Galaxy-using trimmomatics with ChIP seq pair ended (only one file with both reads)

Heads up! This is a static archive of our support site. Please go to help.galaxyproject.org if you want to reach the Galaxy community. If you want to search this archive visit the Galaxy Hub search

Latest

Open

RNA-Seq

ChIP-Seq

SNP

Assembly

Forum

Home

Welcome to Galaxy Biostar! User support for Galaxy! about • faq • rss

Log In

Sign Up

Question: Galaxy-using trimmomatics with ChIP seq pair ended (only one file with both reads)

0

14 months ago by

jramo033 • 20

jramo033 • 20 wrote:

I am trying to run Trimmomatics in Galaxy under "pair end (as collection)" for afastqsanger.gz file with both reads and I got the message "no fastqsanger.gz dataset collection available". What should I do? split the file into two different files? if so, how can I do it? Is there any other way?

chip-seq • 390 views

ADD COMMENT • link •

modified 14 months ago by Jennifer Hillman Jackson ♦ 25k • written 14 months ago by jramo033 • 20

0

14 months ago by

Jennifer Hillman Jackson ♦ 25k

United States

Jennifer Hillman Jackson ♦ 25k wrote:

Hello,

Check the metadata for your input dataset collection - it should be assigned the fastqsanger.gz datatype.

How-to:

Support https://galaxyproject.org/support/ > first two links explain datatype assignment: https://galaxyproject.org/support/#getting-inputs-right-
Learn https://galaxyproject.org/learn/ > dataset collections tutorial: https://galaxyproject.org/tutorials/collections/

Thanks, Jen, Galaxy team

ADD COMMENT • link written 14 months ago by Jennifer Hillman Jackson ♦ 25k

Please log in to add an answer.

Similar posts • Search »

Help! I'm using trimmomatic in Galaxy, but it doesn't recognize a part of input dataset.
I'm using Trimmomatic to trimming paired end reads. When I set "Single-end or paired-end reads?"...
Trimmomatic output after filtering paired end data - fastqsanger vs fastqsanger.gz
After running Trimmomatic on a paired end PolyA RNA-seq dataset where both forward and reverse re...
Running Trimmomatic on loop for Paired End
I'm need to do trimming for Paired End. Is there any way around where I can run the trimmomatic ...
RNAseq data to be processed in two ways: (i) mapping to de novo Trinity-based transcriptome and (ii) mapping a relatively new genome
Hello all, I am new to RNAseq data and learning this process step by step, so I have a few quest...
Paired end illumina RNAseq reads - running trinity with paired trimmed files and adding unpaired as single read?
We have paired end Illumina HiSeq 4000 reads that we are working to remove adaptors and trim base...
Splitting Biased Paired End FASTQ data
The FASTQ splitter in Galaxy warns that the tool only works if Paired-end data has equal length r...
Trimmomatic and Trim Galore are not working.
I am performing an RNA-seq and am trying to trim adapter sequences with Trim Galore. When I made ...
fastq splitter problem
fastq splitter is not working on paired end read for some of my file and produce output file with...
Nextera pair end adapter cleaning
Can I use Nextera pair end adapter option in Galaxy Trimmomatic program for cleaning my illumina ...
Help with downloading files from EBI SRA
I am new to galaxy and have been trying to figure out how to align RNA-seq reads to a genome in o...
Trimmomatic on paiera end data
Hi I am trying to use Trimmomatic on my Sanger Illumina 1.9 paired end data. Trimmomatic ask fo...
my tool and collections
Hello, I want to do something related to writing my own tool (in perl) and 'collections'. I have...
Data collection and Tophat2
Hi, I am trying to play with data collection (developped by John Chilton) and I am confused on h...
Kraken (assign taxonomic label...)
One Illumina file fastq.gz contain all info about paired-end reads. I used by usegalaxy interface...
Trinity run preprocessing
I am new to Trinity and galaxy instance (https://usegalaxy.org/). I have 17 samples pair ended. I...
filtering pair-end bam file
Hello, I am trying to filter a pairend bam file to get only forward reads in Galaxy. A bam filter...
Combining The Paired Reads From Illumina Run
Hi, I have two fastq files with the forward(/1) and reverse(/2) paired reads. The reads are not ...

Content

Help

About
FAQ

Access

RSS
Stats
API

Use of this site constitutes acceptance of our User Agreement and Privacy Policy.

Powered by Biostar version 16.09

Traffic: 171 users visited in the last hour