IHWpaper 1.22.0
library(dplyr)
library(IHW)
library(fdrtool)
library(ggplot2)
library(cowplot)
theme_set(theme_cowplot())
library(tidyr)
library(scales)
library(latex2exp)
Let us start by loading in the data:
file_loc <- system.file("extdata","real_data", "hqtl_chrom1_chrom2", package = "IHWpaper")
First the two tables with the p-values corresponding to the two chromosomes. Note that only p-values <= 1e-4 are stored in these.
chr1_df <- readRDS(file.path(file_loc, "chr1_subset.Rds"))
chr2_df <- readRDS(file.path(file_loc, "chr2_subset.Rds"))
pval_threshold <- 10^(-4)
Also recall each hypothesis corresponds to a peak (which we call gene below) and a SNP. Hence let us load files about each of the SNPs and peaks:
snp_chr1 <- readRDS(file.path(file_loc, "snppos_chr1.Rds"))
snp_chr2 <- readRDS(file.path(file_loc, "snppos_chr2.Rds"))
all_peaks <- readRDS(file.path(file_loc, "peak_locations.Rds"))
peaks_chr1 <- dplyr::filter(all_peaks, chr=="chr1")
peaks_chr2 <- dplyr::filter(all_peaks, chr=="chr2")
We can use these both to infer how many hypotheses were conducted in total (or at a given distance), but also to calculate our covariates which are a function of SNP and peak (their distance).
Now let us attach the new column with the covariate (distance) to the data frames.
chr1_df <- left_join(chr1_df, select(snp_chr1, snp, pos), by=(c("SNP"="snp"))) %>%
left_join(peaks_chr1, by=(c("gene"="id"))) %>%
mutate( dist = pmin( abs(pos-start), abs(pos-end)))
chr2_df <- left_join(chr2_df, select(snp_chr2, snp, pos), by=(c("SNP"="snp"))) %>%
left_join(peaks_chr2, by=(c("gene"="id"))) %>%
mutate( dist = pmin( abs(pos-start), abs(pos-end)))
Now let us convert the distance to a categorical covariate by binning:
my_breaks <- c(-1,
seq(from=10000,to=290000, by=10000) ,
seq(from=300000, to=0.9*10^6, by=100000),
seq(from=10^6, to=25.1*10^7, by=10^7))
myf1 <- cut(chr1_df$dist, my_breaks)
myf2 <- cut(chr2_df$dist, my_breaks)
To apply our method despite the fact that only small p-values are available, we will count how many hypotheses there are in each of the bins. The above code is not very efficient, so we have precomputed the results and do not run the below chunk.
cnt = 0
ms <- rep(0, length(levels(myf1)))
pb = txtProgressBar(min = 0, max = nrow(peaks_chr1), initial = 0)
for (i in 1:nrow(peaks_chr1)){
setTxtProgressBar(pb,i)
start_pos <- peaks_chr1$start[i]
end_pos <- peaks_chr1$end[i]
dist_vec <- pmin( abs(snp_chr1$pos - start_pos), abs(snp_chr1$pos - end_pos) )
ms <- ms + table(cut(dist_vec, my_breaks))
}
saveRDS( ms, file = "m_groups_chr1.Rds" )
cnt = 0
ms_chr2 <- table(myf2)*0
pb = txtProgressBar(min = 0, max = nrow(peaks_chr2), initial = 0)
for (i in 1:nrow(peaks_chr2)){
setTxtProgressBar(pb,i)
start_pos <- peaks_chr1$start[i]
end_pos <- peaks_chr1$end[i]
dist_vec <- pmin( abs(snp_chr2$pos - start_pos), abs(snp_chr2$pos - end_pos) )
ms_chr2 <- ms_chr2 + table(cut(dist_vec, my_breaks))
}
saveRDS( ms_chr2, file = "m_groups_chr2.Rds" )
Let us load the result from the above execution:
