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  • hui_shi
    Junior Member
    • Oct 2010
    • 6

    problem with sra toolkit fastq-dump sratoolkit.2.1.10-win64

    Hello,

    I was trying to use fastq-dump to convert a .sra file to .fastq format.

    The data contains paired end reads, so when I type in commands,
    fastq-dump --split-files .sra, it gives two files, *_1.fastq and *_2.fastq.

    But the problem is the size of the two files are different, one is a lot bigger than the other. This doesn't seems to be right.

    Does anyone know why this happens? and how to fix it? Shouldn't the two files contain the same number of reads, so that the size should be the same as well?

    Thank you,

    Hui
    Last edited by hui_shi; 06-15-2012, 05:11 AM.
  • vadim
    Member
    • Sep 2009
    • 37

    #2
    Could you post the run accession please?

    Comment

    • hui_shi
      Junior Member
      • Oct 2010
      • 6

      #3
      Thanks for your reply. I didn't use --accession or -A, don't know if that's what you mean. Actually, I don't understand why using -A, except to modify the output name.

      The full command I typed in was:

      fastq-dump --split-files SRR443885.sra

      it generates two files, SRR443885_1.fastq and SRR443885_2.fastq, but they are of different size.

      Thanks,

      Hui
      Last edited by hui_shi; 06-15-2012, 06:01 AM.

      Comment

      • vadim
        Member
        • Sep 2009
        • 37

        #4
        The spot descriptor claims that the read length is 150bp, 75 forward and 75 reverse. But the actual read length is 100 bases only. I guess fastq-dump just obeys the rules by splitting the read at 75, so the reverse read becomes 3 times smaller than the forward.

        The run metadata is here:


        The experiment metadata is here:


        You can contact them at sra@ncbi about this.

        Comment

        • emp
          Member
          • Jan 2014
          • 11

          #5
          regarding small sra format file

          I wanted to convert .sra file of size 289.98 Mb. when i am using sratool fastq-dump.. it is generating error message as:-



          An error occurred during processing.
          A report was generated into the file '.../ncbi_error_report.xml'.
          If the problem persists, you may consider sending the file


          kindly help me out for this ASAP

          Comment

          • dpryan
            Devon Ryan
            • Jul 2011
            • 3478

            #6
            Did you try looking at what was in the file? Given that it's an error report, perhaps it's informative...

            Comment

            • emp
              Member
              • Jan 2014
              • 11

              #7
              Respected dpryan,


              The file is in xml format which on opening with google chrome is giving code. It does'nt have any error specified there in...

              Here in is the file which i am trying to convert to fastq.

              Comment

              • dpryan
                Devon Ryan
                • Jul 2011
                • 3478

                #8
                Try upgrading your copy of the SRA toolkit, that usually fixes this sort of issue (I tried to extract the file you linked and couldn't until I upgraded my local copy of fastq-dump).

                Comment

                • emp
                  Member
                  • Jan 2014
                  • 11

                  #9
                  kindly tell me how can i upgrade sra tool kit??


                  Is it through verbose??

                  Comment

                  • dpryan
                    Devon Ryan
                    • Jul 2011
                    • 3478

                    #10
                    Try here, on NCBI

                    Comment

                    • tw7649116
                      Junior Member
                      • Mar 2014
                      • 8

                      #11
                      Dear hui_shi,

                      I have the same problem with convert the sra to pair-end fastq.
                      Do you remember how to solve this problem?

                      Thank you very much!!

                      Comment

                      • GenoMax
                        Senior Member
                        • Feb 2008
                        • 7142

                        #12
                        Are you using the latest SRAtoolkit? Have you done the steps described in this post: http://seqanswers.com/forums/showpos...6&postcount=7?

                        Comment

                        • tw7649116
                          Junior Member
                          • Mar 2014
                          • 8

                          #13
                          Thank you GenoMax,

                          I used the latest version.
                          In that way we need to redownload the file?
                          Thank you! If I can't solve this, may be I need to download again!

                          Best wishes

                          Comment

                          • GenoMax
                            Senior Member
                            • Feb 2008
                            • 7142

                            #14
                            If you have downloaded the .sra file have you tried the command this way?

                            Code:
                            c:\> fastq-dump.exe -F --split-files c:\path_to\SRAfile.sra
                            Sometimes people do submit unequal length data sets so if you have mismatched cycle numbers that is a possibility. What SRA# are you looking at?

                            Comment

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