This is a continuation of the process for identification of lncRNAs,. I aligned FastQs which were previously trimmed earlier today to our Panopea-generosa-v1.0 genome FastA using HISAT2. I used the HISAT2 genome index created on 20190723, which was created with options to identify exons and splice sites. The GFF used was from 20220323. StringTie was used to identify alternative transcripts, assign expression values, and create expression tables for use with ballgown. The job was run on Mox.
SLURM script posted below is very long. Skip to RESULTS section.
SLURM script (GitHub):
#!/bin/bash
## Job Name
#SBATCH --job-name=20230426-pgen-HISAT2-stringtie-gffcompare-RNAseq
## Allocation Definition
#SBATCH --account=srlab
#SBATCH --partition=srlab
## Resources
## Nodes
#SBATCH --nodes=1
## Walltime (days-hours:minutes:seconds format)
#SBATCH --time=7-00:00:00
## Memory per node
#SBATCH --mem=120G
##turn on e-mail notification
#SBATCH --mail-type=ALL
#SBATCH --mail-user=samwhite@uw.edu
## Specify the working directory for this job
#SBATCH --chdir=/gscratch/scrubbed/samwhite/outputs/20230426-pgen-HISAT2-stringtie-gffcompare-RNAseq
## Script for HiSat2 alignments to P.generosa genome assembly Panopea-generosa-v1.0, running Stringtie to identify splice sites and calculate gene/transcript
##expression values (FPKM), formatted for import into Ballgown (R/Bioconductor), and gffcompare for GTF annotation.
## Process is part of identification of long non-coding RNAs (lnRNA) in geoduck.
## HiSat2 index generated on 20220914.
## https://robertslab.github.io/sams-notebook/posts/2022/2022-09-14-RNAseq-Alignments---P.generosa-Alignments-and-Alternative-Transcript-Identification-Using-Hisat2-and-StringTie-on-Mox/
## Using trimmed FastQs from 20230426.
## Expects FastQ input filenames to match <sample name>_val_[12].fastp-trim.20230426.fq.gz
## E.g. ctenidia_1_val_1.fastp-trim.20230426.fq.gz
###################################################################################
# These variables need to be set by user
## Assign Variables
# Set total number of SAMPLES (NOT number of FastQ files)
total_samples=5
# Set number of CPUs to use
threads=28
# Index name for Hisat2 use
# Needs to match index name used in previous Hisat2 indexing step
genome_index_name="Panopea-generosa-v1.0"
# Set input FastQ patterns
R1_fastq_pattern='*_val_1*fq.gz'
R2_fastq_pattern='*_val_2*fq.gz'
# Location of Hisat2 index files
# Must keep variable name formatting, as it's used by HiSat2
HISAT2_INDEXES=$(pwd)
export HISAT2_INDEXES
# Paths to programs
gffcompare="/gscratch/srlab/programs/gffcompare-0.12.6.Linux_x86_64/gffcompare"
hisat2_dir="/gscratch/srlab/programs/hisat2-2.1.0"
hisat2="${hisat2_dir}/hisat2"
samtools="/gscratch/srlab/programs/samtools-1.10/samtools"
stringtie="/gscratch/srlab/programs/stringtie-2.2.1.Linux_x86_64/stringtie"
# Input files/directories
genome_index_dir="/gscratch/srlab/sam/data/P_generosa/genomes"
genome_gff="${genome_index_dir}/Panopea-generosa-v1.0.a4_biotype-trna_strand_converted-no_RNAmmer.gff"
fastq_dir="/gscratch/scrubbed/samwhite/outputs/20230426-pgen-fastqc-fastp-multiqc-RNAseq/"
index_tarball="Panopea-generosa-v1.0-hisat2-indices.tar.gz"
# Output files/directories
gtf_list="gtf_list.txt"
merged_bam="20230216-pver-stringtie-pver_v1.0-sorted-bams-merged.bam"
# Declare associative array of sample names and metadata
declare -A samples_associative_array=()
# Programs associative array
declare -A programs_array
programs_array=(
[gffcompare]="${gffcompare}" \
[hisat2]="${hisat2}" \
[samtools_index]="${samtools} index" \
[samtools_merge]="${samtools} merge" \
[samtools_sort]="${samtools} sort" \
[samtools_view]="${samtools} view" \
[stringtie]="${stringtie}"
)
###################################################################################################
