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6,547 bytes added , 14:37, 13 November 2014

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'''Note:''' the latest version of this practical is available at: [[SeqShop: Variant Calling and Filtering for SNPs Practical]]

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* The ones here is the original one from the June workshop (updated to be run from elsewhere)

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==Introduction==

See the [[Media:SeqShop - GotCloud snpcall.pdf|introductory slides]] for an intro to this tutorial.

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** How to examine the variants at particular genomic positions

** How to evaluate the quality of SNP calls

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== Setup in person at the SeqShop Workshop ==

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''This section is specifically for the SeqShop Workshop computers.''

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''If you are not running during the SeqShop Workshop, please skip this section.''

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== Setup your run environment==

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=== Setup your run environment===

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This is the same setup you did for the previous tutorial, but you need to redo it each time you log in.

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This ~~is the same setup you did for the previous tutorial, but you need to redo it each time you log in. It~~ will setup some environment variables to point you to:

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This will setup some environment variables to point you to

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* GotCloud program

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* [[GotCloud]] program

* Tutorial input files

* Setup an output directory

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* You won't see any output after running <code>source</code>

** It silently sets up your environment

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** If you want to view the detail of the ~~set up~~, type

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** If you want to view the detail of the setup, type

less /home/mktrost/seqshop/setup.txt

and press 'q' to finish.

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View setup.txt

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</div>

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</div>

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</div>

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== Setup when running on your own outside of the SeqShop Workshop ==

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''This section is specifically for running on your own outside of the SeqShop Workshop.''

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''If you are running during the SeqShop Workshop, please skip this section.''

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This tutorial builds on the alignment tutorial, if you have not already, please first run that tutorial: [[SeqShop:_Sequence_Mapping_and_Assembly_Practical, June 2014|Alignment Tutorial]]

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== Examining GotCloud SnpCall Input files ==

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Per sample BAM files contain sequence reads that are mapped to positions in the genome.

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For a reminder on how to look at/read BAM files, see: [[SeqShop:_Sequence_Mapping_and_Assembly_Practical#BAM_Files|SeqShop Aligment: BAM Files]]

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For a reminder on how to look at/read BAM files, see: [[SeqShop:_Sequence_Mapping_and_Assembly_Practical, June 2014#BAM_Files|SeqShop Aligment: BAM Files]]

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For this tutorial, we will use the 4 BAMs produced in the [[SeqShop: Sequence Mapping and Assembly Practical]] as well as with 58 BAMs that were pre-aligned to that 1MB region of chromosome 22.

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For this tutorial, we will use the 4 BAMs produced in the [[SeqShop: Sequence Mapping and Assembly Practical, June 2014]] as well as with 58 BAMs that were pre-aligned to that 1MB region of chromosome 22.

=== Reference Files ===

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We looked at them yesterday, but you can take another look at the chromosome 22 reference files included for this tutorial:

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ls ${~~REF~~}

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ls ${SS}/ref22

<ul>

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<li>View Screenshot</li>

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[[File:RefDir.png|~~500px~~]]

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[[File:RefDir.png|700px]]

</div>

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The alignment pipeline only processed 4 samples, but for snpcall, we want to run on 62 samples.

* The other 58 samples were already aligned:

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ls ${IN}/bams

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ls ${SS}/bams

Look at the BAM index for those BAMs:

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less ${IN}/bams/bam.index

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less ${SS}/bams/bam.index

Remember, use <code>'q'</code> to exit out of <code>less</code>

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;Do you notice a difference between this index and yours?

<ul>

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<li>Answer:</li>

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<li>It doesn't have a full path to the BAM file, while your index has /home/...</li>

[[File:Bamindex1.png|300px]]

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<li>That's ok, <code>gotcloud.conf</code> ~~contains~~ the path to ~~those~~ BAMs</li>

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<li>That's ok, we will use the <code>--base_prefix ${SS}</code> command-line option to prefix the BAM paths</li>

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~~[[File~~:~~BamindexConf~~.~~png|300px]]~~

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<li>Alternatively, we could have set BAM_INDEX in <code>gotcloud.conf</code> to the path to the BAMs

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<pre>BAM_INDEX = /home/username/seqshop/example</pre> </li>

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<ul>

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<li>NOTE: the conf file can't interpret ${SS} environment variables or '~', so you would have to specify the full path</li>

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<li>We just used the command-line option for this tutorial since this path will vary by user.</li>

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</ul>

</div>

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We need to add these BAMs to our index

* Append the bam.index from the pre-aligned BAMs to the one you generated from the alignment pipeline

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cat ${IN}/bams/bam.index >> ${OUT}/bam.index

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** '''Be sure to do this command just once'''

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cat ${SS}/bams/bam.index >> ${OUT}/bam.index

* ">>" will append to the file that follows it

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** Check that your BAM index is the correct size

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**:<pre>wc -l ${OUT}/bam.index</pre>

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*** <code>wc -l</code> counts the number of lines in the file

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*** Should be 62

Verify your BAM index contains the additional BAMs

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We will use the same configuration file as we used yesterday in GotCloud Align.

