Association can be performed using two approaches.

1. Based on testing differences in allele frequencies between cases and controls, using genotype likelihoods
2. Based on a generalized linear framework which also allows for quantitative traits and binary and for including additional covariates, using genotype posteriors.

We recommend that users don't perform association analysis on all sites, but limit the analysis to informative sites, and in the case of alignement data (BAM), we advise that users filter away the low mapping quality reads and the low qscore bases.

The filtering of the alignment data is described in Input, and filtering based on frequencies/polymorphic sites are described here.

-minQ 20 -minMapQ 30 -SNP_pval 1e-6 #Use polymorphic sites with a p-value of 10^-6
-minQ 20 -minMapQ 30 -minMaf 0.05 #Use sites with a MAF >0.05

Brief Overview

./angsd -doAsso
analysisAsso.cpp:
	-doAsso	0
	1: Frequency Test (Known Major and Minor)
	2: Score Test
	3: Frequency Test (Unknown Minor)	
  Frequency Test Options:
	-yBin		(null)	(File containing disease status)	

  Score Test Options:
	-yBin		(null)	(File containing disease status)
	-yQuant		(null)	(File containing phenotypes)
	-minHigh	10	(Require atleast minHigh number of high credible genotypes)
	-minCount	10	(Require this number of minor alleles, estimated from MAF)
	-cov		(null)	(File containing additional covariates)
	-model	1
	1: Additive/Log-Additive (Default)
	2: Dominant
	3: Recessive

Case control association using allele frequencies

To test for differences in the allele frequencies, genotype likelihood needs to be provided or estimated. The test is an implimentation of the likelihoods ratio test for differences between cases and controls described in details in Kim2011.

-doAsso [int]

1: The test is performed assuming the minor allele is known.

-yBin [Filename]

A file containing the case control status. 0 being the controls, 1 being the cases and -999 being missing phenotypes. The file should contain a single phenotype entry per line.

1
0
0
0
1
1
1
1
0
-999
1
0
0
0
0
1

Example

create a large number of individuals by recycling the example files (500 individuals) and simulate some phentypes (case/control) using R

for i in `seq 1 50`;do cat bam.filelist>>large.filelist;done
Rscript -e "write.table(cbind(rbinom(500,1,0.5)),'pheno.ybin',row=F,col=F)"

./angsd -yBin pheno.ybin -doAsso 1 -GL 1 -out out -doMajorMinor 1 -doMaf 1 -SNP_pval 1e-6 -bam large.filelist -r 1: -P 5

Note that because you are reading 500 bam files it takes a little while

Chromosome	Position	Major	Minor	Frequency	LRT
1	14000003	G	A	0.057070	0.016684
1	14000013	G	A	0.067886	0.029014
1	14000019	G	T	0.052904	0.569061
1	14000023	C	A	0.073336	0.184060
1	14000053	T	C	0.038903	0.604695
1	14000170	C	T	0.050756	0.481033
1	14000176	G	A	0.053157	0.424910
1	14000200	C	A	0.085332	0.485030
1	14000202	G	A	0.257132	0.025047

The LRT is the likelihood ration statistics which is chi square distributed with one degree of freedom.

Dependency Chain

The method is based on estimating frequencies from genotype likelihoods. If alignment data has been supplied you need to specify the following.

1. Genotype likelihood model (-GL).
2. Determine Major/Minor (-doMajorMinor).
3. Maf estimator (-doMaf).

If you have supplied genotype likelihood files as input for angsd you can skip 1.

Score statistic

To perform the test in a generalized linear framework posterior genotype probabilities must be provided or estimated. The approach is published here skotte2012.

-doAsso 2

-yBin [Filename]

A file containing the case control status. 0 being the controls, 1 being the cases and -999 being missing phenotypes.

1
0
0
0
1
1
1
1
0
-999
1
0
0
0
0
1

-yQuant [Filename]

File containing the phenotype values.-999 being missing phenotypes. The file should contain a single phenotype entry per line.

-999
2.06164722761138
-0.091935218675602
-0.287527686061831
-999
-999
-1.20996664036026
0.0188541092307412
-2.1122713873334
-999
-1.32920529536579
-1.10582299663753
-0.391773417823766
-0.501400984567535
-999
1.06014677976046
-1.10582299663753
-999
0.223156127557052
-0.189660869820135

-cov [Filename]

Files containing additional covariates in the analysis. Each lines should contain the additional covariates for a single individuals. Thus the number of lines should match the number of individuals and the number of coloums should match the number of additional covariates.

1 0 0 1 
1 0.1 0 0 
2 0 1 0 
2 0 1 0 
2 0.1 0 1 
1 0 0 1 
1 0.3 0 0 
2 0 0 0 
1 0 0 0 
2 0.2 0 1 
1 0 1 0 
1 0 0 0 
1 0.1 0 0 
1 0 0 0 
2 0 0 1 
2 0 0 0 
2 0 0 0 
1 0 0 1 
1 0.5 0 0 
2 0 0 0

-minHigh [int]

default = 10
This approach needs a certain amount of variability in the genotype probabilities. minHigh filters out sites that does not have at least [int] number of of homozygous major, heterozygous and homozygous minor genotypes. At least two of the three genotypes categories needs at least [int] individuals with a genotype probability above 0.9. This filter avoids the scenario where all individuals have genotypes with the same probability e.g. all are heterozygous with a high probability or all have 0.33333333 probability for all three genotypes.