# Exit script if any command fails
set -e
# Load Python Mox module for Python module availability
module load intel-python3_2017
## Load associative array
## Only need to use one set of reads to capture sample name
# Set sample counter for array verification
sample_counter=0
# Load array
# DO NOT QUOTE ${R1_fastq_pattern} - WILL NOT POPULATE ARRAY!
for fastq in "${fastq_dir}"${R1_fastq_pattern}
do
# Increment counter
((sample_counter+=1))
# Remove path
sample_name="${fastq##*/}"
# Get sample name from first _-delimited field
sample_name=$(echo "${sample_name}" | awk -F "_" '{print $1}')
# Set treatment condition for each sample
# Used for setting read group (@RG) in SAM files
if [[ "${sample_name}" == "gonad" ]]
then
treatment="gonad"
elif [[ "${sample_name}" == "heart" ]]
then
treatment="heart"
elif [[ "${sample_name}" == "juvenile" ]]
then
treatment="juvenile"
elif [[ "${sample_name}" == "larvae" ]]
then
treatment="larvae"
fi
# Append to associative array
samples_associative_array+=(["${sample_name}"]="${treatment}")
done
# Check array size to confirm it has all expected samples
# Exit if mismatch
if [[ "${#samples_associative_array[@]}" != "${sample_counter}" ]] \
|| [[ "${#samples_associative_array[@]}" != "${total_samples}" ]]
then
echo "samples_associative_array doesn't have all ${total_samples} samples."
echo ""
echo "samples_associative_array contents:"
echo ""
for item in "${!samples_associative_array[@]}"
do
printf "%s\t%s\n" "${item}" "${samples_associative_array[${item}]}"
done
exit
fi
# Copy Hisat2 genome index files
echo ""
echo "Transferring HiSat2 index file now."
echo ""
rsync -av "${genome_index_dir}/${index_tarball}" .
echo ""
# Unpack Hisat2 index files
echo ""
echo "Unpacking Hisat2 index tarball: ${index_tarball}..."
echo ""
tar -xzvf ${index_tarball}
echo "Finished unpacking ${index_tarball}"
echo ""
#### BEGIN HISAT2 ALIGNMENTS ####
echo "Beginning HiSat2 alignments and StringTie analysis..."
echo ""
for sample in "${!samples_associative_array[@]}"
do
## Inititalize arrays
fastq_array_R1=()
fastq_array_R2=()
# Create array of fastq R1 files
# and generated MD5 checksums file.
# DO NOT QUOTE ${fastq_pattern}
for fastq in "${fastq_dir}"${R1_fastq_pattern}
do
# Remove path
sample_name="${fastq##*/}"
# Get sample name from first _-delimited field
sample_name=$(echo "${sample_name}" | awk -F "_" '{print $1}')
# Check sample names for match
if [[ "${sample_name}" == "${sample}" ]]
then
echo "Now working on ${sample} Read 1 FastQs."
fastq_array_R1+=("${fastq}")
echo "Generating checksum for ${fastq}..."
md5sum "${fastq}" >> input_fastqs_checksums.md5
echo "Checksum for ${fastq} completed."
echo ""
fi
done
# Create array of fastq R2 files
# DO NOT QUOTE ${fastq_pattern}
for fastq in "${fastq_dir}"${R2_fastq_pattern}
do
# Remove path
sample_name="${fastq##*/}"
# Get sample name from first _-delimited field
sample_name=$(echo "${sample_name}" | awk -F "_" '{print $1}')
# Check sample names for match
if [[ "${sample_name}" == "${sample}" ]]
then
echo "Now working on ${sample} Read 2 FastQs."
fastq_array_R2+=("${fastq}")
echo "Generating checksum for ${fastq}..."
md5sum "${fastq}" >> input_fastqs_checksums.md5
echo "Checksum for ${fastq} completed."
echo ""
fi
done
echo "Checksums for ${sample} Read 1 and 2 completed."
