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  • dawe
    Senior Member
    • Apr 2009
    • 258

    SNPs and file formats

    Hi, I'm looking at some sequence data in order to find mutations. Since I (probably) have to filter the variants with known SNP and indels I would like to have some hint on which file format/tools you are using.
    Once I have a list of candidate mutations, I planned to use BEDTools to perform most of the operations. The only problem is that I have different file formats I can operate and this puzzles me:
    1- I call variants as result of samtools/samtools.pl. The format is samtools pileup
    2- I have snp131 data in BED format (from UCSC genome browser)
    3- I guess I can get SNPs from 1000g in VCF format (although I still have to study which is the file(s) I need).

    BEDtools should support either BED and VCF format. What about samtools pileup? I guess I may try to convert it in one of both formats...

    Puzzle #1 (samtools to BED):
    - single nucleotide variations can be converted as CHR:POS-POS+1 (I guess)
    - How do I convert small insertions? CHR:POS-POS ?
    - How do I convert small deletions?

    Puzzle #2 (samtools to VCF):
    - Simply, is there a way to directly convert samtools pileup to VCF?

    Any suggestion is appreciated :-)
    Thanks

    d
  • epigen
    Senior Member
    • May 2010
    • 101

    #2
    I had a similar problem with SNPs, but did not consider indels from samtools pileup. For the dbSNP BED file, I converted insertions into POS-1-POS, because BEDTools doesn't find an overlap for features with start=end. I did the same for samtools pileup SNPs to make them zero-based BED as well. The VCF format I don't know.

    Comment

    • dawe
      Senior Member
      • Apr 2009
      • 258

      #3
      Originally posted by epigen View Post
      I had a similar problem with SNPs, but did not consider indels from samtools pileup. For the dbSNP BED file, I converted insertions into POS-1-POS, because BEDTools doesn't find an overlap for features with start=end. I did the same for samtools pileup SNPs to make them zero-based BED as well. The VCF format I don't know.
      In the end I've found that samtools 0.1.8 comes with a handy sam2vcf.pl script (which converts to VCF v3.3, I've used vcf-convert from vcf tools to further convert to v4.0). VCF files can be intersected with BED files using BEDTools and, apparently, it works. I mean, at least I've been able to filter my VCF from entries in dbSNP (as BED) :-)
      BTW, I had to convert VCF to a 0-based bed-like to use some Useq programs (such as Alleler)... I'm afraid we're far from having some standards here :-(

      d

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