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

    Tile is missing

    Hi all,

    I received some fastq files from a PE HiSeq and when I tried to isolate N reads using the "fastq_illumina_reads -N" I got the following error:

    Input error: file 'STDIN' line 1: Expecting Illumina-CASAVA1.8 ID line structure (@<instrument>:<run number>:<flowcell ID>:<lane>:<tile>:<x-pos>:<y-pos> <read>:<is filtered>:<control number>:<index sequence>) - got '@HS34_23148:4:1313:16347:42480/1' (Can't extract 'Tile’)



    The header of the file shows:
    @HS34_23148:4:2106:12625:73859/2
    CACCAGCTGAGAGAGATGCTCGCCGTTGACTGACGAACTGAATTCCCAGTTCACGGCGGTATGGAATACCGTCGT
    +
    BBBBBFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFF
    @HS34_23148:4:1114:12855:77248/2
    CTCGCCGTTGACTGACGAACTGAATTCCCAGTTCACGGCGGTATGGAATACCGTCGTCGCAGAGCTCAACGGTGA
    +
    BBBBBFFFFFFFFFFFFFFFFFFFBFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFBFFFFFFFFFFFFF
    @HS34_23148:4:1311:2663:94744/2
    CTCGACAGATATTGATTGTCGTCACCGTTGAGCTCTGCGACGACGGTATTCCATACCGCCGTGAACTGGGAATTC

    Does anyone already get the same problem with the tile coordinates?
    (I could ask the facility who sent me the files an explanation but I'm not sure if the problem come from me or not)

    Thank you
    Tags: None
  • #2
    Originally posted by jmlabioinfo View Post
    Hi all,

    I received some fastq files from a PE HiSeq and when I tried to isolate N reads using the "fastq_illumina_reads -N" I got the following error:

    Input error: file 'STDIN' line 1: Expecting Illumina-CASAVA1.8 ID line structure (@<instrument>:<run number>:<flowcell ID>:<lane>:<tile>:<x-pos>:<y-pos> <read>:<is filtered>:<control number>:<index sequence>) - got '@HS34_23148:4:1313:16347:42480/1' (Can't extract 'Tile’)



    The header of the file shows:
    @HS34_23148:4:2106:12625:73859/2
    CACCAGCTGAGAGAGATGCTCGCCGTTGACTGACGAACTGAATTCCCAGTTCACGGCGGTATGGAATACCGTCGT
    +
    BBBBBFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFF
    @HS34_23148:4:1114:12855:77248/2
    CTCGCCGTTGACTGACGAACTGAATTCCCAGTTCACGGCGGTATGGAATACCGTCGTCGCAGAGCTCAACGGTGA
    +
    BBBBBFFFFFFFFFFFFFFFFFFFBFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFFBFFFFFFFFFFFFF
    @HS34_23148:4:1311:2663:94744/2
    CTCGACAGATATTGATTGTCGTCACCGTTGAGCTCTGCGACGACGGTATTCCATACCGCCGTGAACTGGGAATTC

    Does anyone already get the same problem with the tile coordinates?
    (I could ask the facility who sent me the files an explanation but I'm not sure if the problem come from me or not)

    Thank you
    It looks like you got hold of a very old (in Illumina time scale) FastQ file. Have a look at the Illumina sequence identifiers discussion on the FastQ format Wikipedia page. The sequence headers in your file are the pre-CASAVA 1.8 format. The software you are trying to use (fastq_illumina_reads) is expecting the header format to be the post-CASAVA 1.8 format. I can't remember when that format version was first introduced but it was years ago.

    What software package is the fastq_illumina_reads program from? Does it have a command line option to switch between the old and new FastQ sequence ID line formats?

    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