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  • Calculate number of multi-mapped reads?

    Hi, does anyone know how to calculate the number of multi-mapped reads from your bam file?

    This seems like an obvious/silly question but the latest versions of Cufflinks no longer provides this statistic in the basic output and I have been looking everywhere (log files, samtools stats, this website, etc) but can't figure out how to find this out!

    Thanks!

  • #2
    Although primarily to tally up read counts for genes, HT-seq count also adds up the multimap reads "alignment not unique."

    Comment


    • #3
      Thanks! I'll look into it.

      Comment


      • #4
        Something like this might work.

        Code:
        samtools view -F 4 file.bam | awk '{printf $1"\n"}' | sort | uniq -d | wc -l
        
        Explanation
        -----------
        samtools view -F 4 file.bam
            print all lines in SAM format except those flagged as unmapped
        
        awk '{printf $1"\n"}'
            print the first field in the line (the read name)
        
        sort | uniq -d | wc -l
            sort the read names
            print only the duplicates (i.e. those appearing more than once)
            count the lines

        Comment


        • #5
          Thanks, great idea and thanks for the detailed, explanation! I'll give it a try

          Comment


          • #6
            Retrieve mapped reads to certain regions (eg. between 120-140 in a gene)?

            I have my own unannotated reference data base. With it, the reads were mapped with Bowtie, now I need to retrieve all reads which mapped to certain region between 120-140 nt/each gene, how can I do it with samtools ? Thanks in advance.

            Comment


            • #7
              Make a BED file with the gene locations, flank that with bedtools (or awk), and then use it with the "-L" option to "samtools view".

              Comment


              • #8
                more specifics

                Would you please give me more details ? Thanks.

                Comment


                • #9
                  Which part in particular requires more detail?

                  Comment


                  • #10
                    example

                    >Sg01_138835_A_G
                    TGCGAAGTATGCCACCAACATGTTTCACCGCATAACCTTGATCACCTTGGACATTCTGCCACAAGCAGACGACGAGTTCCTCAGAAAATTCATGGACAAATTTGGGCGCACGACCATCTA [GATCGAAAATCTTAATCCCG]AGCTAGTGTTGCATTCCATGCTCCTCGTCTTACACTCCAACAAGTTTGCAGAAAGTTTGTCAAAAATCCACTCGGTAGCATGGACGAGCTGCACGAGTGAGCCAAGGGTTACATATAGATGGAAGAAATGTCCAAATTCTGGAAAGAAGTCCGTCAAGCCGAACACAAGCACGAAAAGTGCAAAGCAAACTCCAAGGCCGACTTGCACAAGTCAAACAAGAGGCCCAATTCAGACAAGCGCTAACCTCTCCCCAAAGAGC

                    I want to retrieve reads aligned to [GATCGAAAATCTTAATCCCG] within gene above.

                    Comment


                    • #11
                      If you aligned to the gene itself, then "samtools view alignments.bam Sg01_138835_A_G:120-140". If you aligned to the genome then find out where in the genome that is.

                      Comment


                      • #12
                        how about multiple genes in reference

                        >Sg01_138835_A_G
                        TGCGAAGTATGCCACCAACATGTTTCACCGCATAACCTTGATCACCTTGGACATTCTGCCACAAGCAGACGACGAGTTCCTCAGAAAATTCATGGACAAATTTGGGCGCACGACCATCTAGATCGAAAATCTTAATCCCGAGCTAGTGTTGCATTCCATGCTCCTCGTCTTACACTCCAACAAGTTTGCAGAAAGTTTGTCAAAAATCCACTCGGTAGCATGGACGAGCTGCACGAGTGAGCCAAGGGTTACATATAGATGGAAGAAATGTCCAAATTCTGGAAAGAAGTCCGTCAAGCCGAACACAAGCACGAAAAGTGCAAAGCAAACTCCAAGGCCGACTTGCACAAGTCAAACAAGAGGCCCAATTCAGACAAGCGCTAACCTCTCCCCAAAGAGC
                        >Sg01_281790_T_C
                        CATCTATCTATTGCTTCAACCATGAAAATAATTATTTTCAAAGGCTTGAGTAATAATGTTTACCAATATAATGCCTATAATAATGTTACAAAATTCTAGTTTATATACCAAGTTTGATCGATGTTTGTAAAATTTAGCATATTCTTGCCTTGAATATCCTTTTGACACACACAAATACCATATAACTAACCCACAATATTCTGACTTATATGGGTGCAGCGGATCATTTGAGCGAAGCTGTGGGCGACAACGAATCCAAGGAACTTTTTGAATCATTTCGAGTCTTCTGCAATAGAAAAAGTGTTAGTACTAATGCATTTTCATCATTCAACAATTAATATAAATATATATATATATAGAGAGAGAGAGAGAGAGAGAAGTGCACTCATGAACAAAATCC
                        >Sg01_334575_A_G
                        ATTTTCTTAGTCCGCAAAAGTTAAACAGTATGTTAAGAATATAGGTTAAGAAACTTAAAAGTAAAAATATTTTTATTAAGAGGTGAAAAATTTTGTACAATAACTTGACTTGGAAAATTCTGCAGTTCCTGTTCTTCCAAATGTAATCTATGGACTATGGCAACAACAAAACTCAGAGACGCTACGTCCATTACACTTCACTTGGACAGTAAGTTAGACATCAACCAGGGGCCAAATTCTTGATGAAAAAAGCCTGCACGAACAGCATCTGGGATTAAAACATTCCAGACCTCCTTAGCCGCATAACATTTGGATGGATCATATAATTATATGGATAGATAACTATATGGATCATAATTAATTCAGCATAATTTTTTTTAATACTCTCTAAGCGCCTCTC
                        >Sg01_402061_A_C
                        CATAACCTGATAATATATTTTATATATCTACTATGAAAATAAATAGAATATCATATATACTAAGTAAGAAACGATCTGGTGTGTATCAAACAATGAATAATAAAATGTTGTTATCCAATTCTTATATAATATCTTATTTTAAGCAACAATCAAACAATGAATATTTTAAGAACTTATTTATCATGTTCTTATGGAGGCCTCTAGGGTAAGTCGTGACTGTATAGCATAGAAAATAAAGCTGCAGGAGCGTGGTATATCTTGTCAGAGCATGTATGTGTCTTGAGTGTGAAAGAGGGTTGGAGAAAGCAAAGGAATGTTGGAGGTCATTATTGGCTTCAAGCAGAGAGTGCTTACGAACCTATTAAAGTTGGAGCAGTGAGATATATAGTATAGTTGAGCT

                        If I want retrieve reads mapped to same region on multiple (several thousands) genes, do I need to list all, like this, Sg01_138835_A_G:120-140, Sg01_281790_T_C:120-140 ... ?

                        Comment


                        • #13
                          Make a BED file of the regions and use that with the "-L" option.

                          Comment


                          • #14
                            thanks.

                            I will do that.

                            Comment

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