ms_chr1 <- readRDS(file.path(file_loc, "m_groups_chr1.Rds"))
ms_chr2 <- readRDS(file.path(file_loc, "m_groups_chr2.Rds"))
Let us put the data for the two chromosomes together:
chr1_chr2_df <- rbind(chr1_df, chr2_df)
chr1_chr2_groups <- as.factor(c(myf1,myf2))
folds_vec <- as.factor(c(rep(1, nrow(chr1_df)), rep(2, nrow(chr2_df))))
m_groups <- cbind(ms_chr1, ms_chr2)
m <- sum(m_groups) #total number of hypotheses
m
## [1] 15725016812
Get our colors:
beyonce_colors <- c("#b72da0", "#7c5bd2", "#0097ed","#00c6c3",
"#9cd78a", "#f7f7a7", "#ebab5f", "#e24344",
"#04738d")#,"#d8cdc9")
beyonce_colors[6] <- c("#dbcb09") # thicker yellow
pretty_colors <- beyonce_colors[c(2,1,3:5)]
qs <- c(0.025, 0.05)
cutoffs <- c(0, quantile(chr1_chr2_df$dist,qs), Inf)
cov_scatter_gg <- ggplot(chr1_chr2_df, aes(x=rank(dist)/nrow(chr1_chr2_df),
y=-log10(pvalue))) +
geom_bin2d(bins=150, drop=TRUE) + # geom_point(alpha=0.2, col=pretty_colors[1]) +
geom_vline(xintercept=qs, linetype="dashed") +
ylab(expression(paste(-log[10],"(p-value)"))) +
xlab(expression(paste("Quantile of distance"))) +
scale_fill_gradientn(trans="log10", colors=alpha(pretty_colors[1], c(0.2,1)))
cov_scatter_gg
ggsave(cov_scatter_gg, filename="cov_scatter_gg.pdf", width=4,height=3)
chr1_chr2_df$cutoff_groups <- cut(chr1_chr2_df$dist, cutoffs)
table(chr1_chr2_df$cutoff_groups)
##
## (0,1.13e+05] (1.13e+05,2.34e+06] (2.34e+06,Inf]
## 60404 60404 2295337
First let us plot the marginal histogram:
gg_marginal_hist <- ggplot(chr1_chr2_df, aes(x=pvalue*10^4)) +
geom_histogram(aes(y=..density..), alpha=0.5, binwidth=0.05, boundary = 0, colour="black",fill=pretty_colors[1]) +
scale_x_continuous(expand = c(0.02, 0), breaks=c(0,0.5,1)) +
scale_y_continuous(expand = c(0.02, 0), limits=c(0,2.5)) +
ylab(expression(paste("Density")))+
xlab(TeX("p-value ($\\times 10^{-4}$)"))
gg_marginal_hist
ggsave(gg_marginal_hist, filename="gg_marginal_hist.pdf", width=4,height=3)
gg_stratified_hist <- ggplot(chr1_chr2_df, aes(x=pvalue*10^4)) +
geom_histogram(aes(y=..density..), alpha=0.5, binwidth=0.05, boundary = 0, colour="black",fill=pretty_colors[1]) +
scale_x_continuous(expand = c(0.02, 0), breaks=c(0,0.5,1)) +
scale_y_continuous(expand = c(0.02, 0), limits=c(0,11)) +
ylab("Density")+
xlab(TeX("p-value ($\\times 10^{-4}$)")) +
facet_grid(~cutoff_groups) +
theme(strip.background = element_blank(), strip.text.y = element_blank()) +
theme(panel.spacing = unit(2, "lines"))
gg_stratified_hist
ggsave(gg_stratified_hist, filename="gg_stratified_hist.pdf", width=7,height=3)
We want to apply the Benjamini-Yekutieli at alpha=0.1, thus we will apply Benjamini-Hochberg at the corrected level:
alpha <- .01/(log(m)+1)
Now let us run the IHW procedure:
ihw_chr1_chr2 <- ihw(chr1_chr2_df$pvalue, chr1_chr2_groups, alpha, folds=folds_vec,
m_groups=m_groups, lambdas=2000)
Rejections of BY:
sum(p.adjust(chr1_chr2_df$pvalue, n = m, method="BH") <= alpha)
## [1] 9110
Rejections of IHW-BY:
rejections(ihw_chr1_chr2)
## [1] 21903
So we see that discoveries have more than doubled.
