Quick start
The package diemr incorporates the diagnostic index
expectation maximisation algorithm used to estimate which genomic
alleles belong to which side of a barrier to geneflow. To start using
diemr, load the package or install it from CRAN if it is
not yet available:
# Attempt to load a package, if the package was not available, install and load
if(!require("diemr", character.only = TRUE)){
install.packages("diemr", dependencies = TRUE)
library("diemr", character.only = TRUE)
}
Next, assemble paths to all files containing the data to be used by
diemr. Here, we will use a tiny example dataset that is
included in the package for illustrating the analysis workflow. A good
practice is to check that all files contain data in the correct format
for all individuals and markers. Additionally, the analysis will need a
list with ploidies for all genomic compartments and individuals, and a
vector with indices of samples that will be included in the
analysis.
filepaths <- system.file("extdata", "data6x3.txt", package = "diemr")
# Assuming diploid markers of all individuals
ploidies <- list(rep(2, 6))
# Analysing all individuals
samples <- 1:6
CheckDiemFormat(files = filepaths,
ChosenInds = samples,
ploidy = ploidies)
# File check passed: TRUE
# Ploidy check passed: TRUE
If the CheckDiemFormat() function fails, work through
the error messages and fix the stored input files accordingly. The
algorithm repeatedly accesses data from the harddisk, so seeing the
passed file and variable check prior to the analysis is critical.
To estimate the marker polarities, their diagnostic indices and
support, run the function diem() with default settings.
Here, we have only one file with data, so paralelisation is unnecessary,
and we set nCores = 1. This setting must always be
used on Windows. Other operating systems can process multiple
genomic compartments (e.g. chromosomes) in parallel, and the analysis
of different genomic compartment files can run on multiple
processors.
res <- diem(files = filepaths,
ploidy = ploidies,
markerPolarity = list(c(FALSE, FALSE, TRUE)),
ChosenInds = samples,
nCores = 1)
The result is a list, where the element res$DI contains
a table with marker polarities, their diagnostic indices and
support.
res$DI
# newPolarity DI Support Marker
# 1 FALSE -4.872256 15.930181 1
# 2 TRUE -3.520647 18.633399 2
# 3 TRUE -13.274822 6.130625 3
The column newPolarity means that marker 1 should be
imported for subsequent analyses as is, and markers 2 and 3 should be
imported with 0 replaced with 2 and 2 replaced with 0. The marker 3 has
the lowest diagnostic index and low support, indicating that the
genotypes scored at this marker are poorly related to the barrier to
geneflow arbitrated by the data.
With the marker polarities optimised to detect a barrier to geneflow,
a plot of the polarised genome will show how genomic regions cross the
barrier. First, the genotypes need to be imported with optimal marker
polarities. Second, individual hybrid indices need to be calculated from
the polarised genotypes. And last, the data will be plotted as a raster
image.
genotypes <- importPolarized(file = filepaths,
changePolarity = res$markerPolarity,
ChosenInds = samples)
h <- apply(X = res$I4,
MARGIN = 1,
FUN = pHetErrOnStateCount)[1, ]
plotPolarized(genotypes = genotypes,
HI = h)
Multiple compartments with different ploidies
Some genomic compartments differ between individuals in their ploidy.
For example, markers located on chromosome X in mammals will be diploid
in females, but haploid in males. Ploidy differences between individuals
influence calculation of the hybrid index, which in turn has an effect
on the diem analysis.
To set up the diem analysis with multiple compartments, the
markers with different individual ploidies must be stored in separate
files. The file analysed in the Quick start chapter
could contain markers from autosomes and an additional file will contain
markers from an X chromosome, with individuals 2 and 6 being males. The
respective ploidies for the second genomic compartment will be
c(2, 1, 2, 2, 2, 1).
Arguments files and ploidy will need to
reflect the information, taking care that the order of filenames
corresponds to the order of elements in the list of ploidies.
diem cannot check that the order of the elements is
correct, only that the information is in the correct format.
filepaths2 <- c(system.file("extdata", "data6x3.txt", package = "diemr"),
system.file("extdata", "data7x10.txt", package = "diemr"))
ploidies2 <- list(rep(2, 6),
c(2, 1, 2, 2, 2, 1))
CheckDiemFormat(files = filepaths2,
ChosenInds = samples,
ploidy = ploidies2)
# File check passed: TRUE
# Ploidy check passed: TRUE
# Set random seed for repeatibility of null polarities (optional)
set.seed(39583782)
# Run diem with verbose = TRUE to store hybrid indices with ploidy-aware allele counts
res2 <- diem(files = filepaths2,
ploidy = ploidies2,
markerPolarity = FALSE,
ChosenInds = samples,
nCores = 1,
verbose = TRUE)
Plotting polarised genomes from multiple compartments requires
separate import of the compartment data. The polarities in the
res2$markerPolarity element are combined across all
compartments, and extracting them requires knowledge of the number of
markers in each compartment. Alternatively, the marker polarities from
each compartment can be extracted from the list in the
res2$PolarityChanges element.
