Seqanswers Leaderboard Ad

Collapse

Announcement

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

  • Trinity contig filtering

    Hello, all,

    I have just got my Trinity assembly, the N50 looks good. However, I have 100 contigs length extends from 4000bp to 11700bp.
    Because we don't expect the contig size to be above 4000bp, so is this because of some genomic contaimination?
    And can anyone suggest a program or script that can filter out the bad contigs? Thanks a lot,

  • #2
    I'm not sure what those contigs would be. Maybe chimeras? Have you tried blasting them?

    If you're just looking to get rid of all sequences over 'x' length, then you can do something like below (if you have bioPerl installed). Usage: perl script.pl --in startingfile.fas --cutoff 4000 --out prunedfile.fas


    Code:
    #!/usr/bin/perl
    
    use strict;
    use warnings;
    use Getopt::Long;
    use Bio::SeqIO;
    
    my $inFile;
    my $cutoff;
    my $outFile;
    
    GetOptions  ("in=s"      => \$inFile,
                 "cutoff=i"  => \$cutoff,
                 "out=s"     => \$outFile) || die "Couldn't get parameters with Getopt::Long.\n";
    
    my $seqIn = Bio::SeqIO->new(-file   => $inFile,
                                -format => 'fasta');
    my $seqOut = Bio::SeqIO->new(-file   => ">$outFile",
                                 -format => 'fasta');
    
    while (my $seq = $seqIn->next_seq()) {
        if ($seq->length() < $cutoff) {
            $seqOut->write_seq($seq);
        }
    }
    Last edited by atcghelix; 10-10-2013, 09:30 PM. Reason: Mention that you need bioPerl for this to run.

    Comment


    • #3
      Thanks, it helps

      Comment


      • #4
        Originally posted by ripeapple View Post
        Hello, all,

        I have just got my Trinity assembly, the N50 looks good. However, I have 100 contigs length extends from 4000bp to 11700bp.
        Because we don't expect the contig size to be above 4000bp, so is this because of some genomic contaimination?
        And can anyone suggest a program or script that can filter out the bad contigs? Thanks a lot,
        Its possible its prespliced or incompletely spliced RNAs. However, why do you assume you shouldn't have >4000bp contigs? Ttn is >100,000bp. So certainly there are genes this big.

        Also, have you tried Trinity's downstream analysis modules. They are very good at picking out protein coding orfs and blasting your dataset to identify orthologs

        Comment


        • #5
          Yes, you're right,
          I was thinking to remove the possible genomic contamination at first to set a cutoff for contig size.
          Now I guess I need to map the sequence back to assembly see how it goes,
          Thanks,

          Comment

          Latest Articles

          Collapse

          • seqadmin
            Recent Developments in Metagenomics
            by seqadmin





            Metagenomics has improved the way researchers study microorganisms across diverse environments. Historically, studying microorganisms relied on culturing them in the lab, a method that limits the investigation of many species since most are unculturable1. Metagenomics overcomes these issues by allowing the study of microorganisms regardless of their ability to be cultured or the environments they inhabit. Over time, the field has evolved, especially with the advent...
            09-23-2024, 06:35 AM
          • seqadmin
            Understanding Genetic Influence on Infectious Disease
            by seqadmin




            During the COVID-19 pandemic, scientists observed that while some individuals experienced severe illness when infected with SARS-CoV-2, others were barely affected. These disparities left researchers and clinicians wondering what causes the wide variations in response to viral infections and what role genetics plays.

            Jean-Laurent Casanova, M.D., Ph.D., Professor at Rockefeller University, is a leading expert in this crossover between genetics and infectious...
            09-09-2024, 10:59 AM

          ad_right_rmr

          Collapse

          News

          Collapse

          Topics Statistics Last Post
          Started by seqadmin, 10-02-2024, 04:51 AM
          0 responses
          8 views
          0 likes
          Last Post seqadmin  
          Started by seqadmin, 10-01-2024, 07:10 AM
          0 responses
          13 views
          0 likes
          Last Post seqadmin  
          Started by seqadmin, 09-30-2024, 08:33 AM
          0 responses
          18 views
          0 likes
          Last Post seqadmin  
          Started by seqadmin, 09-26-2024, 12:57 PM
          0 responses
          16 views
          0 likes
          Last Post seqadmin  
          Working...
          X