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  • read counts from samtools idxstats

    Hi,

    I want to get the read counts for gene expression analysis. I used "samtools idxstats <bam file>" and got the four columns of "contig ID, read length, #mapped reads and # unmapped reads".

    My question is I should use #mapped reads(the third column) or (#mapped reads + # unmapped reads)/2 as the raw reads count?

    Thank you in advance!
    Victoria

  • #2
    Raw read count = mapped reads + unmapped reads

    Comment


    • #3
      Thank you for the response. Alternatively, this adding value divided by two also makes sense, in this case the read counts are the fragments.
      I am not sure which result is from the htseq-count, which is generally used as the input for differential gene expression.

      THanks!
      Victoria

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      • #4
        htseq-count doesn't count multimappers, so the "total reads" that it would report for something and that reported by samtools idxstats may not be very closely related.

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