What if we had applied BH and IHW-BH instead of BY and IHW-BY?
alpha_bh <- 0.01
ihw_chr1_chr2_bh <- ihw(chr1_chr2_df$pvalue, chr1_chr2_groups, alpha_bh,
folds=folds_vec, m_groups=m_groups, lambdas=2000)
sum(p.adjust(chr1_chr2_df$pvalue, n = m, method="BH") <= alpha_bh)
## [1] 19055
rejections(ihw_chr1_chr2_bh)
## [1] 52488
For our table we show one hypothesis on Chromosome 1 that gets rejected both times (by BH and IHW):
idx <- which(rejected_hypotheses(ihw_chr1_chr2) & (p.adjust(chr1_chr2_df$pvalue, n = m, method="BH") > alpha) &
(covariates(ihw_chr1_chr2)==3) & (ihw_chr1_chr2@df$fold == 1))
idx_max <- which.max(pvalues(ihw_chr1_chr2)[idx])
ihw_chr1_chr2@df[idx[idx_max],]
## [1] pvalue adj_pvalue weight weighted_pvalue
## [5] group covariate fold
## <0 rows> (or 0-length row.names)
chr1_df[idx[idx_max],]
## # A tibble: 0 × 11
## # … with 11 variables: SNP <chr>, gene <int>, beta <dbl>, tstat <dbl>,
## # pvalue <dbl>, FDR <dbl>, pos <int>, chr <chr>, start <int>, end <int>,
## # dist <int>
We show one hypothesis on Chromosome 1 that gets weight 0:
idx <- which( !rejected_hypotheses(ihw_chr1_chr2) & (p.adjust(chr1_chr2_df$pvalue, n = m, method="BH") > alpha) &
(covariates(ihw_chr1_chr2)==15) & (ihw_chr1_chr2@df$fold == 1))
idx_max <- which.max(pvalues(ihw_chr1_chr2)[idx])
ihw_chr1_chr2@df[idx[idx_max],]
## [1] pvalue adj_pvalue weight weighted_pvalue
## [5] group covariate fold
## <0 rows> (or 0-length row.names)
chr1_df[idx[idx_max],]
## # A tibble: 0 × 11
## # … with 11 variables: SNP <chr>, gene <int>, beta <dbl>, tstat <dbl>,
## # pvalue <dbl>, FDR <dbl>, pos <int>, chr <chr>, start <int>, end <int>,
## # dist <int>
Next we find a hypothesis which gets rejected in both cases from Chr2 :
idx <- which( rejected_hypotheses(ihw_chr1_chr2) & (p.adjust(chr1_chr2_df$pvalue, n = m, method="BH") <= alpha) &
(covariates(ihw_chr1_chr2)==3) & (ihw_chr1_chr2@df$fold == 2))
ihw_chr1_chr2@df[idx[9],]
## pvalue adj_pvalue weight weighted_pvalue group covariate fold
## NA NA NA NA NA <NA> <NA> <NA>
chr2_df[idx[9]-nrow(chr1_df),]
## # A tibble: 1 × 11
## SNP gene beta tstat pvalue FDR pos chr start end dist
## <chr> <int> <dbl> <dbl> <dbl> <dbl> <int> <chr> <int> <int> <int>
## 1 <NA> NA NA NA NA NA NA <NA> NA NA NA
And another one that only gets rejected in one case
idx <- which( rejected_hypotheses(ihw_chr1_chr2) & (p.adjust(chr1_chr2_df$pvalue, n = m, method="BH") > alpha) &
(covariates(ihw_chr1_chr2)==1) & (ihw_chr1_chr2@df$fold == 2))
idx_max <- which.max(pvalues(ihw_chr1_chr2)[idx])
ihw_chr1_chr2@df[idx[idx_max],]
## [1] pvalue adj_pvalue weight weighted_pvalue
## [5] group covariate fold
## <0 rows> (or 0-length row.names)
chr2_df[idx[idx_max]-nrow(chr1_df),]
## # A tibble: 0 × 11
## # … with 11 variables: SNP <chr>, gene <int>, beta <dbl>, tstat <dbl>,
## # pvalue <dbl>, FDR <dbl>, pos <int>, chr <chr>, start <int>, end <int>,
## # dist <int>
First get the threshold below which BY rejects:
t_bh <- get_bh_threshold(chr1_chr2_df$pvalue, alpha, mtests = m)
t_bh
## [1] 2.363825e-10
Next write a function to estimate the local fdr at a given threshold:
get_local_fdr <- function(fold, group){
idx <- (chr1_chr2_groups == group) & (folds_vec == fold)
pvals <- sort(chr1_chr2_df$pvalue[idx])
