for (i in 1:nrow(peaks)){
#plot_lod_chr(out,gm$gmap, peaks$chr[i])
plot_lod_chr(out,gm$gmap, i)
}
} else {
print(paste0("There are no peaks that have a LOD that reaches suggestive (p<0.05) level of ",summary(operm,alpha=0.05)$A, " [autosomes]/",summary(operm,alpha=0.05)$X, " [x-chromosome]"))
}
[1] “There are no peaks that have a LOD that reaches suggestive (p<0.05) level of 2.90390330401799 [autosomes]/3.46408571465806 [x-chromosome]”
print("peaks in MB positions")
[1] “peaks in MB positions”
peaks_mba <- find_peaks(out, gm$pmap, threshold=summary(operm,alpha=0.05)$A, thresholdX = summary(operm,alpha=0.05)$X, peakdrop=3, drop=1.5)
if(nrow(peaks) >0){
peaks_mba$marker <- find_marker(gm$pmap, chr=peaks_mba$chr,pos=peaks_mba$pos)
names(peaks_mba)[2] <- c("phenotype")
peaks_mba <- peaks_mba[-1]
#peaks_mbl <- list()
##corresponding info in Mb
#for(i in 1:nrow(peaks)){
# #lodindex <- peaks$lodindex[i]
# phenotype <- peaks$phenotype[i]
# chr <- as.character(peaks$chr[i])
# lod <- peaks$lod[i]
# mark <- peaks$marker[i]
# pos <- mapdf[mapdf$marker==mark,]$pmapdf
# ci_lo <- mapdfnd$pmapdf[which(mapdfnd$gmapdf == peaks$ci_lo[i] & mapdfnd$chr == peaks$chr[i])]
# ci_hi <- mapdfnd$pmapdf[which(mapdfnd$gmapdf == peaks$ci_hi[i] & mapdfnd$chr == peaks$chr[i])]
# peaks_mb=as.data.frame(cbind(phenotype, chr, pos, lod, ci_lo, ci_hi, mark))
# names(peaks_mb)[7] <- c("marker")
# peaks_mbl[[i]] <- peaks_mb
#}
#peaks_mba2 <- do.call(rbind, peaks_mbl)
#peaks_mba2 <- as.data.frame(peaks_mba)
#peaks_mba[,c("chr", "pos", "lod", "ci_lo", "ci_hi")] <- sapply(peaks_mba[,c("chr", "pos", "lod", "ci_lo", "ci_hi")], as.numeric)
rownames(peaks_mba) <- NULL
print(kable(peaks_mba, escape = F, align = c("cccccccc"), "html")
%>% kable_styling("striped", full_width = T)%>%
column_spec(1, bold=TRUE)
)
plot_lod_chr_mb<-function(out,map,chrom){
for (i in 1:dim(out)[2]){
#png(filename=paste0("/Users/chenm/Documents/qtl/Jai/",colnames(out)[i], "_lod.png"))
#par(mar=c(5.1, 6.1, 1.1, 1.1))
ymx <- maxlod(out) # overall maximum LOD score
plot(out, map, chr = chrom, lodcolumn=i, col="slateblue", ylim=c(0, ymx+0.5))
#legend("topright", lwd=2, colnames(out)[i], bg="gray90")
title(main = paste0(colnames(out)[i], " - chr", chrom, " [positions in MB]"))
add_threshold(map, summary(operm,alpha=0.1), col = 'purple')
add_threshold(map, summary(operm, alpha=0.05), col = 'red')
add_threshold(map, summary(operm, alpha=0.01), col = 'blue')
#for (j in 1: dim(summary_table)[1]){
# abline(h=summary_table[j, i],col="red")
# text(x=400, y =summary_table[j, i]+0.12, labels = paste("p=", row.names(summary_table)[j]))
#}
#dev.off()
ymx <- 11
plot(out, map, chr = chrom, lodcolumn=i, col="slateblue", ylim=c(0, ymx+0.5))
#legend("topright", lwd=2, colnames(out)[i], bg="gray90")
title(main = paste0(colnames(out)[i], " - chr", chrom, " [positions in MB]\n(using same scale as eoi vs. ici for easier comparison)"))
add_threshold(map, summary(operm,alpha=0.1), col = 'purple')
add_threshold(map, summary(operm, alpha=0.05), col = 'red')
