Tophat errors with alignment summary and insertions data

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: Tophat errors with alignment summary and insertions data

1

2.3 years ago by

darsha_7 • 10

darsha_7 • 10 wrote:

Hello,

I have encountered a problem after using Tophat. I started off with fasta file of my genome reference and a gff3 file of annotation reference. Nine sets of rnaseq data uploaded in my history. I managed to run TopHat for the first two RNAseq data sets and was able to obtain all results from Tophat. However for 5 datasets, there was a problem with the alignment summary, saying that an error occurred setting the metadata for this dataset. It was suggested to set it manually or retry auto-detection.

For the last two datasets, both alignment summary and insertions data from Tophat had this problem. Do you reckon if there is a problem with the RNAseq data file? If so, will there be a way to repair RNAseq data file? Could you please look into this for me and advice.

Many thanks, Darsha

rna-seq tophat alignment • 766 views

ADD COMMENT • link •

modified 2.3 years ago by Jennifer Hillman Jackson ♦ 25k • written 2.3 years ago by darsha_7 • 10

Dear Darsha,

I've had a similar problem awhile back. You can try setting the metadata manually by clicking the pencil icon (edit attributes) next to your file that failed and then see if it can perform the downstream analysis steps (cufflinks etc).

From my experience it wont, and it was due to a miss-match with my gff3 file. Is there a specific reason you aren't running tophat using a genome already on galaxy?

ADD REPLY • link written 2.3 years ago by VY • 120

0

2.3 years ago by

Jennifer Hillman Jackson ♦ 25k

United States

Jennifer Hillman Jackson ♦ 25k wrote:

Hello Darsha,

Resetting the metadata is enough to create output that can be used with downstream tools. The jobs do not need to be re-run.

This has been reported a few times but we didn't have an example history with undeleted/uncorrected datasets present. But I was able to grab a quick copy of yours for our administrator to reference - he is troubleshooting right now.

Apologies for the confusion and thanks for reporting the problem!! Jen, Galaxy team

ADD COMMENT • link written 2.3 years ago by Jennifer Hillman Jackson ♦ 25k

Thank you for your help Jen and team. It works now!

ADD REPLY • link written 2.3 years ago by darsha_7 • 10

Please log in to add an answer.

Similar posts • Search »

TopHat align summary
Hello, I am using galaxy to analyze RNA seq of 100bp sing end data, sequenced with Illumina 2500...
Insert sizes in Galaxy
I am new to RNASeq analysis. I used tophat to generate BAM files from FASTQ files but in the para...
Cannot join combined R1 and R2 files
Hi Everyone, From reading around, I'm not sure whether a solution has been found to the probl...
Problem running Clustal 2.1 Multiple Sequences Alignment - an instance of 'std::bad_alloc'
Dear All, I've been trying to analyze reads from a short transcript. The data I have was obtaine...
Re: Trouble Getting Tophat To Run On Built-In Index Genome
Hi Noa, There are two issues: Using the correct genome and setting up paired data properly. 1 -...
Tophat Gapped-read mapper for RNA-seq data
1 job has been successfully added to the queue - resulting in the following datasets: 18: Tophat...
i cannot find the fastq files inside datasets of bwa-mem although present in history
please help me in that i uploaded two fastq files into history and started bwa-mem to align them...
Problem with Tophat
I'm trying follow the steps of the example from the Galaxy Training on RNAseq. After loading the...
analysis of tophat results
hi i have done qc and then groomed single end sra sequences from ebi. i ran tophat. i am getting...
Problems With Tophat
Hello, I have successfully used the public server for processing RNAseq data but I have run into...
De novo transcriptome assembly and reference guided transcriptome assembly
Hi, I have four related questions about de novo RNAseq data analysis. I have 4 RNAseq data obtai...
Cloudman - Galaxy - TopHat2 error
Hi all, I'm going through the RNAseq tutorial posted here: https://usegalaxy.org/u/jeremy/p/gal...
Paired-end insert size upper limit
I am mapping paired-end reads using Bowtie2 and setting "maximum insert size for valid paired-end...
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...
TopHat error message
Hi, I've been trying to run TopHat on my RNAseq data. I ran my data through FastQC and then Trim...
Errors in post alignment files
Hello. I was trying to perform an alignment of data (Tophat) which had been run through Fast Gro...
Dataset generation errors while running Bowtie these days
Dear Galaxy, I found from two days ago, when I used Bowtie to map my RNAseq data, it either show...
cummerbund tool error
Hello, I recently tried differential gene expression analysis using an established workflow. I h...
Tophat Settings
In the new version of tophat they allow for over 3 mismatches in the initial alignment, however y...
zero cuffdiff FPKM values SusScrofa
Good morning, I am a beginner in RNAseq Galaxy interface and I have a problem with all zero FPKM...
Reference Annotation error using HISAT2
I keep getting a reference annotation error when I run cuffdiff using HISAT2 alignment files. The...
Tophat Results
Dear galaxy users, I aligned my RNA-seq data by using Tophat in galaxy. It generated some "...

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: 183 users visited in the last hour