m_true <- m_groups[group,fold]
gren <- IHW:::presorted_grenander(pvals, m_true)
myt <- thresholds(ihw_chr1_chr2, levels_only=TRUE)[group,fold]
id_ihw_myt <- which(myt < gren$x.knots)[1]
local_fdr_ihw <- ifelse(myt == 0, 0, 1/gren$slope.knots[id_ihw_myt-1])
id_bh_thresh <- which(t_bh < gren$x.knots)[1]
local_fdr_bh <- 1/gren$slope.knots[id_bh_thresh-1]
pi0 <- (m_true - length(pvals))/(1-10^(-4))/m_true
data.frame(fold=fold, group=group, pi0=pi0, t_ihw=myt,
local_fdr_ihw = local_fdr_ihw,
local_fdr_bh = local_fdr_bh)
}
fold_groups <- expand.grid(1:62, 1:2)
Precompute the below too because it takes a while:
lfdrs <- bind_rows(mapply(get_local_fdr, fold_groups[[2]], fold_groups[[1]], SIMPLIFY = FALSE))
saveRDS(lfdrs,file="hqtl_estimated_lfdrs.Rds")
lfdrs <- readRDS(file.path(file_loc, "hqtl_estimated_lfdrs.Rds"))
lfdrs <- mutate(lfdrs, Chromosome=paste0("chr", fold), stratum=group, t_bh=t_bh)
breaks <- my_breaks/10^3
breaks <- breaks[-1]
break_min <- 3000/10^3
breaks_left <- c(break_min,breaks[-length(breaks)])
stratum <- 1:62
step_df_weight <- data.frame(stratum=stratum, chr2=weights(ihw_chr1_chr2,levels_only=TRUE)[,1],
chr1=weights(ihw_chr1_chr2, levels_only=TRUE)[,2] ) %>%
gather(Chromosome, weight , -stratum)
step_df_threshold <- data.frame(stratum=stratum,
chr2=thresholds(ihw_chr1_chr2,levels_only=TRUE)[,2],
chr1=thresholds(ihw_chr1_chr2, levels_only=TRUE)[,1] ) %>%
gather(Chromosome, threshold , -stratum)
step_df <- left_join(step_df_weight, step_df_threshold) %>% left_join(lfdrs)
## Joining, by = c("stratum", "Chromosome")
## Joining, by = c("stratum", "Chromosome")
step_df <- step_df %>% mutate(break_left = breaks_left[stratum],
break_right = breaks[stratum],
break_ratio = break_right/break_left,
break_left_init = break_left,
break_right_init = break_right,
break_left =break_left * break_ratio^.2,
break_right = break_right *break_ratio^(-.2))
stratum_fun <- function(df, colname="weight"){
stratum <- df$stratum
weight <- df[[colname]]
stratum_left <- stratum[stratum != length(stratum)]
weight_left <- weight[stratum_left]
break_left <- df$break_right[stratum_left]
stratum_right <- stratum[stratum != 1]
weight_right <- weight[stratum_right]
break_right <- df$break_left[stratum_right]
data.frame(stratum_left= stratum_left, weight_left= weight_left,
stratum_right = stratum_right, weight_right = weight_right,
break_left = break_left, break_right = break_right)
}
connecting_df_weights <- step_df %>% group_by(Chromosome) %>%
do(stratum_fun(.)) %>%
mutate(dashed = factor(ifelse(abs(weight_left - weight_right) > 0.5 , TRUE, FALSE),
levels=c(FALSE,TRUE)))
weights_panel <- ggplot(step_df, aes(x=break_left, xend=break_right,y=weight, yend=weight, col=Chromosome)) +
geom_segment(size=0.8)+
geom_segment(data= connecting_df_weights, aes(x=break_left, xend=break_right,
y=weight_left, yend=weight_right,
linetype=dashed),
size=0.8)+
scale_x_log10(breaks=c(10^4, 10^5,10^6,10^7,10^8),
labels = trans_format("log10", math_format(10^.x))) +
xlab("Genomic distance (bp)")+
ylab("Weight")+
theme(legend.position=c(0.8,0.6)) +
theme(plot.margin = unit(c(2, 1.5, 1, 2.5), "lines"))+
theme(axis.title = element_text(face="bold" ))+
scale_color_manual(values=pretty_colors)+
guides(linetype=FALSE)
