Introduction to MAPpoly
2024-03-05
MAPpoly is an R package to construct genetic maps in autopolyploids
with even ploidy levels. This quick start guide will present some
essential functions to construct a tetraploid potato map. Please refer
to MAPpoly’s Reference Manual
and the Extended
Tutorial for a comprehensive description of all functions.
Reading data set
There are several functions to read discrete and probabilistic
dosage-based genotype data sets in MAPpoly. You can read a data set from
TXT, CSV, VCF, fitPoly-generated or import it from the R packages
polyRAD, polymapR, and updog. The data set distributed along with
MAPpoly is a subset of markers from (Pereira et al.,
2021) in CSV
format. Let us read it into MAPpoly
library(mappoly)
file.name <- system.file("extdata/potato_example.csv", package = "mappoly")
dat <- read_geno_csv(file.in = file.name, ploidy = 4)
print(dat, detailed = T)
plot(dat)
The output figure shows a bar plot on the left-hand side with the
number of markers in each allele dosage combination in \(P_1\) and \(P_2\), respectively. The upper-right plot
contains the \(\log_{10}(p-value)\)
from \(\chi^2\) tests for all markers,
considering the expected segregation patterns under Mendelian
inheritance.
Data quality control
Quality control (QC) procedures are fundamental to identify:
- Individuals from crosses other than \(P_1
\times P_2\)
- Individuals and markers that exceeds a defined threshold of missing
data points
- Markers with distorted segregation
- Markers with the same genotypic information (redundant markers).
Removed markers are positioned into the final map.
Depending on the data set, these procedures can be conducted in any
order. Let us first remove individuals from crosses other than \(P_1 \times P_2\). When using the
interactive function, the user needs to select a polygon around the
individuals to be removed by clicking its vertices and pressing Esc.
dat <- filter_individuals(dat)
Now, let us filter out markers and individuals with more than 5% of
missing data. You can update the threshold interactively
dat <- filter_missing(dat, type = "marker", filter.thres = .05)
dat <- filter_missing(dat, type = "individual", filter.thres = .05)
Finally, we can filter out markers with distorted segregation and
redundant information. At this point, we do not consider preferential
pairing and double reduction.
seq.filt <- filter_segregation(dat, chisq.pval.thres = 0.05/dat$n.mrk)
seq.filt <- make_seq_mappoly(seq.filt)
seq.red <- elim_redundant(seq.filt)
After filtering, 1990 markers were left to be mapped. Now, let us
create a sequence of ordered markers to proceed with the analysis. You
can also plot the data set for a specific sequence of markers
seq.init <- make_seq_mappoly(seq.red)
plot(seq.init)
and check the distribution of the markers in the reference genome, if
the information is available
go <- get_genomic_order(input.seq = seq.init) ## get genomic order of the sequence
plot(go)
Two-point analysis
The two-point analysis calculates the pairwise recombination fraction
in a sequence of markers. At this point of the analysis, where we have
many markers, we use the function est_pairwise_rf2, which
has a less detailed output than the original
est_pairwise_rf (which will be used later) but can handle
tens of thousands of markers, even when using a personal computer.
Nevertheless, the analysis can take a while depending on the number of
markers if few cores are available.
ncores <- parallel::detectCores() - 1
tpt <- est_pairwise_rf2(seq.init, ncpus = ncores)
m <- rf_list_to_matrix(tpt) ## converts rec. frac. list into a matrix
sgo <- make_seq_mappoly(go) ## creates a sequence of markers in the genome order
plot(m, ord = sgo, fact = 5) ## plots a rec. frac. matrix using the genome order, averaging neighbor cells in a 5 x 5 grid
Grouping
We can cluster the markers in linkage groups by using function
group_mappoly. The function uses the recombination fraction
matrix and UPGMA method to group markers. Use the option
comp.mat = TRUE to compare the linkage-based clustering
results with the chromosome information. If your data set does not
contain chromosome information, use the option
comp.mat = FALSE. You also can use the interactive version
to change the number of expected groups
g <- group_mappoly(m, expected.groups = 12, comp.mat = TRUE)
plot(g)
g
In the table above, the rows indicate linkage groups obtained using
linkage information and, the columns are the chromosomes in the
reference genome. Notice the diagonal indicating the concordance between
the two sources of information.
Ordering markers
Markers are ordered within linkage groups. In this tutorial, we will
show the step-by-step procedure using Linkage Group 1 (LG1). You can do
the same for the remaining linkage groups.
Since we had a good concordance between genome and linkage
information, we will use only markers assigned to a particular linkage
group using both sources of information. We will do that using
genomic.info = 1 , so the function uses the intersection of
the markers assigned using linkage and the chromosome with the highest
number of allocated markers. To use only the linkage information, do not
use the argument genomic.info. You also need the
recombination fraction matrix for that group.
s1 <- make_seq_mappoly(g, 1, ## Select LG1
genomic.info = 1)
m1 <- make_mat_mappoly(m, s1)
Let us order the markers in the sequence using the MDS algorithm.
mds.o1 <- mds_mappoly(input.mat = m1)
s1.mds <- make_seq_mappoly(mds.o1)
plot(m1, ord = s1.mds)
Usually, at this point, the user can use diagnostic plots to remove
markers that disturb the ordering procedure. We didn’t use that
procedure in this tutorial, but we encourage the user to check the
example in ?mds_mappoly. Now, let us use the reference
genome to order the markers.
