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  • fastq.gz size for human WGS coverage calculation

    I have got 3 pair fastq.gz file of human WGS, the size are 3.9 + 4.2, 1.7 + 1.8, 1.5 + 1.6 respectively, how to calculate coverage of these results.
    sequence plantform: illumina x ten
    seq model: pair-end 150
    thx
    Last edited by yipukangda; 11-07-2016, 09:22 PM.

  • #2
    If you want average coverage, assuming the data is all human:

    Code:
    avg_coverage=(#reads)*150/3000000000
    To count the reads, you can use Reformat from the BBMap package:

    Code:
    cat *.fastq.gz | reformat.sh in=stdin.fq
    You can get more accurate numbers by mapping the reads after adapter-trimming, since some of the data is probably not human.

    Comment


    • #3
      Originally posted by Brian Bushnell View Post
      If you want average coverage, assuming the data is all human:

      Code:
      avg_coverage=(#reads)*150/3000000000
      To count the reads, you can use Reformat from the BBMap package:

      Code:
      cat *.fastq.gz | reformat.sh in=stdin.fq
      You can get more accurate numbers by mapping the reads after adapter-trimming, since some of the data is probably not human.
      thanks, I estimated like this: file_size x 1/2 x compression fold / genome size

      Comment

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