## Warning: `guides(<scale> = FALSE)` is deprecated. Please use `guides(<scale> =
## "none")` instead.
weights_panel
# Weights chromosome 1
weights_panel_1 <- ggplot(filter(step_df, Chromosome == "chr1"), aes(x=break_left, xend=break_right,y=weight, yend=weight, col=Chromosome)) +
geom_segment(size=0.8,lineend="round")+
geom_segment(data= filter(connecting_df_weights, Chromosome=="chr1"), aes(x=break_left, xend=break_right,
y=weight_left, yend=weight_right,
linetype=dashed),
size=0.8,lineend="round")+
scale_x_log10(breaks=c(10, 10^2,10^3,10^4),
labels = trans_format("log10", math_format(10^.x))) +
scale_y_continuous(breaks=c(0,1000,2000))+
xlab(expression(paste("Distance (kbp)")))+
ylab(expression(paste("Weight")))+
theme(legend.position="none") +
theme(plot.margin = unit(c(2, 1.5, 1, 2.5), "lines"))+
theme(axis.title = element_text(face="bold" ))+
scale_color_manual(values=pretty_colors)+
guides(linetype=FALSE)
## Warning: `guides(<scale> = FALSE)` is deprecated. Please use `guides(<scale> =
## "none")` instead.
weights_panel_1
ggsave(weights_panel_1, filename="chr1_weights.pdf", width=3.5,height=2.5)
weights_panel_2 <- ggplot(filter(step_df, Chromosome == "chr2"), aes(x=break_left, xend=break_right,y=weight, yend=weight, col=Chromosome)) +
geom_segment(size=0.8, lineend="round")+
geom_segment(data= filter(connecting_df_weights, Chromosome=="chr2"), aes(x=break_left, xend=break_right,
y=weight_left, yend=weight_right,
linetype=dashed),
size=0.8, lineend="round")+
scale_x_log10(breaks=c(10, 10^2,10^3,10^4),
labels = trans_format("log10", math_format(10^.x))) +
scale_y_continuous(breaks=c(0,1000,2000))+
xlab(expression(paste("Distance (kbp)")))+
ylab(expression(paste("Weight")))+
theme(legend.position="none") +
theme(plot.margin = unit(c(2, 1.5, 1, 2.5), "lines"))+
theme(axis.title = element_text(face="bold" ))+
scale_color_manual(values=pretty_colors)+
guides(linetype=FALSE)
## Warning: `guides(<scale> = FALSE)` is deprecated. Please use `guides(<scale> =
## "none")` instead.
weights_panel_2
ggsave(weights_panel_2, filename="chr2_weights.pdf", width=3.5,height=2.5)
connecting_df_thresholds_ihw <- step_df %>% group_by(Chromosome) %>%
do(stratum_fun(., colname="t_ihw")) %>%
mutate(dashed = FALSE)#factor(ifelse(abs(weight_left - weight_right) > 10^{-7} , TRUE, FALSE),
# levels=c(FALSE,TRUE)))
thresholds_ihw_panel <- ggplot(step_df, aes(x=break_left, xend=break_right,y=t_ihw*10^6, yend=t_ihw*10^6, col=Chromosome)) +
geom_segment(size=0.8, lineend="round")+
geom_segment(data= connecting_df_thresholds_ihw, aes(x=break_left, xend=break_right,
y=weight_left*10^6, yend=weight_right*10^6,
linetype=dashed),
size=0.8, lineend="round")+
scale_x_log10(breaks=c(10, 10^2,10^3,10^4),
labels = trans_format("log10", math_format(10^.x))) +
scale_y_continuous(limits=c(0,1.8), breaks=c(0,1))+
xlab(expression(paste("Distance (kbp)")))+
ylab(expression(paste("IHW s(x) (",10^-6,")")))+
theme(legend.position=c(0.6,0.7), legend.title = element_blank()) +
theme(plot.margin = unit(c(2, 1.5, 1, 2.5), "lines"))+
theme(axis.title = element_text(face="bold" ))+
scale_color_manual(values=pretty_colors)+
guides(linetype=FALSE)