You also can order the markers the reference genome
gen.o1 <- get_genomic_order(s1)
s1.gen <- make_seq_mappoly(gen.o1)
plot(m1, ord = s1.gen)
For the sake of this short tutorial, let us use the MDS order
(s1.mds) to phase the markers. Still, you can also try the
genome order (s1.gen) and compare the resulting maps using
function compare_maps, and you will notice that the genomic
order yields a better map since its likelihood is higher.
Phasing markers and estimating multilocus recombination
fractions.
Estimating the genetic map for a given order involves the computation
of recombination fraction between adjacent markers and inferring the
linkage phase configuration of those markers in both parents. The core
function to perform these tasks in MAPpoly is
est_rf_hmm_sequential. This function uses the pairwise recombination fraction as the first source of
information to sequentially position allelic variants in specific
parental homologs. The algorithm relies on the likelihood obtained
through a hidden Markov model (HMM) for situations where pairwise
analysis has limited power. Once all markers are positioned, the final
map is reconstructed using the HMM multipoint algorithm. For a detailed
description of the est_rf_hmm_sequential arguments, please
refer to MAPpoly’s Reference Manual
and the Extended
Tutorial.
First we need to calculate the pairwise recombination fraction for
markers in sequence s1.mds using
est_pairwise_rf, which contains the information necessary
to the proper working of the phasing algorithm.
tpt1 <- est_pairwise_rf(s1.mds, ncpus = ncores)
lg1.map <- est_rf_hmm_sequential(input.seq = s1.mds,
start.set = 3,
thres.twopt = 10,
thres.hmm = 20,
extend.tail = 50,
info.tail = TRUE,
twopt = tpt1,
sub.map.size.diff.limit = 5,
phase.number.limit = 20,
reestimate.single.ph.configuration = TRUE,
tol = 10e-3,
tol.final = 10e-4)
Now, use the functions print and plot to
view the map results:
print(lg1.map)
plot(lg1.map, mrk.names = TRUE, cex = 0.7)
Now let us update the recombination fractions by allowing a global
error in the HMM recombination fraction re-estimation. Using this
approach, the genetic map’s length will be updated by removing spurious
recombination events. This procedure can be applied using either the
probability distribution provided by the genotype calling software using
function est_full_hmm_with_prior_prob or assuming a global
genotype error like the following example
lg1.map.up <- est_full_hmm_with_global_error(input.map = lg1.map, error = 0.05,
verbose = TRUE)
plot(lg1.map.up, mrk.names = TRUE, cex = 0.7)
We can also use the ordinary least squares (OLS) method and the
weighted MDS followed by fitting a one dimensional principal curve
(wMDS_to_1D_pc)
lg1.map.ols <- reest_rf(lg1.map, m1, method = "ols")
lg1.map.mds <- reest_rf(lg1.map, m1, method = "wMDS_to_1D_pc", input.mds = mds.o1)
Now let us create a list with the maps and plot the results
map.list.lg1 <- list(orig = lg1.map,
updt = lg1.map.up,
ols = lg1.map.ols,
mds = lg1.map.mds)
plot_map_list(map.list.lg1, col = "ggstyle", title = "Estimation method")
Homolog probability and preferential pairing profile
To use the genetic map in conjunction with QTL analysis software, we
need to obtain the homolog probability for all linkage groups for all
individuals in the full-sib population. In this short guide, we will
proceed only with one linkage group, but this procedure should be
applied to all chromosomes in real situations. Let us use the updated
map
g1 <- calc_genoprob_error(lg1.map.up, step = 1, error = 0.05)
to.qtlpoly <- export_qtlpoly(g1) #export to QTLpoly
h1 <- calc_homologprob(g1)
plot(h1, lg = 1, ind = 10)
Now let us compute the preferential pairing profile for linkage group
1
p1 = calc_prefpair_profiles(g1)
plot(p1, min.y.prof = 0.25, max.y.prof = 0.4, P1 = "Atlantic", P2 = "B1829.5")
Exporting a phased map
It is possible to export a phased map to an external CSV file
using
export_map_list(lg1.map.up, file = "output_file.csv")
For a script with a complete analysis of the data set presented here,
please refer to the Complete
script
Utility functions
To use the next functions, let us load the complete genetic map
in.file <- "https://github.com/mmollina/SCRI/raw/main/docs/tetra/maps_updated.rda"
map_file <- tempfile()
download.file(in.file, map_file)
load(map_file)
Plot genome vs. map
plot_genome_vs_map(MAPs.up, same.ch.lg = TRUE)
