[IGBF-3143] Run RNA-Seq data processing pipeline on positive splicing control and experimental samples - JIRA UNCC

Details

Type: Task
Status: Closed (View Workflow)
Priority: Major
Resolution: Done
Affects Version/s: None
Fix Version/s: None
Labels:
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Story Points:
3
Epic Link:
Support NSF pollen grant
Sprint:
Summer 4 2022 July 4, Summer 5 2022 July 18, Summer 6 2022 Aug 1, Fall 1 2022 Aug 15

Description

Data sets to process:

Positive control: SRP328042 Data are published in this article.
Experimental: SRP252265

To-Do:

Obtain data in fastq format from Sequence Read Archive using fasterqdump options for paired end data - DONE
Please data into directories named for the SRP number, e.g., SRP328042 and SRP252265 within a directory named "alt_splicing" under "nobackup" - DONE
Make a note of the particular commands used to perform the data retrieval (see comment below)
Create "samples" text file listing the SRR fastq files for running nf-core/rna-seq nextflow
Run nf-core/rnaseq using proper maximum intron size parameter using "tomato.config"

Notes:

Experimental datasets originally processed using code in https://bitbucket.org/hotpollen/rna-seq/src/master/ and https://bitbucket.org/hotpollen/flavonoid-rnaseq
All Pollen project datasets are now in the SRA under the same project number ! (SRP252265)
Ann is using a fork of flavonoid-rnaseq for all new code she's writing, on branch ~~IGBF-3143~~. To find her fork, go to https://bitbucket.org/hotpollen/flavonoid-rnaseq and select "forks"
Documentation for the pipeline we are using is here: https://nf-co.re/rnaseq/3.4/usage

Methods used to create positive control RNA-Seq data from SRP328042, according to the paper:

2.5.2. Preparation of RNA-Seq Library and Sequencing Total RNA was extracted utilizing Trizol reagent (Invitrogen, Waltham, MA, USA). RNA quantity and quality were determined by NanoDrop 1000 spectrophotometer (Thermo Scientific Inc., Waltham, MA, USA), 1% agarose gel electrophoresis and Agilent 2100 Bioanalyzer (Agilent Technologies, Palo Alto, CA, USA). Following the protocol described by [28], strand-specific RNA-Seq libraries from 3 biological replicates for each group from WW and DS anthers were prepared using 1 ng/µL of total RNA sample and sequenced by Novogene Biotech (Beijing, China) on Illumina HiSeq 4000 system (Illumina, Inc., San Diego, CA, USA) according to the manufacturer’s instructions. The raw sequence reads were deposited into NCBI Sequence Read Archive under accession the number PRJNA746070.

A PDF copy of the protocol paper (reference 28) for RNA-Seq library synthesis is attached.

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Attachments

10.1.1.1052.3871.pdf
393 kB
25/Jul/22 1:39 PM

Issue Links

blocks

IGBF-3144 Make annots.xml for RNA-Seq junction, alignment, and coverage graphs

Closed

IGBF-3165 Make junction files for experimental and positive control alignments data

Closed

is blocked by

IGBF-3127 Version control nf-core configuration files used for rna-seq analysis

Closed

relates to

IGBF-2970 Re-run nf-core/rnaseq using proper strand designation and better sample prefix

Closed

IGBF-3127 Version control nf-core configuration files used for rna-seq analysis

Closed

IGBF-3162 Generate scaled coverage graphs for RNA-Seq alignments

Closed

IGBF-3228 Download and process data for SRP100604 and SRP268884

Closed

IGBF-2947 Investigate using nf-core/rnaseq pipeline

Closed

IGBF-3135 Add new tomato genome and annotations to IGB Quickload repository

Closed

Show 4 more links (4 relates to)

Activity

People

Assignee:

Molly Davis

Reporter:

Ann Loraine

Votes:

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Watchers:

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Dates

Created:

07/Jul/22 12:16 PM

Updated:

17/Nov/22 12:49 PM

Resolved:

26/Aug/22 12:54 PM