# Create comma-separated lists of FastQs for Hisat2
printf -v joined_R1 '%s,' "${fastq_array_R1[@]}"
fastq_list_R1=$(echo "${joined_R1%,}")
printf -v joined_R2 '%s,' "${fastq_array_R2[@]}"
fastq_list_R2=$(echo "${joined_R2%,}")
# Create and switch to dedicated sample directory
echo ""
echo "Creating ${sample} directory."
mkdir "${sample}" && cd "$_"
echo "Now in ${sample} directory."
# HiSat2 alignments
# Sets read group info (RG) using samples array
echo ""
echo "Running HiSat2 for sample ${sample}."
"${programs_array[hisat2]}" \
-x "${genome_index_name}" \
-1 "${fastq_list_R1}" \
-2 "${fastq_list_R2}" \
-S "${sample}".sam \
--rg-id "${sample}" \
--rg "SM:""${samples_associative_array[$sample]}" \
--threads "${threads}" \
2> "${sample}-hisat2_stats.txt"
echo ""
echo "Hisat2 for ${fastq_list_R1} and ${fastq_list_R2} complete."
echo ""
# Sort SAM files and convert to BAM
echo ""
echo "Sorting ${sample}.sam and creating sorted BAM."
echo ""
${programs_array[samtools_view]} \
-@ "${threads}" \
-Su "${sample}".sam \
| ${programs_array[samtools_sort]} - \
-@ "${threads}" \
-o "${sample}".sorted.bam
echo "Created ${sample}.sorted.bam"
echo ""
# Index BAM
echo ""
echo "Indexing ${sample}.sorted.bam..."
${programs_array[samtools_index]} "${sample}".sorted.bam
echo ""
echo "Indexing complete for ${sample}.sorted.bam."
echo ""
echo ""
echo "HiSat2 completed for sample ${sample}."
echo ""
#### END HISAT2 ALIGNMENTS ####
#### BEGIN STRINGTIE ####
# Run stringtie on alignments
# Uses "-B" option to output tables intended for use in Ballgown
# Uses "-e" option; recommended when using "-B" option.
# Limits analysis to only reads alignments matching reference.
echo "Beginning StringTie analysis on ${sample}.sorted.bam."
"${programs_array[stringtie]}" "${sample}".sorted.bam \
-p "${threads}" \
-o "${sample}".gtf \
-G "${genome_gff}" \
-C "${sample}.cov_refs.gtf" \
-B
echo "StringTie analysis finished for ${sample}.sorted.bam."
echo ""
#### END STRINGTIE ####
# Add GTFs to list file, only if non-empty
# Identifies GTF files that only have header
echo ""
echo "Adding ${sample}.gtf to ../${gtf_list}."
gtf_lines=$(wc -l < "${sample}".gtf )
if [ "${gtf_lines}" -gt 2 ]; then
echo "$(pwd)/${sample}.gtf" >> ../"${gtf_list}"
fi
echo ""
# Delete unneeded SAM files
echo "Removing SAM files."
echo ""
rm ./*.sam
# Generate checksums
for file in *
do
echo ""
echo "Generating MD5 checksum for ${file}."
echo ""
md5sum "${file}" | tee --append "${sample}_checksums.md5"
echo ""
echo "${file} checksum added to ${sample}_checksums.md5."
echo ""
done
echo "Finished HiSat2 alignments and StringTie analysis for ${sample} FastQs."
echo ""
# Move up to orig. working directory
echo "Moving to original working directory."
echo ""
cd ..
echo "Now in $(pwd)."
echo ""
done
echo "Finished all HiSat2 alignments and StringTie analysis."
echo ""
#### BEGIN MERGING BAMs ####
# Merge all BAMs to singular BAM for use in transcriptome assembly later
## Create list of sorted BAMs for merging
echo ""
echo "Creating list file of sorted BAMs..."
find . -name "*sorted.bam" > sorted_bams.list
echo "List of BAMs created: sorted_bams.list"
echo ""
## Merge sorted BAMs
echo "Merging all BAM files..."
echo ""
${programs_array[samtools_merge]} \
-b sorted_bams.list \
${merged_bam} \
--threads ${threads}
echo ""
echo "Finished creating ${merged_bam}."
