Seqanswers Leaderboard Ad

Collapse

Announcement

Collapse
No announcement yet.
X
 
  • Filter
  • Time
  • Show
Clear All
new posts

  • How can one identify "real" antisense transcripts in prokaryote genomes?

    Hello everyone,

    We are using directional RNA-seq (Illumina TruSeq® Stranded mRNA Sample Preparation Low Sample (LS) kit) to look at transcriptomes of marine microbes and have noticed that ~3-6% of our reads (after removal of rRNA both experimentally and computationally) map to the antisense of known genes. This can be very interesting biologically, but in some cases the antisense reads seem "sporadic" when compared to the sense reads, so we are looking for a computational method to differentiate between real antisense transcripts and "noise" generated during the library preparation.

    Does anyone have any idea what is the level of "strand fidelity" one can expect during library prep, or ideas on how to computationally select "bona-fide" antisense transcripts?

    Thanks
    Daniel

  • #2
    Maybe you can measure the antisense read coverage of the transcripts and calculate FPKM values, just like in "normal" RNA-Seq.

    Comment


    • #3
      First, if you used directional RNA-seq protocol you should be able to obtain directional libraries. So, if you made it right, antisense or reverse reads just reflect that; reverse reads to the gene direction.
      Second, I don't know too much about antisense or regulatory RNAs on prokaryotes; but they do exist. Maybe you have to leave it as a side project, but bacteria carries argonaute proteins which can be associated with small RNAs having regulatory activities over foreign gene, for instance:
      Eukaryotic Argonautes bind small RNAs and use them as guides to find complementary RNA targets and induce gene silencing. Though homologs of eukaryotic Argonautes are present in many bacteria and archaea, their small RNA partners and functions are unknown. We found that the Argonaute of Rhodobacter …


      As TiborNagy mentioned, look at the levels of these kind of antisense RNAs. You can use FPKM values or just measure count levels with htseq-count (-s reverse option). Don't know, on total mRNA experiment, the proportion of reverse reads that can be reflected (especially small RNAs). You normally have to do a specific library method for this kind of RNAs.

      Comment

      Latest Articles

      Collapse

      • seqadmin
        Advancing Precision Medicine for Rare Diseases in Children
        by seqadmin




        Many organizations study rare diseases, but few have a mission as impactful as Rady Children’s Institute for Genomic Medicine (RCIGM). “We are all about changing outcomes for children,” explained Dr. Stephen Kingsmore, President and CEO of the group. The institute’s initial goal was to provide rapid diagnoses for critically ill children and shorten their diagnostic odyssey, a term used to describe the long and arduous process it takes patients to obtain an accurate...
        12-16-2024, 07:57 AM
      • seqadmin
        Recent Advances in Sequencing Technologies
        by seqadmin



        Innovations in next-generation sequencing technologies and techniques are driving more precise and comprehensive exploration of complex biological systems. Current advancements include improved accessibility for long-read sequencing and significant progress in single-cell and 3D genomics. This article explores some of the most impactful developments in the field over the past year.

        Long-Read Sequencing
        Long-read sequencing has seen remarkable advancements,...
        12-02-2024, 01:49 PM

      ad_right_rmr

      Collapse

      News

      Collapse

      Topics Statistics Last Post
      Started by seqadmin, 12-17-2024, 10:28 AM
      0 responses
      33 views
      0 likes
      Last Post seqadmin  
      Started by seqadmin, 12-13-2024, 08:24 AM
      0 responses
      49 views
      0 likes
      Last Post seqadmin  
      Started by seqadmin, 12-12-2024, 07:41 AM
      0 responses
      34 views
      0 likes
      Last Post seqadmin  
      Started by seqadmin, 12-11-2024, 07:45 AM
      0 responses
      46 views
      0 likes
      Last Post seqadmin  
      Working...
      X