Hi Folks

I wanted to make a plot in R and Im struggling with it!

I was hoping to use a BED file to plot blocks of equal height but varying length (peak positions) along the x axis (genomic position) the reason I want equal height is so I could plot using color intensity based on the fold enrichment values from the MACs peak caller. Exactly like the UCSC genome browser "dense" view. Can somebody give me an example of this??

Many thanks in advance

Basically like this track on hg19

http://genome-euro.ucsc.edu/cgi-bin/hgTracks?db=hg19&position=chr21%3A33031597-33041570&hgsid=202635987_ULlPiiRDsWNKFm0lTj8C7b9KG0IS

This is a pretty low level way of achieving it, if I correctly understand:

## Dummy data in ~bed format
n<- 10
chrom<- rep('chr1', n)
start<- seq(1, 1000, length.out= n)
end<- start + rpois(n, 50)
logfc<- rgamma(n, 2)

## Prepare colours based on logFC
pal<- colorRampPalette(c('blue', 'red'))
cols<- paste0(pal(n)[as.numeric(cut(logfc, breaks = n))], 99)

## Plot
plot(x= start, y= rep(0, n), type= 'n', bty= 'n', yaxt= 'n',
    ylab= '', xlab= 'Position', xlim= range(c(start, end)), ylim= c(0, 1))
rect(xleft= start, xright= end, ybottom= 0, ytop= 0.1, border= NA, col= cols)
text(x= start, y= 0.12, labels= sprintf("%.2f", logfc), adj= c(0,0))

## Legend
nlg<- 5
lgcols<- paste0(pal(nlg)[1:nlg], 99)
lg<- round(seq(min(logfc), max(logfc), length.out= nlg), 1)
legend('topleft', pch= 15, bty= 'n', col= lgcols, legend= lg, pt.cex= 2, cex= 1)

Maybe just export the UCSC browser shot directly from an existing session, or use a fetch tool, if automation is needed.