#### END MERGING BAMs ####
#### BEGIN INDEXING MERGED BAM ####
## Index merged BAM
echo ""
echo "Indexing ${merged_bam}..."
echo ""
${programs_array[samtools_index]} ${merged_bam}
echo "Finished indexing ${merged_bam}."
echo ""
#### END INDEXING MERGED BAM ####
#### BEGIN MERGE STRINGTIE GTFs ####
# Create singular transcript file, using GTF list file
echo "Merging GTFs..."
echo ""
"${programs_array[stringtie]}" --merge \
"${gtf_list}" \
-p "${threads}" \
-G "${genome_gff}" \
-o "${genome_index_name}.stringtie.gtf"
echo ""
echo "Finished merging GTFs into ${genome_index_name}.stringtie.gtf"
echo ""
#### END MERGE STRINGTIE GTFs ####
# Delete unneccessary index files
echo ""
echo "Removing HiSat2 *.ht2 genome index files..."
echo ""
rm "${genome_index_name}"*.ht2
echo "All genome index files removed."
echo ""
#### BEGIN GFFCOMPARE ####
echo ""
echo "Beginning gffcompare..."
echo ""
# Make ggfcompare output directory and
# change into that directory
mkdir --parents gffcompare && cd "$_"
# Run gffcompare
"${programs_array[gffcompare]}" \
-r "${genome_gff}" \
-o "${genome_index_name}-gffcmp" \
../"${genome_index_name}.stringtie.gtf"
echo ""
echo "Finished gffcompare"
echo ""
# Generate checksums
for file in *
do
echo ""
echo "Generating checksum for ${file}..."
echo ""
md5sum "${file}" | tee --append checksums.md5
echo "Checksum generated."
done
# Move to previous directory
echo "Moving to previous directory..."
echo ""
cd -
echo "Now in $(pwd)."
echo ""
#### END GFFCOMPARE ####
# Generate checksums
echo "Generating checksums for files in $(pwd)."
for file in *
do
echo ""
echo "Generating checksum for ${file}..."
echo ""
md5sum "${file}" | tee --append checksums.md5
echo "Checksum generated."
done
# Remove genome index tarball
echo ""
echo "Removing ${index_tarball}."
rm "${index_tarball}"
echo "${index_tarball} has been deleted."
echo ""
#######################################################################################################
# Capture program options
if [[ "${#programs_array[@]}" -gt 0 ]]; then
echo "Logging program options..."
for program in "${!programs_array[@]}"
do
{
echo "Program options for ${program}: "
echo ""
# Handle samtools help menus
if [[ "${program}" == "samtools_index" ]] \
|| [[ "${program}" == "samtools_sort" ]] \
|| [[ "${program}" == "samtools_view" ]]
then
${programs_array[$program]}
# Handle DIAMOND BLAST menu
elif [[ "${program}" == "diamond" ]]; then
${programs_array[$program]} help
# Handle NCBI BLASTx menu
elif [[ "${program}" == "blastx" ]]; then
${programs_array[$program]} -help
fi
${programs_array[$program]} -h
echo ""
echo ""
echo "----------------------------------------------"
echo ""
echo ""
} &>> program_options.log || true
# If MultiQC is in programs_array, copy the config file to this directory.
if [[ "${program}" == "multiqc" ]]; then
cp --preserve ~/.multiqc_config.yaml multiqc_config.yaml
fi
done
echo "Finished logging programs options."
echo ""
fi
# Document programs in PATH (primarily for program version ID)
echo "Logging system $PATH..."
{
date
echo ""
echo "System PATH for $SLURM_JOB_ID"
echo ""
printf "%0.s-" {1..10}
echo "${PATH}" | tr : \\n
} >> system_path.log
echo "Finished logging system $PATH."
echo ""
echo "Script complete!"RESULTS
Run time was ~5.5hrs:
Output folder:
Due to the number of files and various subdirectories, I won’t be providing links to individual files. Instead, there’s a tree overview of the directory layouts below.
The resulting gffcompare/Panopea-generosa-v1.0-gffcmp.annotated.gtf will be used for downstream lncRNA identification.
Also, the resulting *.ctab files can be used for gene/isoform expression analysis in ballgown.
[4.0K] .
