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I have one table with coordinates (start, end) of ca. 500000 fragments and another table with 60000 single coordinates that I would like to match with the former fragments. I.e., for each record from dtCoords table I need to search a record in dtFrags table having the same chr and start<=coord<=end (and retrieve the type from this record of dtFrags). Is it good idea at all to use R for this, or I should rather look to other languages?

Here is my example:


dtFrags <- fread(

dtCoords <- fread(

At the end, I would like to have something like this:

 10,  1,  150,  1, exon
 20,  2,  300,  2, intron
 20,  2,  300,  4, exon
 30,  Y,  500, NA, NA

I can simplify a bit the task by splitting the table to subtables by chr, so I would concentrate only on coordinates

setkey(dtCoords, 'chr')
setkey(dtFrags,  'chr')

for (chr in unique(dtCoords$chr)) {
  dtCoordsSub <- dtCoords[chr];
  dtFragsSub  <-  dtFrags[chr];
  dtCoordsSub[, {
    # ????  
  }, by=id]  

but it's still not clear for me how should I work inside... I would be very grateful for any hints.

UPD. just in case, I put my real table in the archive here. After unpacking to your working directory, tables can be loaded with the following code:

dtCoords <- fread("dtCoords.txt", sep="\t", header=TRUE)
dtFrags  <- fread("dtFrags.txt",  sep="\t", header=TRUE)
share|improve this question
I do not have a way to run R right now, but this problems seems interesting to me. and I think first divide data by chromosome and then I hope you do not have duplicate coord in the range, then make coord column based on start and position.then merge later with that coord. I will get back to the problem tomorrow, if it is not solved by that time –  Ananta Nov 3 '13 at 2:41

2 Answers 2

up vote 6 down vote accepted

In general, it's very appropriate to use the bioconductor package IRanges to deal with problems related to intervals. It does so efficiently by implementing interval tree. GenomicRanges is another package that builds on top of IRanges, specifically for handling, well, "Genomic Ranges".

gr1 = with(dtFrags, GRanges(Rle(factor(chr, 
          levels=c("1", "2", "X", "Y"))), IRanges(start, end)))
gr2 = with(dtCoords, GRanges(Rle(factor(chr, 
          levels=c("1", "2", "X", "Y"))), IRanges(coord, coord)))
olaps = findOverlaps(gr2, gr1)
dtCoords[, grp := seq_len(nrow(dtCoords))]
dtFrags[subjectHits(olaps), grp := queryHits(olaps)]
setkey(dtCoords, grp)
setkey(dtFrags, grp)
dtFrags[, list(grp, id, type)][dtCoords]

   grp id   type id.1 chr coord
1:   1  1   exon   10   1   150
2:   2  2 intron   20   2   300
3:   2  4   exon   20   2   300
4:   3 NA     NA   30   Y   500
share|improve this answer
well, for the moment I get an error with the last command (dtFrags[, list(grp, id, type)][dtCoords]): Error in '[.data.table'(dtFrags[, list(grp, id, type)], dtCoords) : When i is a data.table (or character vector), x must be keyed (i.e. sorted, and, marked as sorted) so data.table knows which columns to join to and take advantage of x being sorted. Call setkey(x,...) first, see ?setkey. - but overall it seems to be a solution, I will try to sort it out, thanks! –  Vasily A Nov 3 '13 at 12:40
sure, I did setkey, as in your code (and when I check by key(dtCoords) and key(dtCoords), both return "grp") - still the same error. –  Vasily A Nov 3 '13 at 13:03
it shows 1.8.10 (R version 3.0.2) –  Vasily A Nov 3 '13 at 13:21
oups, it seems I made not very good sample dataset... For my real data, typical situation is that one fragment contains multiple coordinates - just add one more record to the dtCoords table: say, 50,2,250 - so that it will match the fragment #4 of dtFrags - in this case your code seems to give not the output I would expect... –  Vasily A Nov 3 '13 at 16:53

Does this work? You can use merge first and then subset

> kk
   chr id.x start end   type id.y coord
1:   1    1   100 200   exon   10   150
2:   2    2   300 500 intron   20   300
3:   2    4   250 600   exon   20   300
4:   X    3   400 600 intron   NA    NA

 kk[coord>=start & coord<=end]
   chr id.x start end type id.y coord
1:   1    1   100 200 exon   10   150
2:   2    4   250 600 exon   20   300
share|improve this answer
It's hard to recognize the OP's desired output here... –  Frank Nov 3 '13 at 0:58
@Frank, the output is almost OK (it should be just >= and <= instead of > and <), but I can't use it for my big tables –  Vasily A Nov 3 '13 at 1:04
Unfortunately my tables seem to be too big, I get this: Error in vecseq(f__, len__, if (allow.cartesian) NULL else as.integer(max(nrow(x), : Join results in 1447477452 rows; more than 519176 = max(nrow(x),nrow(i)). Check for duplicate key values in i, each of which join to the same group in x over and over again. If that's ok, try including 'j' and dropping 'by' (by-without-by) so that j runs for each group to avoid the large allocation. –  Vasily A Nov 3 '13 at 1:05
@VasilyA Is that a problem of size? I suspect that that error can be made to show up in a small reproducible example. I know I've run into it with a four-row data.table before –  Frank Nov 3 '13 at 1:07
thanks @Frank, I will try to dig out about the roll option. As for reproducing the error - I don't see how to do this with small example, but I added the link to my real data ('UPD' at the end of the post). –  Vasily A Nov 3 '13 at 1:41

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