add_threshold(map, summary(operm, alpha=0.01), col = 'blue')
}
}
for(i in unique(peaks_mba$chr)){
#for (i in 1:nrow(peaks_mba)){
#plot_lod_chr_mb(out,gm$pmap, peaks_mba$chr[i])
plot_lod_chr_mb(out,gm$pmap,i)
}
} else {
print(paste0("There are no peaks that have a LOD that reaches suggestive (p<0.05) level of ",summary(operm,alpha=0.05)$A, " [autosomes]/",summary(operm,alpha=0.05)$X, " [x-chromosome]"))
}
[1] “There are no peaks that have a LOD that reaches suggestive (p<0.05) level of 2.90390330401799 [autosomes]/3.46408571465806 [x-chromosome]”
For each peak LOD location we give a list of gene
query_variants <- create_variant_query_func("/Users/corneb/Documents/MyJax/CS/Projects/support.files/qtl2/cc_variants.sqlite")
query_genes <- create_gene_query_func("/Users/corneb/Documents/MyJax/CS/Projects/support.files/qtl2/mouse_genes_mgi.sqlite")
if(nrow(peaks) >0){
for (i in 1:nrow(peaks)){
#for (i in 1:1){
#Plot 1
g <- maxmarg(pr.qc, gm$gmap, chr=peaks$chr[i], pos=peaks$pos[i], return_char=TRUE)
#png(filename=paste0("/Users/chenm/Documents/qtl/Jai/","qtl_effect_", i, ".png"))
#par(mar=c(4.1, 4.1, 1.5, 0.6))
plot_pxg(g, gm$covar[,peaks$phenotype[i]], ylab=peaks$phenotype[i], sort=FALSE)
title(main = paste0("chr: ", chr=peaks$chr[i], "pos: ", peaks$pos[i], "cM /",peaks_mba$pos[i],"MB\n(",peaks$phenotype[i]," )"), line=0.2)
##dev.off()
chr = peaks$chr[i]
# Plot 2
pr_sub <- pull_genoprobint(pr.qc, gm$gmap, chr, c(peaks$ci_lo[i], peaks$ci_hi[i]))
#coeff <- scan1coef(pr[,chr], cross$pheno[,peaks$lodcolumn[i]], addcovar = addcovar)
#coeff <- scan1coef(pr[,chr], cross$pheno[,peaks$lodcolumn[i]], Xcovar=Xcovar)
#coeff <- scan1coef(pr.qc[,chr], gm$covar[peaks$lodcolumn[i]], model="binary")
#coeff_sub <- scan1coef(pr_sub[,chr], gm$covar[peaks$lodcolumn[i]], model="binary")
blup <- scan1blup(pr.qc[,chr], gm$covar[peaks$phenotype[i]])
blup_sub <- scan1blup(pr_sub[,chr], gm$covar[peaks$phenotype[i]])
write.csv(as.data.frame(blup_sub), paste0("data/ici-early.vs.pbs_blup_sub_chr-",chr,"_peak.marker-",peaks$marker[i],"_lod.drop-1.5_5.batches.csv"), quote=F)
#plot_coef(coeff,
# gm$gmap, columns=1:2,
# bgcolor="gray95", legend="bottomleft",
# main = paste("chr", chr=peaks$chr[i], "pos: ", peaks$pos[i], "cM /",peaks_mba$pos[i],"MB\n(",peaks$lodcolumn[i]," [scan1coeff; positions in cM])")
# )
#plot_coef(coeff_sub,
# gm$gmap, columns=1:2,
# bgcolor="gray95", legend="bottomleft",
# main = paste("chr", chr=peaks$chr[i], "pos: ", peaks$pos[i], "cM /",peaks_mba$pos[i],"MB\n(",peaks$lodcolumn[i],"; 1.5 LOD drop interval [scan1coeff; positions in cM] ) ")
# )
plot_coef(blup,
gm$gmap, columns=1:2,
bgcolor="gray95", legend="bottomleft",
main = paste0("chr: ", chr=peaks$chr[i], "pos: ", peaks$pos[i], "cM /",peaks_mba$pos[i],"MB\n(",peaks$phenotype[i]," [scan1blup; positions in cM])")
)
plot_coef(blup_sub,
gm$gmap, columns=1:2,
bgcolor="gray95", legend="bottomleft",
main = paste0("chr: ", chr=peaks$chr[i], "pos: ", peaks$pos[i], "cM /",peaks_mba$pos[i],"MB\n(",peaks$phenotype[i],"; 1.5 LOD drop interval [scan1blup; positions in cM])")
