Versions Compared

Key

  • This line was added.
  • This line was removed.
  • Formatting was changed.
Comment: Migrated to Confluence 5.3

Samtools

Setup output directory.

Code Block

mkdir samtools_bowtie

If you do not have an alignment file in the SAM format you may want to start with Introduction to mapping.

...

SAMtools is a suite of commands for dealing with databases of mapped reads. You'll be using it quite a bit throughout the course. It includes programs for performing variant calling (mpileup-bcftools).

Table of Contents

Calling variants in reads mapped by bowtie

Right now, we'll be using it to call variants (find mutations) in the re-sequenced E. coli genome from the Mapping tutorial. You will need the output SAM files from that tutorial to continue here.

Warning

If you do not have the output from the Mapping tutorial, run these commands to copy over the output that would have been produced. Then, you can immediately start this tutorial!

Code Block

cds
mkdir intro_to_mapping
cd intro_to_mapping
cp -r $BI/ngs_course/intro_to_mapping/bowtie .
cp -r $BI/ngs_course/intro_to_mapping/bwa . 
cp -r $BI/ngs_course/intro_to_mapping/bowtie2 .

We assume that you are still working in the main directory called intro_to_mapping data that you created on $SCRATCH.

Load SAMtools

Load the SAMtools module (if not already loaded).

Expand
I want to copy-paste...
I want to copy-paste...
Code Block

module load samtools

Can you figure out what version of samtools is loaded on TACC and where it is installed?

Expand
No, give me the commands...
No, give me the commands...

This should work:

Code Block

samtools
which samtools

Prepare your directories

Create a new output directory called samtools_bowtie or whatever makes sense to you.

Let's copy over just the read alignment file in the SAM format and the reference genome in FASTA format to this new directory, so that we don't have so many files cluttering our space.

Expand
Commands for doing this if you've been following the tutorials...
Commands for doing this if you've been following the tutorials...
Code Block

mkdir samtools_bowtie
cp bowtie/SRR030257.sam samtools_bowtie
/

cp bowtie/
REL606
NC_012967.
5
1.fasta samtools_bowtie
/

Index the FASTA reference file

First, you need to index the reference file. (This isn't indexing it for read mapping. It's indexing it so that SAMtools can quickly jump to a certain base in the reference.)

Then run this command to index the reference file.

Code Block
samtools faidx samtools_bowtie/NC_012967.1.fasta

Take a look at the new *.fai file that was created by this command. Any idea what some of the numbers mean?

Expand
For example, by using this command...
For example, by using this command...
Code Block

less samtools_bowtie/
REL606
NC_012967.
5
1.fasta.fai

Hint: Type q to exit less.

Convert mapped reads from SAM to BAM, sort, and index

SAM is a text file, so it is slow to access information about how any given read was mapped. SAMtools and many of the commands that we will run later work on BAM files (essentially GZIP compressed binary forms of the text SAM files). These can be loaded much more quickly. Typically, they also need to be sorted, so that when the program wants to look at all reads overlapping position 4,129,888, it can easily find them all at once without having to search through the entire BAM file.

Convert from SAM to BAM format.

Code Block
samtools view -bSb -S -o samtools_bowtie/REL606SRR030257.5.bam samtools_bowtie/REL606.5SRR030257.sam |borderStyle=solid}

Sort and index the BAM file.

Code Block
samtools sort samtools_bowtie/REL606.5.bam samtools_bowtie/sorted_REL606.5

Output VCF file.

Code Block
SRR030257.bam samtools_bowtie/SRR030257.sorted
samtools index samtools_bowtie/SRR030257.sorted.bam

This is a really common sequence of commands, so you might want to add it to your personal cheat sheet.

  • What new files were created by these commands?
    Expand
    Check that
    Check that
    Code Block
    titleList the contents of the output directory
    
    ls samtools_bowtie
    
    Code Block
    titleExpected output
    
    NC_012967.1.fasta      SRR030257.sorted.bam.bai
    NC_012967.1.fasta.fai  SRR030257.sam
    SRR030257.bam          SRR030257.sorted.bam
    
  • Why didn't we name the output SRR030257.sorted.bam in the samtools sort command?
    Expand
    Answer...
    Answer...

    Samtools appends an extra .bam to whatever we put here, so it would have created SRR030257.sorted.bam.bam, and we would have had to make a joke about the Flintstones.

  • Can you guess what a *.bai file is?
    Expand
    Answer...
    Answer...

    Sure enough, it's the index file for the BAM file.

Hint: You might be tempted to gzip BAM files when copying them from one computer to another. Don't bother! They are already internally compressed, so you won't be able to shrink the file. On the other hand, compressing SAM files will save a fair bit of space.

Call genome variants

Now we use the mpileup command from samtools to compile information about the bases mapped to each reference position.

