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  • #1

    a question in using Flux Simulator

    I am using Flux Simulator to simulate RNA-Seq experiment, and after running

    flux-simulator -p /HS_simu1.par

    I got the following error message:

    [ERROR] Error while preparing sequences: Problems reading sequence GL000191.1: pos -1, len 171, check whether chromosomal sequence exists / has the correct size

    Can I know which file I should check for chromosomal sequence? Thanks!
    Tags: None
  • #2
    I have just had a similar problem with Flux Simulator - I think this problem is caused by a transcript (in your ENSEMBL(?) GTF) that belongs to GL000191.1 "non-chromosomal" contig, while you only provided Flux with "chromosomal" fasta files. The easiest way to solve it is to filter all the "non-chromosomal" annotations from the GTF, or you can add the "non-chromosomal" fasta files.

    Comment

    • #3
      Originally posted by alexdobin View Post
      I have just had a similar problem with Flux Simulator - I think this problem is caused by a transcript (in your ENSEMBL(?) GTF) that belongs to GL000191.1 "non-chromosomal" contig, while you only provided Flux with "chromosomal" fasta files. The easiest way to solve it is to filter all the "non-chromosomal" annotations from the GTF, or you can add the "non-chromosomal" fasta files.
      Thank you alexdobin for the suggestions! Can I know how you solved this problem (i.e. modifications of the GTF file...)?

      Comment

      • #4
        Since I did not need annotations on non-chromosomal scaffolds, I simply removed all the non-chromosomal entries from the GTF file. For ENSEMBL GTF, the chromosomes are 1-22,X,Y,MT, so you could simply do:
        grep ^[0-9XYM] ENSEMBL.gtf > ENSEMBL.chrOnly.gtf

        On the other hand, if you want to simulate RNA-seq from non-chromosomal scaffolds, you will need to downolad the "nonchromosomal" fasta file from ENSEMBL (e.g. ftp://ftp.ensembl.org/pub/release-72...omosomal.fa.gz), split the file into separate fasta files for each of the scaffolds, and add these fasta files to the GEN_DIR directory.

        Comment

        • #5
          I've run into a similar problem with whole chromosomes. At the time I assumed the simulator may try to grab sequence past the end of a chromosome when there are genes near the end of a chromosome. My simple workaround was to pad the end of each chromosome sequence with enough N's to accommodate my desired read size.

          It's possible the same solution would work with contigs/scaffolds if you don't want to eliminate them from your simulations.

          Comment

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