Provided by: qtltools_1.3.1+dfsg-2build2_amd64 
NAME
QTLtools cis - cis QTL analysis
SYNOPSIS
QTLtools cis --vcf [in.vcf|in.vcf.gz|in.bcf|in.bed.gz] --bed quantifications.bed.gz
[--nominal float | --permute integer | --mapping in.txt] --out output.txt [OPTIONS]
DESCRIPTION
This mode maps cis (proximal) quantitative trait loci (QTLs) that affect the phenotype,
using linear regression. The method is detailed in
<https://www.nature.com/articles/ncomms15452>. We first regress out the provided
covariates from the phenotype data, followed by running the linear regression between the
phenotype residuals and the genotype. If --normal and --cov are provided at the same
time, then the residuals after the covariate correction are rank normal transformed. It
incorporates an efficient permutation scheme to control for differential multiple testing
burden of each phenotype. You can run a nominal pass (--nominal threshold) listing all
genotype-phenotype associations below a certain threshold, a permutation pass (--permute
no_of_permutations) to empirically characterize the null distribution of associations for
each phenotype separately, thus adjusting the nominal p-value of the best association for
a phenotype, or a conditional analysis pass (--mapping filename) to discover multiple
proximal QTLs with independent effects on a phenotype.
As multiple molecular phenotypes can belong to higher order biological entities, e.g.
exons of genes, QTLtools cis allows grouping of phenotypes to maximize the discoveries in
such particular cases. Specifically, QTLtools can either aggregate multiple phenotypes in
a given group into a single phenotype via PCA (--grp-pca1) or by taking their mean (--grp-
mean), or directly use all individual phenotypes in an extended permutation scheme that
accounts for their number and correlation structure (--grp-best). In our experience,
--grp-best outperforms the other options for expression QTLs (eQTLs).
The conditional analysis pass first uses permutations to derive a nominal p-value
threshold per phenotype that varies and reflects the number of independent tests per
cis-window. Then, it uses a forward-backward stepwise regression to learn the number of
independent signals per phenotype, determine the best candidate variant per signal and
assign all significant hits to the independent signal they relate to.
Since linear regressions assumes normally distributed data, we highly recommend using the
--normal option to rank normal transform the phenotype quantifications in order to avoid
false positive associations due to outliers.
OPTIONS
--vcf [in.vcf|in.bcf|in.vcf.gz|in.bed.gz]
Genotypes in VCF/BCF format, or another molecular phenotype in BED format. If
there is a DS field in the genotype FORMAT of a variant (dosage of the genotype
calculated from genotype probabilities, e.g. after imputation), then this is used
as the genotype. If there is only the GT field in the genotype FORMAT then this is
used and it is converted to a dosage. REQUIRED.
--bed quantifications.bed.gz
Molecular phenotype quantifications in BED format. REQUIRED.
--out output.txt
Output file. REQUIRED.
--cov covariates.txt
Covariates to correct the phenotype data with.
--normal
Rank normal transform the phenotype data so that each phenotype is normally
distributed. RECOMMENDED.
--std-err
Calculate and output the standard error of the beta (slope).
--window integer
Size of the cis window flanking each phenotype's start position. DEFAULT=1000000.
RECOMMENDED=1000000.
--nominal float
Calculate the nominal p-value for the genotype-phenotype associations and print out
the ones that pass the provided threshold. Give 1.0 to print everything. Mutually
exclusive with --permute and --mapping.
--permute integer
Adjust the best nominal p-value for this phenotype accounting for the number of
variants and the linkage disequilibrium in its cis-window. We recommend at least
1000 permutation for the final analysis, and in most cases you will see diminishing
returns when going over 5000. However, if you are doing exploratory analyses like
which/how many covariates to include, you can go as low as 100. Mutually exclusive
with --nominal and --mapping. RECOMMENDED=1000.
--mapping thresholds_filename
The conditional analysis. First you need to run a permutation analysis, then
generate a thresholds file using the runFDR_cis.R script in the script directory.
Mutually exclusive with --nominal and --permute.
--grp-best
Correct for multiple phenotypes within a phenotype group. Mutually exclusive with
--grp-pca1 and --grp-mean.
