Overview of today’s session:
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inspect the results from Session 2
run an advanced RNA-seq pipeline to measure the expression of genes
(optional) run statistical analysis to identify differentially expressed genes
Task 1: Evaluation of RNA-seq results using a basic (generic) nextflow pipeline
The nextflow/RNA-seq pipeline automatically generates two output folders:
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Connect to the work folder via HPC-FS (See session 2). Browse to the fastqc output folder: run1_star_salmon → results → multiqc.
Task 2: Run the nextflow nf-core/rnaseq pipeline by including advanced filtering parameters
Requirements:
index.csv → a file that provides a list of sample IDs and their associated FASTQ files (read 1 and read 2)
launch.pbs → a script to submit the job to the HPC cluster
Example index.csv file for nf-core/rnaseq version 3.3:
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group,fastq_1,fastq_2,strandedness control_r1,/work/kenna_team/data/raw_data/SRR1039508_1.fastq.gz,/work/kenna_team/data/raw_data/SRR1039508_2.fastq.gz,unstranded dex_r1,/work/kenna_team/data/raw_data/SRR1039509_1.fastq.gz,/work/kenna_team/data/raw_data/SRR1039509_2.fastq.gz,unstranded control_r2,/work/kenna_team/data/raw_data/SRR1039512_1.fastq.gz,/work/kenna_team/data/raw_data/SRR1039512_2.fastq.gz,unstranded dex_r2,/work/kenna_team/data/raw_data/SRR1039513_1.fastq.gz,/work/kenna_team/data/raw_data/SRR1039513_2.fastq.gz,unstranded control_r3,/work/kenna_team/data/raw_data/SRR1039516_1.fastq.gz,/work/kenna_team/data/raw_data/SRR1039516_2.fastq.gz,unstranded dex_r3,/work/kenna_team/data/raw_data/SRR1039517_1.fastq.gz,/work/kenna_team/data/raw_data/SRR1039517_2.fastq.gz,unstranded control_r4,/work/kenna_team/data/raw_data/SRR1039520_1.fastq.gz,/work/kenna_team/data/raw_data/SRR1039520_2.fastq.gz,unstranded dex_r4,/work/kenna_team/data/raw_data/SRR1039521_1.fastq.gz,/work/kenna_team/data/raw_data/SRR1039521_2.fastq.gz,unstranded |
Example of a launch.pbs script with advanced parameter options:
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cp /work/kenna_team/scripts/star_rsem/session3/* . |
Task 3 - Differential gene expression analysis
Differential expression analysis using https://maayanlab.cloud/biojupies/analyze
From session 2, we will use the feature counts generated using the ‘star_salmon’ parameter setting. Either copy the relevant files (see below) to your laptop from the HPC or download the files below.
File | File name | File | ||||
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Gene feature counts | salmon_merged.gene_counts.tsv |
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Transcript feature counts | salmon_merged.transcript_counts.tsv |
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Follow up task:
Once the session 3 run_start_salmon has completed, run task 3 above with the newly generated feature counts. Do you observe the same findings?