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  • #1

    Bam quality vs read quality

    I have a cancer bam file and want to check its read qualities. I have two options in mind.
    1. Check bam quality through fastqc
    2. Convert the bam file into paired-end reads (in fastq) and check their quality in fastqc.
    Are both the processes equivalent?
    Tags: bam conversion, next gen sequencing
  • #2
    Yes, because FastQC is a QC program. FastQC does not modify raw data. It is going to show you summary of the same Q-scores whether they come from the BAM or the fastq reads extracted from the BAM file.

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    • #3
      Sorry for the late followup to your reply. If that is the case, then why am I getting poorer quality when I convert the bam to 2 fastq files(read 1 and 2) whereas good quality when just checking the bam file as a whole?

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      • #4
        Probably, there is the problem with sorting. (check https://twitter.com/davisjmcc/status/931298649841188864 )

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