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See [[SeqShop:~~_Sequence_Mapping_and_Assembly_Practical~~#GotCloud Configuration File|SeqShop: Alignment: GotCloud Configuration File]] for more details

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See [[SeqShop:_Sequence Mapping and Assembly Practical, June 2014#GotCloud Configuration File|SeqShop: Alignment: GotCloud Configuration File]] for more details

* Note we want to limit snpcall to just chr22 so the configuration already has <code>CHRS = 22</code> (default was 1-22 & X).

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Now that we have all of our input files, we need just a simple command to run:

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${GC}/gotcloud snpcall --conf ${IN}/gotcloud.conf --numjobs 4 --region 22:36000000-37000000

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${GC}/gotcloud snpcall --conf ${SS}/gotcloud.conf --numjobs 4 --region 22:36000000-37000000 --base_prefix ${SS} --outdir ${OUT}

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* <code>${GC}/gotcloud</code> runs GotCloud

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* <code>align</code> tells GotCloud you want to run the alignment pipeline.

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* <code>--conf</code> tells GotCloud the name of the configuration file to use.

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** The configuration for this test was downloaded with the seqshop input files.

* --numjobs tells GotCloud how many jobs to run in parallel

** Depends on your system

* --region 22:36000000-37000000

** The sample files are just a small region of chromosome 22, so to save time, we tell GotCloud to ignore the other regions

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* <code>--base_prefix</code> tells GotCloud the prefix to append to relative paths.

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** The Configuration file cannot read environment variables, so we need to tell GotCloud the path to the input files, ${SS}

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** Alternatively, gotcloud.conf could be updated to specify the full paths

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* <code>--out_dir</code> tells GotCloud where to write the output.

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** This could be specified in gotcloud.conf, but to allow you to use the ${OUT} to change the output location, it is specified on the command-line

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If you cancelled GotCloud part way through, just rerun your GotCloud command and it will pick up where it left off.

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If you want to understand more detailed step of GotCloud SNP calling, here is a schematic picture with a little bit more details

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[[File:Gotcloudoverview.png|600px]]

== Examining GotCloud SnpCall Output ==

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View ~~Annotated~~ Screenshot

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View Screenshot

[[File:filterSum.png]]

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</div>

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'''To understand how to interpret the filtering summary statistics, please refer to [[Understanding vcf-summary output]]'''

=== Filtered VCF ===

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** Use down arrow to move down one line

* Scroll right until you should see per sample genotype information

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Remember, use <code>'q'</code> to exit out of <code>less</code>

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q

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* Scroll down: they all look like they <code>PASS</code>

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Remember, use 'q' to exit out of less

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q

Let's check if they are all PASS.

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=== Genotype Refinement Input ===

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The GotCloud genotype refinement pipeline takes the VCF file of PASS'ing SNPs from snpcall ~~as input~~.

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The GotCloud genotype refinement pipeline takes as input ${OUT}/split/chr22/chr22.filtered.PASS.vcf.gz (the VCF file of PASS'ing SNPs from snpcall).

The bam index and the configuration file we used for GotCloud snpcall will tell GotCloud genotype refinement everything it needs to know, so no new input files need to be prepared.

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Note: the configuration file overrides the THUNDER command to make it go faster than the default settings so the tutorial will run faster:

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[[File:thunderConf.png|600px]]

=== Running GotCloud Genotype Refinement ===

Since everything is setup, just run the following command (very similar to snpcall).

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${GC}/gotcloud ldrefine --conf ${IN}/gotcloud.conf --numjobs 2 --region 22:36000000-37000000

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${GC}/gotcloud ldrefine --conf ${SS}/gotcloud.conf --numjobs 2 --region 22:36000000-37000000 --base_prefix ${SS} --outdir ${OUT}

* Beagle will take about 2-3 minutes to complete

* Thunder will automatically run and will take another 3-4 minutes

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When completed, it should look like this:

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[[File:GcldrefineOut.png]]

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</div>

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</div>

=== Genotype Refinement Output ===

; What's new in the output directory?

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<ul>

<li>Answer</li>

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:<pre>ls ${OUT}</pre>

<ul>

<li><code>beagle</code> directory : Beagle output</li>

<li><code>thunder</code> directory : Thunder output</li>

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<li><code>umake.beagle.~~conf~~</code> : ~~Configuration values~~ used ~~for GotCloud beagle</li>~~

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<li><code>umake.beagle.*</code> : Contain the configuration & steps used in GotCloud beagle</li>

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~~<li><code>umake.beagle.Makefile</code> : GNU makefile for commands run as part of GotCloud beagle</li>~~

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~~<li><code>umake.beagle.Makefile.log</code> : Log of the~~ GotCloud beagle ~~run~~</li>

<li><code>umake.thunder.*</code> files : Contain the configuration & steps used in GotCloud thunder</li>