## Warning: `guides(<scale> = FALSE)` is deprecated. Please use `guides(<scale> =
## "none")` instead.
thresholds_ihw_panel
ggsave(thresholds_ihw_panel, filename="ihw_by_threshold.pdf", width=3.5,height=2.5)
connecting_df_thresholds_bh <- step_df %>% group_by(Chromosome) %>%
do(stratum_fun(., colname="t_bh")) %>%
mutate(dashed = FALSE)#factor(ifelse(abs(weight_left - weight_right) > 10^{-11} , TRUE, TRUE),
#levels=c(FALSE,TRUE)))
scientific_10 = function(x) {ifelse(x==0, "0", parse(text=gsub("[+]", "", gsub("e", " %*% 10^", scientific_format()(x)))))}
thresholds_bh_panel <- ggplot(step_df, aes(x=break_left, xend=break_right,y=10^10*t_bh, yend=10^10*t_bh, col=Chromosome)) +
geom_segment(size=0.8)+
geom_segment(data= connecting_df_thresholds_bh, aes(x=break_left, xend=break_right,
y=weight_left*10^10, yend=weight_right*10^10,
linetype=dashed),
size=0.8)+
scale_x_log10(breaks=c(10, 10^2,10^3,10^4),
labels = trans_format("log10", math_format(10^.x))) +
scale_y_continuous(limits=c(0,5), breaks=c(0,2,4))+
xlab(expression(paste("Distance (kbp)")))+
ylab(expression(paste("BY s(x) (",10^-10,")")))+
theme(legend.position=c(0.6,0.7), legend.title = element_blank()) +
theme(plot.margin = unit(c(2, 1.5, 1, 2.5), "lines"))+
theme(axis.title = element_text(face="bold" ))+
scale_color_manual(values=pretty_colors)+
guides(linetype=FALSE)
## Warning: `guides(<scale> = FALSE)` is deprecated. Please use `guides(<scale> =
## "none")` instead.
thresholds_bh_panel
ggsave(thresholds_bh_panel, filename="by_threshold.pdf", width=3.5,height=2.5)
connecting_df_lfdr_ihw <- step_df %>% group_by(Chromosome) %>%
do(stratum_fun(., colname="local_fdr_ihw")) %>%
mutate(dashed = FALSE)
lfdr_ihw_panel <- ggplot(step_df, aes(x=break_left, xend=break_right,y=10^1*local_fdr_ihw, yend=10^1*local_fdr_ihw, col=Chromosome)) +
geom_segment(size=0.8, lineend="round")+
geom_segment(data= connecting_df_lfdr_ihw, aes(x=break_left, xend=break_right,
y=10^1*weight_left, yend=10^1*weight_right,
linetype=dashed),
size=0.8,lineend="round")+
scale_x_log10(breaks=c(10, 10^2,10^3,10^4),
labels = trans_format("log10", math_format(10^.x))) +
xlab(expression(paste("Distance (kbp)")))+
ylab(expression(paste("IHW fdr(s(x) | x)")))+
theme(legend.position=c(0.6,0.7), legend.title = element_blank()) +
theme(plot.margin = unit(c(2, 1.5, 1, 2.5), "lines"))+
theme(axis.title = element_text(face="bold" ))+
scale_color_manual(values=pretty_colors)+
guides(linetype=FALSE)
## Warning: `guides(<scale> = FALSE)` is deprecated. Please use `guides(<scale> =
## "none")` instead.
lfdr_ihw_panel
ggsave(lfdr_ihw_panel, filename="ihw_by_fdr.pdf", width=3.5,height=2.5)
connecting_df_lfdr_bh <- step_df %>% group_by(Chromosome) %>%
do(stratum_fun(., colname="local_fdr_bh")) %>%
mutate(dashed = FALSE)#factor(ifelse(abs(weight_left - weight_right) > 0.5*10^(-6) , TRUE, FALSE),
# levels=c(FALSE,TRUE)))
lfdr_bh_panel <- ggplot(step_df, aes(x=break_left, xend=break_right,y=local_fdr_bh, yend=local_fdr_bh, col=Chromosome)) +
geom_segment(size=0.8, lineend="round")+
geom_segment(data= connecting_df_lfdr_bh, aes(x=break_left, xend=break_right,
y=weight_left, yend=weight_right,
linetype=dashed),
size=0.8, lineend="round")+
scale_x_log10(breaks=c(10, 10^2,10^3,10^4),
labels = trans_format("log10", math_format(10^.x))) +
scale_y_log10( labels = trans_format("log10", math_format(10^.x)))+
xlab(expression(paste("Distance (kbp)")))+
ylab(expression(paste("BY fdr(s(x) | x)")))+
theme(legend.position=c(0.6,0.4), legend.title = element_blank()) +
theme(plot.margin = unit(c(2, 1.5, 1, 2.5), "lines"))+
theme(axis.title = element_text(face="bold" ))+
scale_color_manual(values=pretty_colors)+
guides(linetype=FALSE)
## Warning: `guides(<scale> = FALSE)` is deprecated. Please use `guides(<scale> =
## "none")` instead.
lfdr_bh_panel
ggsave(lfdr_bh_panel, filename="by_fdr.pdf", width=3.5,height=2.5)