)
# Plot 3
#c2effB <- scan1coef(pr.qc[,chr], gm$covar[peaks$lodcolumn[i]], model="binary", contrasts=cbind(a=c(-1, 0), d=c(0, -1)))
#c2effBb <- scan1blup(pr.qc[,chr], gm$covar[peaks$lodcolumn[i]], contrasts=cbind(a=c(-1, 0), d=c(0, -1)))
##c2effB <- scan1coef(pr[,chr], cross$pheno[,peaks$lodcolumn[i]], addcovar = addcovar, contrasts=cbind(mu=c(1,1,1), a=c(-1, 0, 1), d=c(0, 1, 0)))
##c2effB <- scan1coef(pr[,chr], cross$pheno[,peaks$lodcolumn[i]],Xcovar=Xcovar, contrasts=cbind(mu=c(1,1,1), a=c(-1, 0, 1), d=c(0, 1, 0)))
#plot(c2effB, gm$gmap[chr], columns=1:2,
# bgcolor="gray95", legend="bottomleft",
# main = paste("chr", chr=peaks$chr[i], "pos", peaks$pos[i], "(",peaks$lodcolumn[i],")")
# )
#plot(c2effBb, gm$gmap[chr], columns=1:2,
# bgcolor="gray95", legend="bottomleft",
# main = paste("chr", chr=peaks$chr[i], "pos", peaks$pos[i], "(",peaks$lodcolumn[i],")")
# )
##last_coef <- unclass(c2effB)[nrow(c2effB),2:3] # last two coefficients
##for(t in seq(along=last_coef))
## axis(side=4, at=last_coef[t], names(last_coef)[t], tick=FALSE)
#Table 1
chr = peaks_mba$chr[i]
start=as.numeric(peaks_mba$ci_lo[i])
end=as.numeric(peaks_mba$ci_hi[i])
genesgss = query_genes(chr, start, end)
write.csv(genesgss, file=paste0("data/ici-early.vs.pbs_genes_chr-",chr,"_peak.marker-",peaks$marker[i],"_lod.drop-1.5_5.batches.csv"), quote=F)
rownames(genesgss) <- NULL
genesgss$strand_old = genesgss$strand
genesgss$strand[genesgss$strand=="+"] <- "positive"
genesgss$strand[genesgss$strand=="-"] <- "negative"
#genesgss <-
#table <-
#genesgss[,c("chr","type","start","stop","strand","ID","Name","Dbxref","gene_id","mgi_type","description")] %>%
#kable(escape = F,align = c("ccccccccccc")) %>%
#kable_styling("striped", full_width = T) #%>%
#cat #%>%
#column_spec(1, bold=TRUE)
#
#print(kable(genesgss[,c("chr","type","start","stop","strand","ID","Name","Dbxref","gene_id","mgi_type","description")], escape = F,align = c("ccccccccccc")))
print(kable(genesgss[,c("chr","type","start","stop","strand","ID","Name","Dbxref","gene_id","mgi_type","description")], "html") %>% kable_styling("striped", full_width = T))
#table
}
} else {
print(paste0("There are no peaks that have a LOD that reaches suggestive (p<0.05) level of ",summary(operm,alpha=0.05)$A, " [autosomes]/",summary(operm,alpha=0.05)$X, " [x-chromosome]"))
}
[1] “There are no peaks that have a LOD that reaches suggestive (p<0.05) level of 2.90390330401799 [autosomes]/3.46408571465806 [x-chromosome]”
gm
Object of class cross2 (crosstype "bc")
Total individuals 121
No. genotyped individuals 121
No. phenotyped individuals 121
No. with both geno & pheno 121
No. phenotypes 1
No. covariates 7
No. phenotype covariates 0
No. chromosomes 20
Total markers 34537
No. markers by chr:
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16
2643 2629 1857 1890 1774 1941 1672 1627 1878 1176 1871 1300 1549 1578 1257 935
17 18 19 X
501 913 1014 4532
#detach("package:qtl2", unload=TRUE)
#library(qtl)
cross <- qtl::read.cross("csv", file = "data/ici-early.vs.pbs_gm_qtl_5.batches.csv",alleles=c("A","B"))
