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  • Problem to use Bedtools after filtering uniquely mapped reads with samtools

    Hi there,

    I've aligned my ChIP-seq data with BWA and filtered for uniquely mapped reads with this command:

    samtools view file.bam | grep "XT:A:U" > file.unique.bam

    Then I tried to convert the file.unique.bam to .bed file with Bedtools but failed. The command I used is:

    bamToBed -i file.unique.bam > file.bed

    And I got error message like:

    BgzfStream ERROR: read block failed - invalid block header
    BamHeader ERROR: could not read magic number
    BamReader ERROR: Could not load header data for file.unique.bam

    Does anyone have this problem before? How can I solve it?

    Thanks!

  • #2
    There are two reasons why it doesn't work:

    1. "file.unique.bam" is not in the BAM format (look at "samtools view" for correct usage).
    2. You stripped the SAM headers with your grep command.

    You might need find a better way of filtering for uniquely mapped reads which preserves the SAM headers, or you add the SAM headers back to the header-stripped SAM file you created with your first command afterwards (look at "samtools view").

    Then, convert it to BAM with SAMtools and feed it into BEDTools.

    Comment


    • #3
      Originally posted by eilosei View Post
      Hi there,

      I've aligned my ChIP-seq data with BWA and filtered for uniquely mapped reads with this command:

      samtools view file.bam | grep "XT:A:U" > file.unique.bam

      Then I tried to convert the file.unique.bam to .bed file with Bedtools but failed. The command I used is:

      bamToBed -i file.unique.bam > file.bed

      And I got error message like:

      BgzfStream ERROR: read block failed - invalid block header
      BamHeader ERROR: could not read magic number
      BamReader ERROR: Could not load header data for file.unique.bam

      Does anyone have this problem before? How can I solve it?

      Thanks!
      grab header
      Code:
      samtools view -H .bam > new.sam
      stick on the unique reads
      Code:
      samtools view .bam | grep ... >> new.sam
      convert to bam
      Code:
      samtools view -Sb -o unique.bam new.sam
      also check out samtools reheader.

      Comment

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