Automating a Variant Calling Workflow
Last updated on 2024-06-14 | Edit this page
Overview
Questions
- How can I make my workflow more efficient and less error-prone?
Objectives
- Write a shell script with multiple variables.
- Incorporate a
for
loop into a shell script.
What is a shell script?
You wrote a simple shell script in a previous lesson that we used to extract bad reads from our FASTQ files and put them into a new file.
Here is the script you wrote:
That script was only two lines long, but shell scripts can be much more complicated than that and can be used to perform a large number of operations on one or many files. This saves you the effort of having to type each of those commands over for each of your data files and makes your work less error-prone and more reproducible. For example, the variant calling workflow we just carried out had about eight steps where we had to type a command into our terminal. Most of these commands were pretty long. If we wanted to do this for all six of our data files, that would be forty-eight steps. If we had 50 samples (a more realistic number), it would be 400 steps! You can see why we want to automate this.
We have also used for
loops in previous lessons to
iterate one or two commands over multiple input files. In these
for
loops, the filename was defined as a variable in the
for
statement, which enabled you to run the loop on
multiple files. We will be using variable assignments like this in our
new shell scripts.
Here is the for
loop you wrote for unzipping
.zip
files:
And here is the one you wrote for running Trimmomatic on all of our
.fastq
sample files:
BASH
$ for infile in *_1.fastq.gz
> do
> base=$(basename ${infile} _1.fastq.gz)
> trimmomatic PE ${infile} ${base}_2.fastq.gz \
> ${base}_1.trim.fastq.gz ${base}_1un.trim.fastq.gz \
> ${base}_2.trim.fastq.gz ${base}_2un.trim.fastq.gz \
> SLIDINGWINDOW:4:20 MINLEN:25 ILLUMINACLIP:NexteraPE-PE.fa:2:40:15
> done
Notice that in this for
loop, we used two variables,
infile
, which was defined in the for
statement, and base
, which was created from the filename
during each iteration of the loop.
In this lesson, we will use two shell scripts to automate the variant
calling analysis: one for FastQC analysis (including creating our
summary file), and a second for the remaining variant calling. To write
a script to run our FastQC analysis, we will take each of the commands
we entered to run FastQC and process the output files and put them into
a single file with a .sh
extension. The .sh
is
not essential, but serves as a reminder to ourselves and to the computer
that this is a shell script.
Analyzing quality with FastQC
We will use the command touch
to create a new file where
we will write our shell script. We will create this script in a new
directory called scripts/
. Previously, we used
nano
to create and open a new file. The command
touch
allows us to create a new file without opening that
file.
OUTPUT
read_qc.sh
We now have an empty file called read_qc.sh
in our
scripts/
directory. We will now open this file in
nano
and start building our script.
Enter the following pieces of code into your shell script (not into your terminal prompt).
Our first line will ensure that our script will exit if an error
occurs, and is a good idea to include at the beginning of your scripts.
The second line will move us into the untrimmed_fastq/
directory when we run our script.
OUTPUT
set -e
cd ~/dc_workshop/data/untrimmed_fastq/
These next two lines will give us a status message to tell us that we
are currently running FastQC, then will run FastQC on all of the files
in our current directory with a .fastq
extension.
OUTPUT
echo "Running FastQC ..."
fastqc *.fastq*
Our next line will create a new directory to hold our FastQC output
files. Here we are using the -p
option for
mkdir
again. It is a good idea to use this option in your
shell scripts to avoid running into errors if you do not have the
directory structure you think you do.
OUTPUT
mkdir -p ~/dc_workshop/results/fastqc_untrimmed_reads
Our next three lines first give us a status message to tell us we are
saving the results from FastQC, then moves all of the files with a
.zip
or a .html
extension to the directory we
just created for storing our FastQC results.
OUTPUT
echo "Saving FastQC results..."
mv *.zip ~/dc_workshop/results/fastqc_untrimmed_reads/
mv *.html ~/dc_workshop/results/fastqc_untrimmed_reads/
The next line moves us to the results directory where we have stored our output.
OUTPUT
cd ~/dc_workshop/results/fastqc_untrimmed_reads/
The next five lines should look very familiar. First we give
ourselves a status message to tell us that we are unzipping our ZIP
files. Then we run our for loop to unzip all of the .zip
files in this directory.
OUTPUT
echo "Unzipping..."
for filename in *.zip
do
unzip $filename
done
Next we concatenate all of our summary files into a single output file, with a status message to remind ourselves that this is what we are doing.