Output BCF file. This is a binary form of the text Variant Call Format (VCF).

Code Block
titleThis is *one* command. Put it all on one line.
samtools mpileup -ufu -f samtools_bowtie/REL606NC_012967.51.fasta samtools_bowtie/SRR030257.sorted_REL606.5.bam \|.bam > samtools_bowtie/SRR030257.bcf

What are all the options doing?

Convert BCF to human-readable VCF:

Code Block
titleThis is *one* command. Put it all on one line.

bcftools view -vcgv -c - \g samtools_bowtie/SRR030257.bcf > samtools_bowtie/output.vcf 

Output

Exercise 1

...

SRR030257.vcf

What are these options doing?

Take a look at the samtools_bowtie/SRR030257.vcf file using less. It has a nice header explaining what the columns mean. Below this are the rows of data describing potential genetic variants.

Optional Exercises

Calling variants in reads mapped by BWA or Bowtie2

Anchor
Calling variants in reads mapped by BWA or Bowtie2
Calling variants in reads mapped by BWA or Bowtie2

Follow the same directions to call variants in the BWA or Bowtie2 mapped reads.

Just be sure you don't write over your old files. Maybe create new directories like samtools_bwa and samtools_bowtie2 for the output in each case.

You could also try running all of the commands from inside of the samtools_bwa directory, just for a change of pace.

Filtering VCF files with grep

VCF format has alternative Allele Frequency tags denoted by AF1. Try the following command to see what values we have in our files.

Code Block

grep cat input.vcf | grep AF1
AF1 samtools_bowtie/SRR030257.vcf

Optional: For the data we are dealing with, predictions with an allele frequency not equal to 1 are not really applicable. (The reference genome is haploid. There aren't any heterozygotes.) How can we remove these lines from the file and continue on?

Expand
Hint...
Hint...

What does the -v flag do in grep?

Code Block
grep -v *something*

Solutions

Output

Determining Differences Between Aligners.

...

Expand
Solution...
Solution...
Code Block

mkdir output cp samtools_bowtie/output.vcf output/bowtie.vcf cp samtools_bwa/output.vcf output/bwa.vcf cd output
cat input.vcf | grep AF1=1 > output.vcf

Is not practical, since we will lose vital VCF formatting and may not be able to use this file in the future.

Code Block

cat input.vcf | grep -v AF1=0 > output.vcf

Will preserve all lines that don't have a AF1=0 value and is one way of doing this.

Code Block

sed -i '/AF1=0/ d' input.vcf

Is a way of doing it in-line and not requiring you to make another file. (But it writes over your existing file!)

Comparing the results of different mappers using bedtools

You will need the output from #Calling variants in reads mapped by BWA or Bowtie2 to complete this exercise.

Often you want to compare the results of variant calling on different samples or using different pipelines. Bedtools is a suite of utility programs that work on a variety of file formats, one of which is conveniently VCF format. Using intersectBed and subtractBed . It provides many ways of slicing, dicing, and comparing the information in VCF files. For example, we can use it to find out what predictions are the same and which are different from the variant calling on reads mapped with different programs.

Set up a new output directory and copy the respective VCF files to it, renaming them so that we know where they came from:

Code Block

mkdir comparison
cp samtools_bowtie/SRR030257.vcf comparison/bowtie.vcf
cp samtools_bwa/SRR030257.vcf comparison/bwa.vcf
cp samtools_bowtie2/SRR030257.vcf comparison/bowtie2.vcf
cd comparison

Use the subcommands bedtools intersect and bedtools subtract we can find equal and different predictions between mappers. Try to figure out how to to do this on your own first. Hint: Remember that adding > output.vcf to the end of a command will pipe the output that is to the terminal into a file, so that you can save it.

Expand
I'm stuck? Show me the commands...
I'm stuck? Show me the commands...

Load Bedtools.

Code Block

module load bedtools

Finding

...

common mutations.

Code Block

bedtools 
intersectBed
intersect -a bowtie.vcf -b bwa.vcf > 
intersect
common_bowtie_bwa.vcf

Finding mutations that are unique

...

for each mapper.

Code Block

bedtools 
subtractBed
subtract -a bowtie.vcf -b 
intersect
common_bowtie_bwa.vcf > unique_bowtie.vcf
bedtools 
subtractBed
subtract -a bwa.vcf -b 
intersect
common_bowtie_bwa.vcf > unique_bwa.vcf

Further Optional Exercises

  • Which mapper finds more variants?
  • Can you figure out how to filter the VCF files on various criteria, like coverage, quality, ... ?
  • How many high quality mutations are there in these E. coli samples relative to the reference genome?

From here...

*Look at how the reads supporting these variants were aligned to the reference genome in the Integrative Genomics Viewer (IGV) tutorial.
*Look into more sophisticated Variant+calling+with+GATK.