</ul>

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</ul>

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Let's take a look at that interesting location we found in the [[SeqShop:_Sequence_Mapping_and_Assembly_Practical#Accessing_BAMs_by_Position|alignment tutorial]] : chromosome 22, positions 36907000-36907100

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Let's take a look at that interesting location we found in the [[SeqShop:_Sequence_Mapping_and_Assembly_Practical, June 2014#Accessing_BAMs_by_Position|alignment tutorial]] : chromosome 22, positions 36907000-36907100

Use tabix to extract that from the VCFs:

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Remember, type 'q' to quit less.

q

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=== Did I find interesting variants? ===

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The region we selected contains ''APOL1'' gene, which is known to play an important role in kidney diseases such as nephrotic syndrome. One of the non-synonymous risk allele, <code>rs73885139</code> located at position <code>22:36661906</code> increases the risk of nephrotic syndrome by >2-folds. Let's see if we found the interesting variant by looking at the VCF file by position.

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${GC}/bin/tabix ${OUT}/vcfs/chr22/chr22.filtered.vcf.gz 22:36661906 | head -1

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Did you see a variant at the position?

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${GC}/bin/tabix ${OUT}/vcfs/chr22/chr22.filtered.vcf.gz 22:36661906 | head -1

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22 36661906 . A G 18 PASS DP=409;MQ=59;NS=62;AN=124;AC=2;AF=0.013827;AB=0.4065;AZ=-0.5287;

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FIC=-0.0092;SLRT=-0.0075;HWEAF=0.0138;HWDAF=0.0276,0.0000;LBS=36,36,0,0,1,1,0,0;

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OBS=145,191,0,0,3,2,0,0;STR=-0.040;STZ=-0.740;CBR=0.008;CBZ=0.144;IOR=0.000;IOZ=-1.370;

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AOI=-5.614;AOZ=-4.243;LQR=0.178;MQ0=0.000;MQ10=0.000;MQ20=0.000;MQ30=0.000;SVM=1.51214

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GT:DP:GQ:PL 0/0:4:28:0,12,65

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Let's check the sequence data to confirm that the variant really exists

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${GC}/bin/samtools tview ${SS}/bams/HG01242.recal.bam ${SS}/ref22/human.g1k.v37.chr22.fa

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* Type 'g' to go to a specific position

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* Type 22:36661906 to move to the position

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* Press arrows to move between positions

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* Press 'b' if you want to color by base quality

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* Press '?' for more help

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View Screenshot

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[[File:Samtoolstviewsnp.png|600px]]

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</div>

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</div>

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=== Improvements ===

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Let's get some information on the BEAGLE VCF:

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perl ${SS}/ext/bed-diff.pl --vcf1 ${SS}/ref22/1kg.omni.chr22.36Mb.vcf.gz --vcf2 ${OUT}/beagle/chr22/chr22.filtered.PASS.beagled.ALL.vcf.gz --gcRoot ${GC} --out ${OUT}/bedDiff.beagle

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Look at the results:

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more ${OUT}/bedDiff.beagle.summary

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*Results

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OVERALL: 43601 44293 0.9844

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NREF-EITHER: 19667 20359 0.9660

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NMAJ-EITHER: 14585 15277 0.9547

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HOMREF: 23934 100 1 0.9958

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HET: 329 11959 175 0.9596

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HOMALT: 4 83 7708 0.9888

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HOMMAJ: 29016 126 2 0.9956

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HET: 364 11959 140 0.9596

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HOMMIN: 3 57 2626 0.9777

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</div>

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</div>

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Now, let's see if it improved after running Thunder VCF:

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perl ${SS}/ext/bed-diff.pl --vcf1 ${SS}/ref22/1kg.omni.chr22.36Mb.vcf.gz --vcf2 ${OUT}/thunder/chr22/ALL/thunder/chr22.filtered.PASS.beagled.ALL.thunder.vcf.gz --gcRoot ${GC} --out ${OUT}/bedDiff.thunder

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Look at the results:

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more ${OUT}/bedDiff.thunder.summary

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*Results

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OVERALL: 43685 44293 0.9863

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NREF-EITHER: 19758 20366 0.9701

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NMAJ-EITHER: 14688 15296 0.9603

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HOMREF: 23927 106 2 0.9955

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HET: 286 12057 120 0.9674

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HOMALT: 6 88 7701 0.9879

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HOMMAJ: 28997 144 3 0.9950

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HET: 286 12057 120 0.9674

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HOMMIN: 5 50 2631 0.9795

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</div>

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</div>

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There is an improvement.

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== What is GotCloud snpcall doing? ==

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To run GotCloud, you really just needed a single command.

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Well, that one command runs many steps. Here is a diagram of all the steps.

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[[File:SnpcallPipeline.jpg|1200px]]

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Aren't you glad you didn't have to configure & run each one yourself?

Mktrost

Administrators

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Changes

SeqShop: Variant Calling and Filtering for SNPs Practical, June 2014 (view source)

Revision as of 14:37, 13 November 2014

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