--grp-pca1
Run PCA on phenotypes within a phenotype group and use PC1 for association testing.
Mutually exclusive with --grp-best and --grp-mean.
--grp-mean
Average phenotypes within a group and use the results for association testing.
Mutually exclusive with --grp-best and --grp-pca1.
--chunk integer1 integer2
For parallelization. Divide the data into integer2 number of chunks and process
chunk number integer1. Chunk 0 will print a header. Mutually exclusive with
--region and --region-pair. Minimum number of chunks has to be at least the same
number of chromosomes in the --bed file.
--region chr:start-end
Genomic region to be processed. E.g. chr4:12334456-16334456, or chr5 Mutually
exclusive with --chunk and --region-pair.
--region-pair chr:start-end chr:start-end
Genomic region for genotypes followed by region for phenotypes to be processed.
Mutually exclusive with --chunk and --region.
OUTPUT FILES
--nominal output file
Space separated output file with the following columns (certain columns are only printed
based on options). We recommend including chunk 0 to print out a header in order to
avoid confusion.
1 phe_id | grp_id The phenotype ID or if one of the grouping
options is provided, then phenotype group ID
2 phe_chr The phenotype chromosome
3 phe_from Start position of the phenotype
4 phe_to End position of the phenotype
5 phe_strd The phenotype strand
5.1 phe_id | ve_by_pc1 | n_phe_in_grp Only printed if --group-best | --group-pca1 |
--group-mean. The phenotype ID, variance
explained by PC1, or number of phenotypes in
the phenotype group for --group-best, --group-
pca1, and --group-mean, respectively.
5.2 n_phe_in_grp Only printed if --group-pca1 | --group-mean.
The number of phenotypes in the phenotype
group.
6 n_var_in_cis The number variants in the cis window for this
phenotype.
7 dist_phe_var The distance between the variant and the
phenotype start positions.
8 var_id The variant ID.
9 var_chr The variant chromosome.
10 var_from The start position of the variant.
11 var_to The end position of the variant.
12 nom_pval The nominal p-value of the association between
the variant and the phenotype.
13 r_squared The r squared of the linear regression.
14 slope The beta (slope) of the linear regression.
14.1 slope_se The standard error of the beta. Only printed
if --std-err is provided.
15 best_hit Whether this varint was the best hit for this
phenotype.
--permute output file
Space separated output file with the following columns (certain columns are only printed
based on options). We recommend including chunk 0 to print out a header in order to
avoid confusion.
1 phe_id | grp_id The phenotype ID or if one of the grouping
options is provided, then phenotype group ID
2 phe_chr The phenotype chromosome
3 phe_from Start position of the phenotype
4 phe_to End position of the phenotype
5 phe_strd The phenotype strand
5.1 phe_id | ve_by_pc1 | n_phe_in_grp Only printed if --group-best | --group-pca1 |
--group-mean. The phenotype ID, variance
explained by PC1, or number of phenotypes in
the phenotype group for --group-best, --group-
pca1, and --group-mean, respectively.
5.2 n_phe_in_grp Only printed if --group-pca1 | --group-mean.
The number of phenotypes in the phenotype
group.
6 n_var_in_cis The number variants in the cis window for this
phenotype.
7 dist_phe_var The distance between the variant and the
phenotype start positions.
8 var_id The most significant variant ID.
9 var_chr The most significant variant's chromosome.
10 var_from The start position of the most significant
variant.
11 var_to The end position of the most significant
variant.
12 dof1 The number of degrees of freedom used to
compute the p-values.
13 dof2 Estimated number of degrees of freedom used in
beta approximation p-value calculations.
14 bml1 The first shape parameter of the fitted beta
distribution (alpha parameter). These should
be close to 1.
15 bml2 The second shape parameter of the fitted beta
distribution (beta parameter). This
corresponds to the effective number of
independent tests in the region.
16 nom_pval The nominal p-value of the association between
the most significant variant and the
phenotype.
17 r_squared The r squared of the linear regression.
18 slope The beta (slope) of the linear regression.
18.1 slope_se The standard error of the beta. Only printed
if --std-err is provided.
19 adj_emp_pval Adjusted empirical p-value from permutations.