├── [ 70G] 20230216-pver-stringtie-pver_v1.0-sorted-bams-merged.bam
├── [6.6M] 20230216-pver-stringtie-pver_v1.0-sorted-bams-merged.bam.bai
├── [ 14K] 20230426-pgen-HISAT2-stringtie-gffcompare-RNAseq.sh
├── [ 841] checksums.md5
├── [4.0K] ctenidia
│ ├── [ 499] ctenidia_checksums.md5
│ ├── [4.9M] ctenidia.cov_refs.gtf
│ ├── [ 39M] ctenidia.gtf
│ ├── [ 643] ctenidia-hisat2_stats.txt
│ ├── [6.3G] ctenidia.sorted.bam
│ ├── [1.4M] ctenidia.sorted.bam.bai
│ ├── [2.7M] e2t.ctab
│ ├── [ 14M] e_data.ctab
│ ├── [2.3M] i2t.ctab
│ ├── [7.2M] i_data.ctab
│ └── [3.7M] t_data.ctab
├── [4.0K] gffcompare
│ ├── [ 280] checksums.md5
│ ├── [1.5K] Panopea-generosa-v1.0-gffcmp
│ ├── [ 74M] Panopea-generosa-v1.0-gffcmp.annotated.gtf
│ ├── [4.7M] Panopea-generosa-v1.0-gffcmp.loci
│ └── [9.4M] Panopea-generosa-v1.0-gffcmp.tracking
├── [4.0K] gonad
│ ├── [2.7M] e2t.ctab
│ ├── [ 14M] e_data.ctab
│ ├── [ 484] gonad_checksums.md5
│ ├── [2.1M] gonad.cov_refs.gtf
│ ├── [ 26M] gonad.gtf
│ ├── [ 643] gonad-hisat2_stats.txt
│ ├── [6.3G] gonad.sorted.bam
│ ├── [1.4M] gonad.sorted.bam.bai
│ ├── [2.3M] i2t.ctab
│ ├── [7.2M] i_data.ctab
│ └── [3.7M] t_data.ctab
├── [ 519] gtf_list.txt
├── [4.0K] heart
│ ├── [2.7M] e2t.ctab
│ ├── [ 14M] e_data.ctab
│ ├── [ 484] heart_checksums.md5
│ ├── [5.4M] heart.cov_refs.gtf
│ ├── [ 38M] heart.gtf
│ ├── [ 647] heart-hisat2_stats.txt
│ ├── [ 12G] heart.sorted.bam
│ ├── [2.0M] heart.sorted.bam.bai
│ ├── [2.3M] i2t.ctab
│ ├── [7.3M] i_data.ctab
│ └── [3.7M] t_data.ctab
├── [1.5K] input_fastqs_checksums.md5
├── [4.0K] juvenile
│ ├── [2.7M] e2t.ctab
│ ├── [ 15M] e_data.ctab
│ ├── [2.3M] i2t.ctab
│ ├── [7.5M] i_data.ctab
│ ├── [ 499] juvenile_checksums.md5
│ ├── [8.9M] juvenile.cov_refs.gtf
│ ├── [ 69M] juvenile.gtf
│ ├── [ 653] juvenile-hisat2_stats.txt
│ ├── [ 38G] juvenile.sorted.bam
│ ├── [3.9M] juvenile.sorted.bam.bai
│ └── [3.7M] t_data.ctab
├── [4.0K] larvae
│ ├── [2.7M] e2t.ctab
│ ├── [ 15M] e_data.ctab
│ ├── [2.3M] i2t.ctab
│ ├── [7.3M] i_data.ctab
│ ├── [ 489] larvae_checksums.md5
│ ├── [5.4M] larvae.cov_refs.gtf
│ ├── [ 45M] larvae.gtf
│ ├── [ 645] larvae-hisat2_stats.txt
│ ├── [7.9G] larvae.sorted.bam
│ ├── [1.5M] larvae.sorted.bam.bai
│ └── [3.7M] t_data.ctab
├── [2.6M] Panopea-generosa-v1.0-gffcmp.Panopea-generosa-v1.0.stringtie.gtf.refmap
├── [8.7M] Panopea-generosa-v1.0-gffcmp.Panopea-generosa-v1.0.stringtie.gtf.tmap
├── [ 73M] Panopea-generosa-v1.0.stringtie.gtf
├── [ 19K] program_options.log
├── [ 42M] slurm-4571580.out
├── [ 139] sorted_bams.list
└── [1.1K] system_path.log