OUTPUT
echo "Saving summary..."
cat */summary.txt > ~/dc_workshop/docs/fastqc_summaries.txt
Your full shell script should now look like this:
OUTPUT
set -e
cd ~/dc_workshop/data/untrimmed_fastq/
echo "Running FastQC ..."
fastqc *.fastq*
mkdir -p ~/dc_workshop/results/fastqc_untrimmed_reads
echo "Saving FastQC results..."
mv *.zip ~/dc_workshop/results/fastqc_untrimmed_reads/
mv *.html ~/dc_workshop/results/fastqc_untrimmed_reads/
cd ~/dc_workshop/results/fastqc_untrimmed_reads/
echo "Unzipping..."
for filename in *.zip
do
unzip $filename
done
echo "Saving summary..."
cat */summary.txt > ~/dc_workshop/docs/fastqc_summaries.txt
Save your file and exit nano
. We can now run our
script:
OUTPUT
Running FastQC ...
Started analysis of SRR2584866.fastq
Approx 5% complete for SRR2584866.fastq
Approx 10% complete for SRR2584866.fastq
Approx 15% complete for SRR2584866.fastq
Approx 20% complete for SRR2584866.fastq
Approx 25% complete for SRR2584866.fastq
.
.
.
For each of your sample files, FastQC will ask if you want to replace
the existing version with a new version. This is because we have already
run FastQC on this samples files and generated all of the outputs. We
are now doing this again using our scripts. Go ahead and select
A
each time this message appears. It will appear once per
sample file (six times total).
OUTPUT
replace SRR2584866_fastqc/Icons/fastqc_icon.png? [y]es, [n]o, [A]ll, [N]one, [r]ename:
Automating the rest of our variant calling workflow
We can extend these principles to the entire variant calling
workflow. To do this, we will take all of the individual commands that
we wrote before, put them into a single file, add variables so that the
script knows to iterate through our input files and write to the
appropriate output files. This is very similar to what we did with our
read_qc.sh
script, but will be a bit more complex.
Download the script from here. Download to
~/dc_workshop/scripts
.
Our variant calling workflow has the following steps:
- Index the reference genome for use by bwa and samtools.
- Align reads to reference genome.
- Convert the format of the alignment to sorted BAM, with some intermediate steps.
- Calculate the read coverage of positions in the genome.
- Detect the single nucleotide variants (SNVs).
- Filter and report the SNVs in VCF (variant calling format).
Let’s go through this script together:
The script should look like this:
OUTPUT
set -e
cd ~/dc_workshop/results
genome=~/dc_workshop/data/ref_genome/ecoli_rel606.fasta
bwa index $genome
mkdir -p sam bam bcf vcf
for fq1 in ~/dc_workshop/data/trimmed_fastq_small/*_1.trim.sub.fastq
do
echo "working with file $fq1"
base=$(basename $fq1 _1.trim.sub.fastq)
echo "base name is $base"
fq1=~/dc_workshop/data/trimmed_fastq_small/${base}_1.trim.sub.fastq
fq2=~/dc_workshop/data/trimmed_fastq_small/${base}_2.trim.sub.fastq
sam=~/dc_workshop/results/sam/${base}.aligned.sam
bam=~/dc_workshop/results/bam/${base}.aligned.bam
sorted_bam=~/dc_workshop/results/bam/${base}.aligned.sorted.bam
raw_bcf=~/dc_workshop/results/bcf/${base}_raw.bcf
variants=~/dc_workshop/results/vcf/${base}_variants.vcf
final_variants=~/dc_workshop/results/vcf/${base}_final_variants.vcf
bwa mem $genome $fq1 $fq2 > $sam
samtools view -S -b $sam > $bam
samtools sort -o $sorted_bam $bam
samtools index $sorted_bam
bcftools mpileup -O b -o $raw_bcf -f $genome $sorted_bam
bcftools call --ploidy 1 -m -v -o $variants $raw_bcf
vcfutils.pl varFilter $variants > $final_variants
done
Now, we will go through each line in the script before running it.
First, notice that we change our working directory so that we can create new results subdirectories in the right location.