This is the adjusted p-value not using the
beta approximation. Simply calculated as:
(number of p-values observed during
permutations that were smaller than or equal
to the nominal p-value + 1) / (number of
permutations + 1). The most significant p-
value achievable would be 1 / (number of
permutations + 1).
20 adj_beta_pval Adjusted empirical p-value given by the fitted
beta distribution. We strongly recommend
using this adjusted p-value in any downstream
analysis.
--mapping output file
Space separated output file with the following columns (certain columns are only printed
based on options). We recommend including chunk 0 to print out a header in order to
avoid confusion.
1 phe_id | grp_id The phenotype ID or if one of the grouping
options is provided, then phenotype group ID
2 phe_chr The phenotype chromosome
3 phe_from Start position of the phenotype
4 phe_to End position of the phenotype
5 phe_strd The phenotype strand
5.1 phe_id | ve_by_pc1 | n_phe_in_grp Only printed if --group-best | --group-pca1 |
--group-mean. The phenotype ID, variance
explained by PC1, or number of phenotypes in
the phenotype group for --group-best, --group-
pca1, and --group-mean, respectively.
5.2 n_phe_in_grp Only printed if --group-pca1 | --group-mean.
The number of phenotypes in the phenotype
group.
6 n_var_in_cis The number variants in the cis window for this
phenotype.
7 dist_phe_var The distance between the variant and the
phenotype start positions.
8 var_id The most significant variant ID.
9 var_chr The most significant variant's chromosome.
10 var_from The start position of the most significant
variant.
11 var_to The end position of the most significant
variant.
12 rank The rank of the association. This tells you
if the variant has been mapped as belonging to
the best signal (rank=0), the second best
(rank=1), etc ... As a consequence, the
maximum rank value for a given phenotype tells
you how many independent signals there are
(e.g. rank=2 means 3 independent signals).
13 fwd_pval The nominal forward p-value of the association
between the most significant variant and the
phenotype.
14 fwd_r_squared The r squared of the forward linear
regression.
15 fwd_slope The beta (slope) of the forward linear
regression.
15.1 fwd_slope_se The standard error of the forward beta. Only
printed if --std-err is provided.
16 fwd_best_hit Whether or not this variant was the forward
most significant variant.
17 fwd_sig Whether this variant was significant.
Currently all variants are significant so this
is redundant.
18 bwd_pval The nominal backward p-value of the
association between the most significant
variant and the phenotype.
19 bwd_r_squared The r squared of the backward linear
regression.
20 bwd_slope The beta (slope) of the backward linear
regression.
20.1 bwd_slope_se The standard error of the backward beta. Only
printed if --std-err is provided.
21 bwd_best_hit Whether or not this variant was the backward
most significant variant.
22 bwd_sig Whether this variant was significant.
Currently all variants are significant so this
is redundant.
NOMINAL ANALYSIS EXAMPLES
o Nominal pass, correcting for technical covariates, rank normal transforming the
phenotype, and printing out associations with a p-value <= 0.01 on chromosome 22 between
17000000 and 18000000 bp, and excluding some samples (see QTLtools (1)):
QTLtools cis --vcf genotypes.chr22.vcf.gz --bed genes.50percent.chr22.bed.gz --cov
genes.covariates.pc50.txt.gz --nominal 0.01 --region chr22:17000000-18000000 --normal
--out nominals.txt --exclude-samples sample_names_to_exclude.txt
o Nominal pass with parallelization correcting for technical covariates, rank normal
transforming the phenotype, and printing out associations with a p-value <= 0.01. To
facilitate parallelization on compute cluster, we developed an option to run the
analysis into chunks of molecular phenotypes. For instance, to run analysis on chunk 12
when splitting the example data set into 20 chunks, run:
QTLtools cis --vcf genotypes.chr22.vcf.gz --bed genes.50percent.chr22.bed.gz --cov