--Read the following data:
121 individuals
34537 markers
3 phenotypes
--Cross type: bc
cross <- qtl::jittermap(cross)
summary(cross)
Backcross
No. individuals: 121
No. phenotypes: 3
Percent phenotyped: 100 100 100
No. chromosomes: 20
Autosomes: 1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19
X chr: X
Total markers: 34537
No. markers: 2643 2629 1857 1890 1774 1941 1672 1627 1878 1176 1871
1300 1549 1578 1257 935 501 913 1014 4532
Percent genotyped: 99.3
Genotypes (%):
Autosomes: AA:59.9 AB:40.1
X chromosome: AA:95.9 AB:4.1
cross.probs <- qtl::calc.genoprob(cross)
print("method == hk")
[1] "method == hk"
scanone.hk <-qtl::scanone(cross.probs, pheno.col="ICI_Early.vs.PBS" , model="binary", method="hk")
operm.hk <- qtl::scanone(cross.probs, method = "hk", pheno.col="ICI_Early.vs.PBS", n.perm = 10, perm.Xsp = TRUE, model="binary", verbose=FALSE)
plot(operm.hk)
print(summary(operm.hk, alpha=c(0.01, 0.05, 0.1)))
Autosome LOD thresholds (10 permutations)
lod
1% 3.65
5% 3.56
10% 3.45
X chromosome LOD thresholds (181 permutations)
lod
1% 3.49
5% 3.49
10% 3.49
#plot(scanone.hk, bandcol = "grey90",lty=1, cex=1, col = "steelblue")
#qtl::add.threshold(scanone.hk, perms= operm.hk, alpha=0.01, col = 'blue')
#qtl::add.threshold(scanone.hk, perms= operm.hk, alpha=0.05, col = 'red')
#qtl::add.threshold(scanone.hk, perms= operm.hk, alpha=0.1, col = 'purple')
ymx <- maxlod(out) # overall maximum LOD score
plot(scanone.hk, bandcol = "grey90",lty=1, cex=1, col = "slateblue", ylim=c(0, ymx+0.5))
title(main = paste0(colnames(out), " [positions in cM]"))
qtl::add.threshold(scanone.hk, perms= operm.hk, alpha=0.01, col = 'blue')
qtl::add.threshold(scanone.hk, perms= operm.hk, alpha=0.05, col = 'red')
qtl::add.threshold(scanone.hk, perms= operm.hk, alpha=0.1, col = 'purple')
ymx <- 11
plot(scanone.hk, bandcol = "grey90",lty=1, cex=1, col = "slateblue", ylim=c(0, ymx+0.5))
title(main = paste0(colnames(out), " [positions in cM]\n(using same scale as eoi vs. ici for easier comparison)"))
qtl::add.threshold(scanone.hk, perms= operm.hk, alpha=0.01, col = 'blue')
qtl::add.threshold(scanone.hk, perms= operm.hk, alpha=0.05, col = 'red')
qtl::add.threshold(scanone.hk, perms= operm.hk, alpha=0.1, col = 'purple')
print(as.data.frame(summary(scanone.hk, perms=operm.hk, pvalues=TRUE, format="allpeaks")))
chr pos lod pval
UNC163443 1 4.774084 1.0738719 1.0000000
UNCHS005128 2 35.575604 1.4775915 1.0000000
UNC5265500 3 23.363432 1.2956551 1.0000000
UNCHS012528 4 53.470029 1.3628070 1.0000000
JAX00591328 5 52.052170 1.4109255 1.0000000
UNCHS016657 6 10.674201 0.9142663 1.0000000
UNC13819275 7 69.998488 0.8929144 1.0000000
UNCHS023364 8 35.540889 1.2408211 1.0000000
UNC17298291 9 73.251870 1.3049246 1.0000000
UNCHS029562 10 77.099163 0.8825381 1.0000000
UNCHS030476 11 28.025737 0.8874757 1.0000000
ICR4362 12 8.289190 1.2763929 1.0000000
UNC22620355 13 28.179586 0.9768557 1.0000000
UNCHS038071 14 22.374371 1.0506503 1.0000000
UNC25285746 15 12.031164 1.0377531 1.0000000
