How to know synonymous and non-synonymous SNPs from transcriptome sequencing
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6.7 years ago
smallfish ▴ 10

I obtained a SNP list (VCF format) from a sample's transcriptome (assembled by Trinity). ORFs were identified using TransDecoder. How I classify these SNPs? How to calculate ka/ks?

RNA-Seq SNP • 6.6k views
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6.7 years ago

You can annotate VCFs using SnpEFf, but you will first have to build the database: http://snpeff.sourceforge.net/SnpEff_manual.html#databases

This will (in the end) make a new VCF with non-synonymous SNPs and their severity (introduces STOP codons, changes AA, changes nothing etc.). SNPEff's report will also report the total number of Ka and Ks, if I remember correctly.

If you want to calculate Ka/Ks on a more detailed scale, use this script: https://github.com/MerrimanLab/selectionTools/blob/master/extrascripts/kaks.py which takes SNPEff's output and gives out a Ka/Ks table per gene

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Thanks very much. It's a good idea.

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Dear Philipp, I am dealing with an analysis on a vcf that I gave as input to snpeff (from a population of more than 400 closely related individuals (among varieties and species - also polyploids)). Then I've used this script you shared to calculate Ka/Ks table per gene. This analysis is resulting in a very broad ka/ks distribution which goes from 0 to hundreds. Any comment or tip on this?

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Most papers I've seen filter out 'extreme' Ks values, here's a totally random paper that removes Ks > 3 https://onlinelibrary.wiley.com/doi/full/10.1111/mec.15275 Your niche must have something similar to cite

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Thanks for your answer. It looks weird to me as the kaks.txt file after running

grep '^#\|missense_variant\|synonymous_variant' annotated_vcf.vcf > mis_syn.txt 
python kaks.py mis_syn.txt > kaks.txt

gives me these quantiles for ks column (similar quantiles for ka). Is that maybe a too heterogeneous panel ? I am working with cereals.

0%   25%   50%   75%  100% 
0     6    42   178   13976 

while for ka/ks+1 i get

  0%          25%          50%          75%         100% 
   0          0.17        1.07          5.28        2192 
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I have some off-the-chart dN/dS values for few genes (>20) when using your script on VCF obtained from a 20K plasmodium genomes (pf7K).

Gene Coordinate ka ks ka_div_ks_plus1
PF3D7_0930300 Pf3D7_09_v3:1201305-1207576 1241737 175042 7.09389692818
PF3D7_1133400 Pf3D7_11_v3:1292966-1296696 1252020 46689 26.8155922039
PF3D7_0424100 Pf3D7_04_v3:1082005-1084464 63592 3690 17.2289352479
PF3D7_0323400 Pf3D7_03_v3:980706-983966 63452 2016 31.458601884
PF3D7_0731500 Pf3D7_07_v3:1357251-1363653 366973 5520 66.4685745336
PF3D7_0423800 Pf3D7_04_v3:1075910-1077829 12070 2031 5.93996062992
PF3D7_0507500 Pf3D7_05_v3:307090-310120 57532 8246 6.97611252577

These genes should have low polymorphism as they are vaccine candidates as stated here. I am not sure if I did something wrong?

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6.0 years ago
jfo • 0

can we use SNPMeta for this? https://www.ncbi.nlm.nih.gov/pubmed/24237904

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