genes.covariates.pc50.txt.gz --nominal 0.01 --chunk 12 20 --normal --out
nominals_12_20.txt
o If you want to submit the whole analysis with 20 jobs on a compute cluster, just run
(qsub needs to be changed to the job submission system used [bsub, psub, etc...]):
for j in $(seq 0 20); do
echo "QTLtools cis --vcf genotypes.chr22.vcf.gz --bed genes.50percent.chr22.bed.gz
--cov genes.covariates.pc50.txt.gz --nominal 0.01 --chunk $j 20 --normal --out
nominals_$j\_20.txt" | qsub
done
PERMUTATION ANALYSIS EXAMPLES
o Permutation pass, correcting for technical covariates, rank normal transforming the
phenotype, and running 1000 permutations with a specific random seed on chromosome 22
between 17000000 and 18000000 bp:
QTLtools cis --vcf genotypes.chr22.vcf.gz --bed genes.50percent.chr22.bed.gz --cov
genes.covariates.pc50.txt.gz --permute 1000 --region chr22:17000000-18000000 --normal
--seed 1354145 --out permutation.txt
o Permutation pass with parallelization correcting for technical covariates, rank normal
transforming the phenotype, and running 5000 permutations. To facilitate
parallelization on compute cluster, we developed an option to run the analysis into
chunks of molecular phenotypes. For instance, to run analysis on chunk 12 when
splitting the example data set into 20 chunks, run:
QTLtools cis --vcf genotypes.chr22.vcf.gz --bed genes.50percent.chr22.bed.gz --cov
genes.covariates.pc50.txt.gz --permute 5000 --chunk 12 20 --normal --out
permutations_12_20.txt
o If you want to submit the whole analysis with 20 jobs on a compute cluster, just run
(qsub needs to be changed to the job submission system used [bsub, psub, etc...]):
for j in $(seq 0 20); do
echo "QTLtools cis --vcf genotypes.chr22.vcf.gz --bed genes.50percent.chr22.bed.gz
--cov genes.covariates.pc50.txt.gz --permute 5000 --chunk $j 20 --normal --out
permutations_$j\_20.txt" | qsub
done
o When your phenotypes in the BED file are grouped, you can perform a permutation pass at
the phenotype group level in order to discover group-level QTLs:
QTLtools cis --vcf genotypes.chr22.vcf.gz --bed exons.50percent.chr22.bed.gz --cov
genes.covariates.pc50.txt.gz --permute 1000 --normal --grp-best --out
permutation.group.txt
CONDITIONAL ANALYSIS EXAMPLE
Conditional analysis to discover independent signals.
1 First we need to run a permutation analysis (see previous section), then calculate
nominal p-value threshold for each gene. Here an FDR of 5% is given as an example:
cat permutations_*.txt | gzip -c > permutations_all.txt.gz
Rscript ./script/qtltools_runFDR_cis.R permutations_all.txt.gz 0.05 permutations_all
2 Now you can proceed with the actual conditional analysis. Here splitting into 20
chunks, and when all complete concatenate the results:
for j in $(seq 0 20); do
echo "QTLtools cis --vcf genotypes.chr22.vcf.gz --bed genes.50percent.chr22.bed.gz
--cov genes.covariates.pc50.txt.gz --mapping permutations_all.thresholds.txt --chunk
$j 20 --normal --out conditional_$j\_20.txt" | qsub
done
cat conditional_*.txt > conditional_all.txt
3 If you are interested in the most significant variants per independent signal, you can
filter the results, using the backward p-value:
awk '{ if ($21 == 1) print $0 }' conditional_all.txt > conditional_top_variants.txt
SEE ALSO
QTLtools(1)
QTLtools website: <https://qtltools.github.io/qtltools>
BUGS
o Versions up to and including 1.2, suffer from a bug in reading missing genotypes in
VCF/BCF files. This bug affects variants with a DS field in their genotype's FORMAT and
have a missing genotype (DS field is .) in one of the samples, in which case genotypes
for all the samples are set to missing, effectively removing this variant from the
analyses.
Please submit bugs to <https://github.com/qtltools/qtltools>
CITATION
Delaneau, O., Ongen, H., Brown, A. et al. A complete tool set for molecular QTL discovery
and analysis. Nat Commun 8, 15452 (2017). <https://doi.org/10.1038/ncomms15452>
AUTHORS
Olivier Delaneau (olivier.delaneau@gmail.com), Halit Ongen (halitongen@gmail.com)