Seqanswers Leaderboard Ad

Collapse

Announcement

Collapse
No announcement yet.
X
Collapse
 
  • Page of 1
  • Filter
  • Time
  • Show
Clear All
new posts
Previous template Next
  • #1

    Indexing- Exons and splice sites

    Hi,
    I have been following the github tutorial, https://github.com/griffithlab/rnaseq_tutorial/wiki

    to learn RNAseq.

    I was on the indexing step and it says to first export exons and splice sites from reference genome using in-built python scripts before starting the indexing. And then that this information will be used during alignment.

    It would be great if someone could explain the rationale behind this step.
    ----
    Tags: exons, hisat2, indexing, ngs, splice sites
  • #2
    Sometimes if you are happy with the current state of the transcriptome (known expressed parts of the genome) then you could choose to do alignments of your data just to that part.

    While that is not incorrect, you do run a small risk of having some reads mis-align (since an aligner does its best to align and the read may not have originally come from that region) by restricting to just "known" expressed parts of the genome. If splice sites are provided as well then the programs would not try to look for new ones. Both these modifications speed up the alignments to some extent.

    Comment

    • #3
      Originally posted by GenoMax View Post
      Both these modifications speed up the alignments to some extent.
      That's okay. But while using the HISAT2 program, I am extracting the splice site and exon information from the .gtf file. And that information is given to the index builder (Hisat2-build). So, what I am getting is that this information during indexing is helping during alignment.

      If I know the splice sites, the reads will not align to those parts where splice sites lie in the middle. Is this correct?
      I still don't get how exon info is helping in alignment.

      A little more detailed answer would be really really helpful.

      Thank you.
      ----

      Comment

      • #4
        The most intuitive explanation might be that those "known" exons and splice sites are used as a suggestion for the read mapping, making mapping much quicker since the aligner "knows" where to look. Reads that don't behave according to the "known" annotation will still get correctly aligned and new splice sites will be discovered.

        You are just "telling" the aligner a priori where the splice junctions most likely are (but not restricting the mapping to those junctions/exons).

        Comment

        • #5
          Okay. That makes sense.

          Thank you very much.
          ----

          Comment

          • #6
            Does including exons and splice sites make the alignment more accurate, faster, or both?

            Comment

            Previous template Next

            Latest Articles

            Collapse
            • seqadmin
              Best Practices for Single-Cell Sequencing Analysis
              by seqadmin



              While isolating and preparing single cells for sequencing was historically the bottleneck, recent technological advancements have shifted the challenge to data analysis. This highlights the rapidly evolving nature of single-cell sequencing. The inherent complexity of single-cell analysis has intensified with the surge in data volume and the incorporation of diverse and more complex datasets. This article explores the challenges in analysis, examines common pitfalls, offers...
              Today, 07:15 AM
            • seqadmin
              Latest Developments in Precision Medicine
              by seqadmin



              Technological advances have led to drastic improvements in the field of precision medicine, enabling more personalized approaches to treatment. This article explores four leading groups that are overcoming many of the challenges of genomic profiling and precision medicine through their innovative platforms and technologies.

              Somatic Genomics
              “We have such a tremendous amount of genetic diversity that exists within each of us, and not just between us as individuals,”...
              05-24-2024, 01:16 PM
            View All

            ad_right_rmr

            Collapse

            News

            Collapse
            Topics Statistics Last Post
            New Method for DNA Sequence Amplification by seqadmin
            Started by seqadmin, Today, 08:18 AM
            0 responses
            8 views
            0 likes
            		 Last Post seqadmin
            by seqadmin
            Today, 08:18 AM  
            New Tools Enhance Single-Molecule DNA Analysis with Minimal Samples by seqadmin
            Started by seqadmin, Today, 08:04 AM
            0 responses
            10 views
            0 likes
            		 Last Post seqadmin
            by seqadmin
            Today, 08:04 AM  
            SIX2 Protein Identified as a Key Player in Prostate Cancer Treatment Resistance by seqadmin
            Started by seqadmin, 06-03-2024, 06:55 AM
            0 responses
            13 views
            0 likes
            		 Last Post seqadmin
            by seqadmin
            06-03-2024, 06:55 AM  
            Genetic Mosaicism More Prevalent Than Previously Thought by seqadmin
            Started by seqadmin, 05-30-2024, 03:16 PM
            0 responses
            27 views
            0 likes
            		 Last Post seqadmin
            by seqadmin
            05-30-2024, 03:16 PM  
            View All
            Working...
            X