-minCount [int]

default = 10
The minimum expected minor alleles in the sample. This is the frequency multiplied by two times the number of individuals. Performing association on extremely low minor allele frequencies does not make sence.

-model [int]

1. Additive/Log-additive for Linear/Logistic Regression (Default).
2. Dominant.
3. Recessive.

Example

create a large number of individuals by recycling the example files (500 individuals) and simulate some phentypes (case/control) using R

rm large.filelist
for i in `seq 1 50`;do cat bam.filelist>>large.filelist;done
Rscript -e "write.table(cbind(rbinom(500,1,0.5)),'pheno.ybin',row=F,col=F)"
Rscript -e "write.table(cbind(rnorm(500)),'pheno.yquant',row=F,col=F)"
Rscript -e "set.seed(1);write.table(cbind(rbinom(500,1,0.5),rnorm(500)),'cov.file',row=F,col=F)"

For cases control data for polymorphic sites (p-value < 1e-6)

./angsd -yBin pheno.ybin -doAsso 2 -GL 1 -doPost 1 -out out -doMajorMinor 1 -SNP_pval 1e-6 -doMaf 1 -bam large.filelist -P 5 -r 1:

For quantitative traits (normal distributed errors) for polymorphic sites (p-value < 1e-6) and additional covariates

./angsd -yQuant pheno.yquant -doAsso 2 -cov cov.file -GL 1 -doPost 1 -out out -doMajorMinor 1 -SNP_pval 1e-6 -doMaf 1  -bam large.filelist -P 5  -r 1:

Example with imputation (using BEAGLE)

First the polymorphic sites to be analysed needs to be selected (-doMaf 1 -SNP_pval -doMajorMinor) and the genotype likelihoods estimated (-GL 1) for use in the Beagle software (-doGlf 2).

./angsd -GL 1 -out input -doMajorMinor 1 -SNP_pval 1e-6 -doMaf 1  -bam large.filelist -P 5  -r 1: -doGlf 2

Perform the imputation

java -Xmx15000m -jar beagle.jar like=input.beagle.gz out=beagleOut

the reference fai can be obtained by indexing the reference genome or by using a bam files header

samtools view -H  bams/smallNA11830.mapped.ILLUMINA.bwa.CEU.low_coverage.20111114.bam | grep SN |cut -f2,3 | sed 's/SN\://g' |  sed 's/LN\://g' > ref.fai

The association can then be performed on the genotype probabilities using the score statistics

./angsd -doMaf 4 -beagle beagleOut.impute.beagle.gz.gprobs.gz -fai ref.fai  -yBin pheno.ybin -doAsso 2 

Dependency Chain

The method is based on genotype probabilities. If alignment data has been supplied you need to specify the following.

1. Genotype likelihood model (-GL).
2. Determine Major/Minor (-doMajorMinor).
3. Maf estimator (-doMaf).
4. Calculate posterior genotype probability (-doPost). If you use the score statistics -doAsso 2 then calculate the posterior using the allele frequency as prior (-doPost 1).

If you have supplied genotype likelihoods for angsd, then you should skip 1.

If you have supplied genotype probabilities (as beagle output format), there are no dependencies.

Output

The output from the association analysis is a list of files called prefix.lrt. These are tab separated plain text files, with nine columns.

* Indicates that these columns are only used for the score test.

Example:

Chromosome	Position	Major	Minor	Frequency	N	LRT	high_WT/HE/HO
1	14000023	C	A	0.052976	330	2.863582	250/10/0
1	14000072	G	T	0.020555	330	1.864555	320/10/0
1	14000113	A	G	0.019543	330	0.074985	320/10/0
1	14000202	G	A	0.270106	330	0.181530	50/90/0
1	14000375	T	C	0.020471	330	1.845881	320/10/0
1	14000851	T	C	0.016849	330	0.694058	320/10/0
1	14000873	G	A	0.305990	330	0.684507	140/60/10
1	14001008	T	C	0.018434	330	0.031631	320/10/0
1	14001018	T	C	0.296051	330	0.761196	110/40/10

problems with inflation of p-values

You can evaluate the behavior of the tests by making a QQ plot of the LRT. There are several reasons why it might show signs of inflation

-doPost (when using doAsso 2 without the use of posterior input -beagle

if you estimate the posterior genotype probability using a uniform prior (-doPost 2) then small differences in depth between sample will inflate the test statistics (see Skotte2012. Use the allele frequency as a prior (doPost 1)

-minCount/-minHigh

If you set this too low then it will results in inflation of the test statistics.

-yQuant (when using -doAsso 2 with a quantitative trait)

If your trait is not continues or the distribution of the trait is skewed or has outliers then you will get inflation of p-values. Same rules apply as for a standard regression. Consider transforming you trait into a normal distribution

Population structure

If you have population structure then you will have to adjust for it in the regression model (doAssso 2). Consider using NGSadmix or PCAngsd and use the results as covariates. Note that the model will still have some issues because it uses the allele frequency as a prior. For the adventurous you can use PCAngsd or NGSadmix to estimate the individual allele frequencies and calculate your own genotype probabilities that take structure into account. These can then be used in angsd using the -beagle input format.

low N

Usually a GWAS is performed on thousands of samples and we have only tested the use of the score statistics on hundreds of samples. If you have a low number of samples then try to figure out what minor allele frequency you would need in order to have some power. Also be careful with reducing -minCount/-minHigh.