OUTPUT
cd ~/dc_workshop/results
Next we tell our script where to find the reference genome by
assigning the genome
variable to the path to our reference
genome:
OUTPUT
genome=~/dc_workshop/data/ref_genome/ecoli_rel606.fasta
Next we index our reference genome for BWA:
OUTPUT
bwa index $genome
And create the directory structure to store our results in:
OUTPUT
mkdir -p sam bam bcf vcf
Then, we use a loop to run the variant calling workflow on each of
our FASTQ files. The full list of commands within the loop will be
executed once for each of the FASTQ files in the
data/trimmed_fastq_small/
directory. We will include a few
echo
statements to give us status updates on our
progress.
The first thing we do is assign the name of the FASTQ file we are
currently working with to a variable called fq1
and tell
the script to echo
the filename back to us so we can check
which file we are on.
BASH
for fq1 in ~/dc_workshop/data/trimmed_fastq_small/*_1.trim.sub.fastq
do
echo "working with file $fq1"
We then extract the base name of the file (excluding the path and
.fastq
extension) and assign it to a new variable called
base
.
We can use the base
variable to access both the
base_1.fastq
and base_2.fastq
input files, and
create variables to store the names of our output files. This makes the
script easier to read because we do not need to type out the full name
of each of the files: instead, we use the base
variable,
but add a different extension (e.g. .sam
,
.bam
) for each file produced by our workflow.
BASH
#input fastq files
fq1=~/dc_workshop/data/trimmed_fastq_small/${base}_1.trim.sub.fastq
fq2=~/dc_workshop/data/trimmed_fastq_small/${base}_2.trim.sub.fastq
# output files
sam=~/dc_workshop/results/sam/${base}.aligned.sam
bam=~/dc_workshop/results/bam/${base}.aligned.bam
sorted_bam=~/dc_workshop/results/bam/${base}.aligned.sorted.bam
raw_bcf=~/dc_workshop/results/bcf/${base}_raw.bcf
variants=~/dc_workshop/results/bcf/${base}_variants.vcf
final_variants=~/dc_workshop/results/vcf/${base}_final_variants.vcf
And finally, the actual workflow steps:
- align the reads to the reference genome and output a
.sam
file:
OUTPUT
bwa mem $genome $fq1 $fq2 > $sam
- convert the SAM file to BAM format:
OUTPUT
samtools view -S -b $sam > $bam
- sort the BAM file:
OUTPUT
samtools sort -o $sorted_bam $bam
- index the BAM file for display purposes:
OUTPUT
samtools index $sorted_bam
- calculate the read coverage of positions in the genome:
OUTPUT
bcftools mpileup -O b -o $raw_bcf -f $genome $sorted_bam
- call SNVs with bcftools:
OUTPUT
bcftools call --ploidy 1 -m -v -o $variants $raw_bcf
- filter and report the SNVs in variant calling format (VCF):
OUTPUT
vcfutils.pl varFilter $variants > $final_variants
Exercise
It is a good idea to add comments to your code so that you (or a
collaborator) can make sense of what you did later. Look through your
existing script. Discuss with a neighbor where you should add comments.
Add comments (anything following a #
character will be
interpreted as a comment, bash will not try to run these comments as
code).
Now we can run our script:
Exercise
The samples we just performed variant calling on are part of the long-term evolution experiment introduced at the beginning of our variant calling workflow. From the metadata table, we know that SRR2589044 was from generation 5000, SRR2584863 was from generation 15000, and SRR2584866 was from generation 50000. How did the number of mutations per sample change over time? Examine the metadata table. What is one reason the number of mutations may have changed the way they did?
Hint: You can find a copy of the output files for the subsampled
trimmed FASTQ file variant calling in the
~/.solutions/wrangling-solutions/variant_calling_auto/
directory.
BASH
$ for infile in ~/dc_workshop/results/vcf/*_final_variants.vcf
> do
> echo ${infile}
> grep -v "#" ${infile} | wc -l
> done
For SRR2589044 from generation 5000 there were 10 mutations, for SRR2584863 from generation 15000 there were 25 mutations, and SRR2584866 from generation 50000 there were 766 mutations. In the last generation, a hypermutable phenotype had evolved, causing this strain to have more mutations.
Bonus exercise
If you have time after completing the previous exercise, use
run_variant_calling.sh
to run the variant calling pipeline
on the full-sized trimmed FASTQ files. You should have a copy of these
already in ~/dc_workshop/data/trimmed_fastq
, but if you do
not, there is a copy in
~/.solutions/wrangling-solutions/trimmed_fastq
. Does the
number of variants change per sample?