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  • samstat versus tophat overall alignment rate %

    Hi group

    I am trying to map RNAseq single straneded paired end reads using tophat, the alignment rate I get using samtools falgstat is very good (~90%) however checking the logs files of tophat, specifically, bowties.left.keep.reads shows a very low overall alignment rate (~36%). Can someone please help me understand these parameters ?

    Thanks a lot
    Alyaa

    This is the tophat command I use:
    Code:
    $ tophat -g 1 -p 8 -G test.gtf -o test_thout --library-type fr-firststrand test R1_001.fastq R2_001.fastq
    This is the samtools flagstast command:
    Code:
     $ samtools flagstat accepted_hits.bam 
    36919320 + 0 in total (QC-passed reads + QC-failed reads)
    0 + 0 duplicates
    36919320 + 0 mapped (100.00%:-nan%)
    36919320 + 0 paired in sequencing
    18510302 + 0 read1
    18409018 + 0 read2
    33270470 + 0 properly paired (90.12%:-nan%)
    35338762 + 0 with itself and mate mapped
    1580558 + 0 singletons (4.28%:-nan%)
    406722 + 0 with mate mapped to a different chr
    87168 + 0 with mate mapped to a different chr (mapQ>=5)
    The logs files; bowtie.left_kept_reads.log
    Code:
    19786770 reads; of these:
      19786770 (100.00%) were unpaired; of these:
        12585633 (63.61%) aligned 0 times
        6908036 (34.91%) aligned exactly 1 time
        293101 (1.48%) aligned >1 times
    36.39% overall alignment rate

  • #2
    The accepted.bam file only contains mapped reads, not all of them, so the metrics will never be the same.

    Comment

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