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  • sfranzenburg
    Member
    • Mar 2014
    • 28

    MG-RAST ambigious base count

    Hi,
    I wanted to analyze my 150bp Paired-End Metagenome Reads (Illumina) with MG-RAST.

    After uploading, I get the file statistics.

    My forward sequences (R1) have <5% ambiguous characters, but my reverse sequences (R2) have ~75% ambiguous characters (according to MG-RAST). Needless to say, that I can not apply MG-RASTs default quality filtering to these reads, they all would get removed.

    However, when I check my reads with FastQC, the R2 file seems fine:

    So why does MG-RAST tell me, that these reads are of low quality, and why is that no problem with the R1 file?

    A few lines from the R1 file:
    @HWI-ST1348:258:H8UMCADXX:1:1101:1062:2034 1:Y:0:ATCANG
    NATGNTCCTTGATAAGAGNAAAGATAAGTGGCAGATTGTCCGGAAAGCGTATAAATAATATAGTAATGCTAAAAGGTNNCNNCGATGCCGGTATTTATAGTACTATGCAAATTCTCAGCCAGGTTACCATTAATGAAANCATGATAGAAAT
    +
    #0;@#2@@@@@@?@@@?@#3@>@??@??>@??>??????????????????????????>??@?????==?????############################################################################
    @HWI-ST1348:258:H8UMCADXX:1:1101:1237:2154 1:N:0:ATCACG
    CAATACGCAGCAACAATCACATACAGAGCGTACATACAGTATGCTCCGACATGTTAGAACTTGATTATTTTGTGCCATAGTTGCGTACCTAGCGAAGCGAGTTTCGGTGCTTATGCTTTCACGTTTCTATAAAAACTGCGTGACAACGCCA
    +
    CCCFFFFFHAHHHJJJJJIJJIJJIJJGGIGHHIIGIIIIIIJJDHIJGIIIJJJIJJJHHHHEHHFFFFFFAACEEECCDDCCB@?@?CCC@<B><>@BBBBC>B>?@9CCCC@>ADACAC<BD?CCDADDED:5>4499928A485>B9
    @HWI-ST1348:258:H8UMCADXX:1:1101:1370:2035 1:Y:0:ATCACG
    NTGGNACAGTTTAATGACGCGTTTATATGTCGGCGCGGGCAGTTCGTGCTGTGTATGAGTGTGAGGCATTTCCCACGAATCTGGCCGACGCGGGCAGTTCGTTGTATGAGTGTGAGGCATTTCGCAGGAATGTTATTTCATCATTATTTGC
    +
    #0;@#2=@@@@@@?@?@????@@????????????8??#################################################################################################################
    @HWI-ST1348:258:H8UMCADXX:1:1101:1382:2089 1:N:0:ATCACG
    ATTCTAGAGAAACAAATCCTTAATTTTTCTCGCCAGATTTCGCGCTCCTAAAGATCATAGAAGGAGCAAAAAAAATTATCTATATTCTTCAATGACTTATTGGGGGGGGGGGCGACCCCAGCTATAGATCGGAAGACCACACGTCTGAACC


    A few lines from the R2 file:
    @HWI-ST1348:258:H8UMCADXX:1:1101:1237:2154 2:N:0:ATCACG
    CTTTAAGAAGTACCGTTTTAGCGAGACGACAGCGCTACAACGCTGTCGTCGTGTGTGGTTCGGAGCTATGCGGGGAAGTAAGTCTGGCGTTGTCACGCAGTTTTTATAGAAACGTGAAAGCATAAGCACCGAAACTCGCTTCGCTAGGTAC
    +
    CCCFFFFFHHFHHJJJJJJJJJJJJJJJJJJJGIIJJJJIIGGIEHEHFDF<>;?=ABCBDDD?BDDDCDCBDDD99@:CCDCDDDCC@DBD@DECBDBDBCDDDDDDDDDDDD<ADDDDCCCDDDDACDDDDBBCCBBDBDD@BBBB>>:
    @HWI-ST1348:258:H8UMCADXX:1:1101:1370:2035 2:Y:0:ATCACG
    GGCGACAGCGTTGTGGCGCTGTCGCCGCGCTAAAACGGTACCTTCCAAAACTACCAAATGCCATCAGCCAATCGCAACTCAATTAAAGGCTGATGCAATTGCCAAATAATGATGAAATAACATTCCTGCGAAATGCCTCACACTCATACAA
    +
    @CCFFFFFHHHHHIJJJJJIIGIIJJGGGIJJHHHHFFBEDDEDEDDDDDDDCDDDDBD:CDCCDDACDDDDD@BD@DDCDDDEDDDDCDCBBCCCDCCDDCCCDDDDDEDDDDDDD>CC@ACCDDDCDDB@>AACC:>@<:@9>?AA:@3
    @HWI-ST1348:258:H8UMCADXX:1:1101:1382:2089 2:N:0:ATCACG
    ATAGCTGGTGTCGCCCCCCCCCCCAATAAGTCATTGGAGAATATAGATAATTTTTTTTGCCCCTTCTAGGATCTTTAGGAGCGCGAAATCTGGGGAGAAAATTTAAGGATTTGTTTCTCTAGATTAGATCGGAAGAGCGTCGTGTAGGGAA
    +
    @@<D;DDDHHH?F=C@HGHGIIF>>B6;>C#########################################################################################################################
    @HWI-ST1348:258:H8UMCADXX:1:1101:1478:2092 2:Y:0:ATCACG
    GCATTAGACCTTTGCAAACCAGTTTTCCCCCCCATTGCGCGACATTACTCATACGCCAAGTGGAACATTAGCACTTCTCTCCGATGAATAGCTCAGTTCTTCGCCAAATTATGTGAATTTGAAACGTGTGAGCGGGCAAAGAGGTTCATTC