sanger1606q 16 18.965164 0.8858403 1.0000000
UNCHS044622 17 31.021132 1.6037504 1.0000000
UNC28774893 18 8.231033 1.1276765 1.0000000
UNCHS047043 19 3.158002 1.7114108 1.0000000
XiB2 X 45.699832 1.6966992 0.9999632
print("all peaks with a p-value less or equal to 0.05 (suggestive)")
[1] "all peaks with a p-value less or equal to 0.05 (suggestive)"
print(as.data.frame(summary(scanone.hk, perms=operm.hk, alpha=0.05, pvalues=TRUE, format="allpeaks")))
[1] chr pos lod
<0 rows> (or 0-length row.names)
#print("method == ehk")
#scanone.ehk <-qtl::scanone(cross.probs, pheno.col="ICI_Early.vs.PBS" , model="binary", method="ehk")
#operm.ehk <- qtl::scanone(cross.probs, method = "ehk", pheno.col="ICI_Early.vs.PBS", n.perm = 1000, perm.Xsp = TRUE, model="binary", verbose=FALSE)
#plot(operm.ehk)
#print(summary(operm.ehk, alpha=c(0.01, 0.05, 0.1)))
#plot(scanone.ehk, bandcol = "grey90",lty=1, cex=1, col = "steelblue")
#qtl::add.threshold(scanone.ehk, perms= operm.ehk, alpha=0.01, col = 'blue')
#qtl::add.threshold(scanone.ehk, perms= operm.ehk, alpha=0.05, col = 'red')
#qtl::add.threshold(scanone.ehk, perms= operm.ehk, alpha=0.1, col = 'purple')
#print(as.data.frame(summary(scanone.ehk)))
#print(as.data.frame(summary(scanone.ehk, perms=operm.ehk, alpha=0.05, pvalues=TRUE, format="allpeaks")))
R version 3.6.2 (2019-12-12)
Platform: x86_64-apple-darwin15.6.0 (64-bit)
Running under: macOS Catalina 10.15.7
Matrix products: default
BLAS: /Library/Frameworks/R.framework/Versions/3.6/Resources/lib/libRblas.0.dylib
LAPACK: /Library/Frameworks/R.framework/Versions/3.6/Resources/lib/libRlapack.dylib
locale:
[1] en_AU.UTF-8/en_AU.UTF-8/en_AU.UTF-8/C/en_AU.UTF-8/en_AU.UTF-8
attached base packages:
[1] stats graphics grDevices utils datasets methods base
other attached packages:
[1] abind_1.4-5 qtl2_0.22 reshape2_1.4.4 ggplot2_3.3.5
[5] tibble_3.1.2 psych_2.0.7 readxl_1.3.1 cluster_2.1.0
[9] dplyr_1.0.8 optparse_1.6.6 rhdf5_2.28.1 mclust_5.4.6
[13] tidyr_1.0.2 data.table_1.14.0 knitr_1.33 kableExtra_1.1.0
[17] workflowr_1.6.2
loaded via a namespace (and not attached):
[1] httr_1.4.1 bit64_4.0.5 viridisLite_0.4.0 assertthat_0.2.1
[5] highr_0.9 blob_1.2.1 cellranger_1.1.0 yaml_2.2.1
[9] pillar_1.6.1 RSQLite_2.2.7 backports_1.2.1 lattice_0.20-38
[13] glue_1.4.2 digest_0.6.27 promises_1.1.0 rvest_0.3.5
[17] colorspace_2.0-2 htmltools_0.5.1.1 httpuv_1.5.2 plyr_1.8.6
[21] pkgconfig_2.0.3 purrr_0.3.4 scales_1.1.1 webshot_0.5.2
[25] qtl_1.46-2 whisker_0.4 getopt_1.20.3 later_1.0.0
[29] git2r_0.26.1 generics_0.0.2 ellipsis_0.3.2 cachem_1.0.5
[33] withr_2.4.2 cli_3.0.0 mnormt_1.5-7 magrittr_2.0.1
[37] crayon_1.4.1 memoise_2.0.0 evaluate_0.14 fs_1.4.1
[41] fansi_0.5.0 nlme_3.1-142 xml2_1.3.1 tools_3.6.2
[45] hms_0.5.3 lifecycle_1.0.1 stringr_1.4.0 Rhdf5lib_1.6.3
[49] munsell_0.5.0 compiler_3.6.2 rlang_1.0.2 grid_3.6.2
[53] rstudioapi_0.13 rmarkdown_2.1 gtable_0.3.0 DBI_1.1.1
[57] R6_2.5.0 fastmap_1.1.0 bit_4.0.4 utf8_1.2.1
[61] rprojroot_1.3-2 readr_1.3.1 stringi_1.7.2 parallel_3.6.2
[65] Rcpp_1.0.7 vctrs_0.3.8 tidyselect_1.1.2 xfun_0.24