# Import each compartment into a list
genotypes2 <- list(importPolarized(file = filepaths2[1],
changePolarity = res2$markerPolarity[1:3],
ChosenInds = samples),
importPolarized(file = filepaths2[2],
changePolarity = res2$markerPolarity[4:13],
ChosenInds = samples))
# Bind compartment genotypes into one matrix
genotypes2 <- Reduce(cbind, genotypes2)
# Load individual hybrid indices from a stored file
h2 <- unlist(read.table("diagnostics/HIwithOptimalPolarities.txt"))
# Plot the polarised genotypes
plotPolarized(genotypes = genotypes2,
HI = h2)
Frequently asked questions
- How can I install
diemr from the
source?
install.packages(package = "diemr_1.1.tar.gz",
repos = NULL, type = "source")
Make sure to set the R working directory to the folder,
where the package tarball is stored, or include a full path to the file
within the quotes. Update the version number to the specific file.
- How can I calculate the hybrid indices from my polarised
data?
There are two options. First, use diem with argument
verbose = TRUE and the hybrid indices will be stored in a
text file in the diagnostics folder in the working directory. The stored
values will be ploidy-aware. However, these hybrid indices could include
the bias introduced by the small data correction if the data warranted
it. The user might prefer to calculate the hybrid indices without the
small data correction. For this, use the I4 matrix in the
diem output.
apply(res$I4, MARGIN = 1, FUN = pHetErrOnStateCount)
# [,1] [,2] [,3] [,4] [,5] [,6]
# p 0.5000000 0 0.3333333 0.5000000 0.8333333 1.0000000
# Het 0.3333333 0 0.6666667 0.3333333 0.3333333 0.0000000
# Err 0.0000000 0 0.0000000 0.0000000 0.0000000 0.3333333
- I expect more than two groups of samples in my data. Can I
use
diemr?
Yes. Multiple barriers to geneflow between multiple groups of samples
can be identified iteratively with help from the argument
ChosenInds. For example, let’s assume that the individual 2
was identified as belonging to one side of the barrier and being
separated from other by the steepest change in the hybrid index. In the
next diem run, we exclude the individual 2, adjusting the
ploidies to reflect the omission.
ploidies2 <- list(c(2, 2, 2, 2, 2))
samples2 <- c(1, 3:6)
CheckDiemFormat(files = filepaths,
ChosenInds = samples2,
ploidy = ploidies2)
# File check passed: TRUE
# Ploidy check passed: TRUE
res2 <- diem(files = filepaths,
ChosenInds = samples2,
ploidy = ploidies2,
nCores = 1,
markerPolarity = list(c(FALSE, FALSE, TRUE)))
# calculate hybrid indices from updated I4
h.res2 <- apply(res2$I4,
MARGIN = 1,
FUN = pHetErrOnStateCount)[1, ]
# set names for the hybrid index values
h.res2 <- setNames(h.res2, nm = samples2)
# 1 3 4 5 6
# 0.50 0.33 0.50 0.83 1.00
# calculate the center of the maximum hybrid index change
diffs <- data.frame(rollmean = zoo::rollmean(sort(h.res2), k = 2),
diff = diff(sort(h.res2), lag = 1))
h.res2.c <- diffs$rollmean[which.max(diffs$diff)]
# [1] 0.6666667
Since the center of the barrier is at 0.67 now, diem
separated individuals 1, 3, and 4 from a group that includes 5, 6.
Combined with the result from the first diem run, we have
identified three groups in the dataset: (2), (1, 3, 4), and (5, 6).
- The hybrid indices in my dataset are too similar. I expected
them to look more like the rescaled hybrid indices. What is
wrong?
The input data probably contains invariant sites, which weight the
hybrid indices to be similar between individuals. Make sure to use only
variable sites. Alternatively, filter sites with lowest diagnostic index
after the diem analysis and recalculate the hybrid indices
with the filtered data.
- How to cite
diemr?
To use diemr in a publication, please cite:
Baird S. J. E., Petruzela J., Jaron I., Skrabanek P., Martinkova N.
2022. Genome polarisation for detecting barriers to geneflow. Methods in
Ecology and Evolution, doi: 10.1111/2041-210X.14010.