    best regards,
    Soeren
    Last edited by sfranzenburg; 03-25-2014, 06:12 AM.
  • GenoMax
    Senior Member
    • Feb 2008
    • 7142

    #2
    Your sequence files should have no ambiguous characters (just A/C/G/T). It sounds like your file may be corrupted in some way or there is the usual problem with PC/Mac/Unix file format differences to consider (if these files were moved among any of those systems).

    Comment

    • sfranzenburg
      Member
      • Mar 2014
      • 28

      #3
      Just got a reply from the MG-RAST support (didn't expect them to react that fast, thats why I got here for help too). Seems like I have misinterpreted their numbers.
      When I saw average ambig chars: 0.75 and saw that 75% of my reads fail fastq-trimming, I assumed that 75% of my bases must be interpreted as ambiguous. Thats not the case, but however, 75% of my reads (which according to FASTQC have good quality, fail default QC (min score 15, max 5 bases). But I think MG-RAST support will help me from now on.

      Comment

      • Brian Bushnell
        Super Moderator
        • Jan 2014
        • 2709

        #4
        With 150bp reads (I assume this is Hi-seq 2000?) I don't recommend failing reads just because some of the last few bases are below Q15, because you'll throw away tons of good data. Depending on what you want to do with the reads (e.g., map them), you don't necessarily even need to quality-trim them.

        Comment

        • sfranzenburg
          Member
          • Mar 2014
          • 28

          #5
          Thanks.
          I meanwhile found my lost reads. Most of them were removed in MG-RASTs dereplication step (50% removed). Is dereplication state of the art for Illumina data today? 50% loss sound very high for me.

          Comment

          • Brian Bushnell
            Super Moderator
            • Jan 2014
            • 2709

            #6
            It depends on what you're doing and how the data was generated. If you don't do any amplification, then duplicate removal may not be necessary, which is ideal. The shorter your insert size, the smaller the genome, the more PCR cycles are performed, the less random your shearing protocol is, and the more reads you have, the more duplicates will be detected.

            50% is very high for what I consider a "normal" library, but that could be very different from your "normal". Looks like you're studying drosophila... can you say anything about the library prep and the purpose of the study?

            Comment

            • sfranzenburg
              Member
              • Mar 2014
              • 28

              #7
              Hi Brian,
              thanks alot.
              I did MDA for 8h to amplify my original DNA (library prep protocol wanted to have 1 µg, which was far more than I had). Library Prep was basically the same as with the Illumina Kit. Insert size is 200bp, shearing was performed by sonification (Covaris) and 11 PCR cycles were used in the final PCR.

              Comment

              • Brian Bushnell
                Super Moderator
                • Jan 2014
                • 2709

                #8
                Since you started with less DNA than required, and performed a lot of amplification, 50% duplicates is not unexpected. My only experience with MDA is in single-cell sequencing, but our amplified single cells often have 95%+ duplicate rates and highly erratic coverage ranging from 1x to 100000x for the same library.

                Comment

                • sfranzenburg
                  Member
                  • Mar 2014
                  • 28

                  #9
                  Ok, thanks alot Brian.
                  Than I will the discard the reads.
                  I read some papers for MDA before I did it and I don't recall that they brought up this problem.

                  Comment

                  • Brian Bushnell
                    Super Moderator
                    • Jan 2014
                    • 2709

                    #10
                    It might not be due to MDA, just large amounts of amplification in general will create duplicates.

                    Comment

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