[IGBF-3758] Trinity NEXTFLOW alignment - JIRA UNCC

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Type: Task
Status: Closed (View Workflow)
Priority: Major
Resolution: Done
Affects Version/s: None
Fix Version/s: None
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Sprint:
Summer 1

Description

GOAL:

To use the newly annotated Trinity files as a REFERENCE to align reads to and determine gene expression for Kelsey's dataset.

There are 4 newly generated Trinity sets of contigs (TMNH). See ~~IGBF-3741~~.

Want to run NEXTFLOW. One for each variety.

Location of Trinity COntigs:
/projects/tomato_genome/fnb/dataprocessing/trinity/NEXTFLOW/postblat
(there should be 4 fasta files here, if not yet, soon.....)

The reads that will be used are here:
/projects/tomato_genome/rnaseq/renamed_Ravi_Combined

Instead of running ALL reads, we be separating by variety.
So only using the reads fr heinz with the Heinz trinity contig file......

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Robert Reid added a comment - 03/Jun/24 9:38 AM

This is a golden opportunity to test out Molly's pipeline document!

Used this document to run the pipeline: https://docs.google.com/document/d/1ig9ET-ykXF5nAX3P487cXWmZDGUlQpcwrvFXpbyP5vw/edit

And I will have Brandon try this out also and get familiar with the nextflow process.

This time however we will not be aligning to SL4 or SL5 but to the Trinity contigs.

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Robert Reid added a comment - 03/Jun/24 9:38 AM This is a golden opportunity to test out Molly's pipeline document! Used this document to run the pipeline: https://docs.google.com/document/d/1ig9ET-ykXF5nAX3P487cXWmZDGUlQpcwrvFXpbyP5vw/edit And I will have Brandon try this out also and get familiar with the nextflow process. This time however we will not be aligning to SL4 or SL5 but to the Trinity contigs.

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Robert Reid added a comment - 03/Jun/24 4:26 PM

Need all the pieces for next flow:

A csv file for the files (Using data from (SRP499796) sample,fastq_1,fastq_2,strandedness
Fasta file of the trinity Contigs
A GTF file
A genebed file
The tomato config file

Running this here: /projects/tomato_genome/fnb/dataprocessing/trinity/NEXTFLOW/hei-run1

Copied tomato config file from Molly's runs.

Got Fasts? Want GTF ? A perl script is hidden in the Trinity utils folder!! Works great.
perl /apps/pkg/trinity/2.14.0/util/misc/cdna_fasta_file_to_transcript_gtf.pl tamaulipas-trinity.Trinity.fasta | grep -w "exon" - > Trinity.gtf

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Robert Reid added a comment - 03/Jun/24 4:26 PM Need all the pieces for next flow: A csv file for the files (Using data from (SRP499796) sample,fastq_1,fastq_2,strandedness Fasta file of the trinity Contigs A GTF file A genebed file The tomato config file Running this here: /projects/tomato_genome/fnb/dataprocessing/trinity/NEXTFLOW/hei-run1 Copied tomato config file from Molly's runs. Got Fasts? Want GTF ? A perl script is hidden in the Trinity utils folder!! Works great. perl /apps/pkg/trinity/2.14.0/util/misc/cdna_fasta_file_to_transcript_gtf.pl tamaulipas-trinity.Trinity.fasta | grep -w "exon" - > Trinity.gtf

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Robert Reid added a comment - 05/Jun/24 11:53 AM

After presenting a few of these results to Kevin, he suggested that we use tools other than Trinity for this process.

Specifically, the tools RNA-Spades and RNA BLOOM 2.

Going to end this task in favor of exploring these potentially better options.
New tasks will be made for them.

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Robert Reid added a comment - 05/Jun/24 11:53 AM After presenting a few of these results to Kevin, he suggested that we use tools other than Trinity for this process. Specifically, the tools RNA-Spades and RNA BLOOM 2. Going to end this task in favor of exploring these potentially better options. New tasks will be made for them.

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Robert Reid

Reporter:

Robert Reid

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Dates

Created:

30/May/24 3:40 PM

Updated:

05/Jun/24 11:53 AM

Resolved:

05/Jun/24 11:53 AM