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  • m_elena_bioinfo
    Member
    • Oct 2009
    • 99

    alignment reads in homologous region

    Hi NGS users,
    I'm analyzing SureSelect sequencing
    I noticed that BWA/SAMTOOLS in mapping step, align reads in target genes and also in regions that are homologous to my target gene but the are not in baits.
    does anyone knows how correct this bias? This unappropriate alignment could affect the SNP calling.
    Thanx a lot,
    bye!
  • stefanoberri
    Member
    • Jan 2010
    • 35

    #2
    Hi. I have never done capture, but we will very soon, so I though about these problems. I hope my contribution is useful.

    You could use, as "reference genome", a file that only contains your targets.

    however, the pull down is probably not 100% on target, so this might introduce artifacts

    The baits, on the other hand, might actually pull down a region very similar to their desired target, so it might be that your sequence comes from a homologous region, and the aligner get it right.

    Comment

    • m_elena_bioinfo
      Member
      • Oct 2009
      • 99

      #3
      Thanx a lot Stefano.
      I have already tried to align my reads against my target sequence (using sure select design as reference genome) but for experience, I can say that it forces too much the alignment with high risk of false positive.

      I don't know if my problem is at an experimental level (in the enrichment protocol) or in the mapping, because it's not a problem of repetitive regions but a problem in enrichment for homology.

      Comment

      • stefanoberri
        Member
        • Jan 2010
        • 35

        #4
        just to know, what sort of similarity is there between a homologous region and your target?

        Comment

        • adamdeluca
          Member
          • Jul 2010
          • 95

          #5
          Limiting your reference is a bad idea as similar regions differing by a single base will look like a SNP if both regions are not included in the reference.

          A common approach to dealing with this is to scale the quality of your alignment based on the uniqueness of the mapping (following the GATK best practices will do this).

          While some the the off-target effect you are seeing is likely due to incorrect mapping, because you are enriching for these regions by hybridization, there is likely off-target capture as well.

          Comment

          • m_elena_bioinfo
            Member
            • Oct 2009
            • 99

            #6
            about 94% of homology

            Comment

            • m_elena_bioinfo
              Member
              • Oct 2009
              • 99

              #7
              Adamdeluca, you are right!
              in my alignment pipeline, I used always GATk realign and recalibration score. But I can observe reads mapped in homologuos region in the final bam.
              So...the question is: it is an experimental problem of enrichment for homology (and in this case I cannot do anything) or there is a way (parameter-script...) to understand when I map reads off target in homologuos genes?

              And, if the problem is an incorrect mapping (I use BWA and Samtools for this step), how can I limit the mapping to other region? In some case, mapping quality of the reads is very low, so I can discriminate off target region, in other cases I have a high mapping quality and a high coverage, so I can't differentiate target and off target (with the risk of false positive in SNP calling)

              Comment

              • adamdeluca
                Member
                • Jul 2010
                • 95

                #8
                Originally posted by m_elena_bioinfo View Post
                Adamdeluca, you are right!
                in my alignment pipeline, I used always GATk realign and recalibration score. But I can observe reads mapped in homologuos region in the final bam.
                So...the question is: it is an experimental problem of enrichment for homology (and in this case I cannot do anything) or there is a way (parameter-script...) to understand when I map reads off target in homologuos genes?

                And, if the problem is an incorrect mapping (I use BWA and Samtools for this step), how can I limit the mapping to other region? In some case, mapping quality of the reads is very low, so I can discriminate off target region, in other cases I have a high mapping quality and a high coverage, so I can't differentiate target and off target (with the risk of false positive in SNP calling)
                great questions. Let me know if you figure them out.

                By manually inspecting reads in these types of regions I can observe obvious miss-mapping, and obvious off-target capture.

                Comment

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