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  • analyst
    Member
    • Jan 2011
    • 18

    FastQC per base sequence content

    Does it seems acceptable (Global GC cotent for the species = 40%)

    <original link removed>



    Last edited by analyst; 11-28-2011, 01:48 PM.
  • simonandrews
    Simon Andrews
    • May 2009
    • 870

    #2
    Can you attach it to the forum? That site is blocked from here. Also it would be useful to see the per sequence GC plot as well as the per base plot.

    Comment

    • Bukowski
      Senior Member
      • Jan 2010
      • 388

      #3
      Originally posted by analyst View Post
      Does it seems acceptable (Global GC cotent for the species = 40%)

      <link removed>
      Please do not use that host for images - it has NSFW content displayed prominently, and I have no desire to get sacked for viewing SeqAnswers links in an open plan office.

      Comment

      • analyst
        Member
        • Jan 2011
        • 18

        #4
        I understand and apologize. and thanks to the person moderating who posted image correctly

        Can anyone please comment on the fastQC finding

        Comment

        • simonandrews
          Simon Andrews
          • May 2009
          • 870

          #5
          I can't see an image reposted. The moderator only removed the original link. We still can't see your data.

          Comment

          • Orr Shomroni
            Member
            • Oct 2011
            • 26

            #6
            analyst, you may want to look at the following website:



            Introduction gives some general information on the FastQC algorithm. For specific information on the modules (what the developers consider as "pass", "warn" and "fail"), see under "Analysis modules" there will be some text files about each module and what their thresholds are.

            This is a quote from the section on GC content:

            Warning

            This module issues a warning it the GC content of any base strays more than 5% from the mean GC content.

            Failure

            This module will fail if the GC content of any base strays more than 10% from the mean GC content.
            Does this answer your question?
            "Though it may seem that all's been said and done, originality still lives on" - some unoriginal guy who had nothing better to write as his signature

            Comment

            • pmiguel
              Senior Member
              • Aug 2008
              • 2328

              #7
              Looks acceptable to me.

              What concerns you? If it is the low-level but periodic fluctuations in base levels across the read, that has been commented on before in another thread. There the period is three bases per cycle and more regular than what you see here.

              --
              Phillip

              Comment

              • analyst
                Member
                • Jan 2011
                • 18

                #8
                Thanks for the comments orr and phillip. Consider me beginner, just wanted to make sure the peaks at certain positions is nothing to worry about. It is more pronounced in the second picture I just posted, at 43. FastQC is warning me but I am not reading too much into it.

                Simon, can you see the new picture I just posted, if not, I am also attaching here.
                Attached Files

                Comment

                • pmiguel
                  Senior Member
                  • Aug 2008
                  • 2328

                  #9
                  Okay, the new plot (the second one) is a different story. The G peak at 42 bases may indicate an issue of some sort.

                  --
                  Phillip

                  Comment

                  • stacy09
                    Junior Member
                    • Apr 2013
                    • 2

                    #10
                    help with fastQC per base sequence content

                    Hi,

                    I am a beginner of RNA-seq data analysis. I did fastQC of my samples and I found some variations at the beginning of reads for per base seqence content check. would you please tell me whether it is ok?

                    Many thanks in advance!
                    Attached Files

                    Comment

                    • kmcarr
                      Senior Member
                      • May 2008
                      • 1181

                      #11
                      Originally posted by stacy09 View Post
                      Hi,

                      I am a beginner of RNA-seq data analysis. I did fastQC of my samples and I found some variations at the beginning of reads for per base seqence content check. would you please tell me whether it is ok?

                      Many thanks in advance!
                      See this previous thread for a discussion of this phenomenon.

                      Comment

                      • stacy09
                        Junior Member
                        • Apr 2013
                        • 2

                        #12
                        kmcarr,

                        Thanks a lot!

                        Comment

                        • Aditi Verma
                          Junior Member
                          • Mar 2016
                          • 3

                          #13
                          Hello,

                          I ran FastQC through RNA-seq done on ribodepleted samples and the per base sequence content and per base GC content shows a very heavy bias (If I am correctly interpreting the results). Is this expected in data from ribodepleted RNA. Can this data be used at all?
                          Please find the image attached. Thanks for your help in advance!
                          Attached Files
                          Last edited by Aditi Verma; 02-15-2017, 01:52 AM.

                          Comment

                          • GenoMax
                            Senior Member
                            • Feb 2008
                            • 7142

                            #14
                            @Aditi: Have you scanned/trimmed this data for presence of Illumina adapters? I wonder if you have a large percentage of adapter dimers (and no real inserts).

                            I recommend using bbduk.sh from BBMap for this purpose. Search for the thread on bbduk here.

                            Comment

                            • pmiguel
                              Senior Member
                              • Aug 2008
                              • 2328

                              #15
                              Looks like about 20-25% of your reads are from adapter dimers.

                              --
                              Phillip

                              Comment

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