In benstory/mitoClone2: Clonal Population Identification in Single-Cell RNA-Seq Data using Mitochondrial and Somatic Mutations
Before you begin
library(mitoClone2)
You should have identified true somatic variants in the mitochondrial
(and nuclear) genome. The remaining vignettes of this package document
how to get there. Here, we start with count matrices of the alternative
and the reference alleles, across a number of sites of interest. Such
data is available from two patients (P1, P2) as part of this package.
Only P1 is analyzed as part of this vignette but the commented code
for P2 should be fully functional.
knitr::opts_chunk$set(
collapse = TRUE,
comment = "#>",
tidy.opts=list(width.cutoff=70),
tidy=TRUE
)
load(system.file("data/M_P1.RData",package = "mitoClone2"))
load(system.file("data/N_P1.RData",package = "mitoClone2"))
P1 <- mutationCallsFromMatrix(as.matrix(M_P1), as.matrix(N_P1))
A first important step is to decide which mutations to include in the
clustering. The default is to use all mutations that are covered in at
least 20% of the cells, but this assignment can be changed manually.
Compute a phylogenetic tree
The next step is to run SCITE or
PhISCS to compute the most likely
phylogenetic tree. PhISCS is bundled in this package, but the package needs
to be run in an environment where gurobi and the
gurobipy python package are available. For example, you could set up a
conda environment that contains this package. SCITE does not require any
additional licenses but may need to be manually compiled.
## this next step takes approx 4.1 minutes to run
tmpd <- tempdir()
dir.create(paste0(tmpd,'/p1'))
P1 <- varCluster(P1, tempfolder=paste0(tmpd,'/p1'),method='SCITE')
This step can take a while to run. It computes a likely phylogenetic tree of
all the mutations. In the case of SCITE, multiple equally likely tree can be
produced. In it's current state, this package simply selects the first tree
from the list.
Identify clones and assign cells to clones
In many cases, the order of the leaves on these trees is arbitrary, because
mutations systematically co-occur. We therefore cluster the mutations into
clones. In detail, we take every every branch on the tree and then shuffle
the order of mutations in that branch while re-calculating the likelihood.
If swapping nodes leads to small changes in the likelihood, these nodes
are then merged into a "clone". The parameter min.lik that controls
the merging is set arbitrarily, see below for more information.
P1 <- clusterMetaclones(P1, min.lik = 1)
This step also assigns each cell to the most likely clone, and provides an
estimate of the likelihood. Refer to help(mutationCalls) for more info
on how these results are stored.
Finally, the clustering can be plotted.
plotClones(P1)
Parameter choice
The parameter min.lik that controls the merging is set arbitrarily. In
practice, the goal of these analyses is to group mutations into clones
for subsequent analyses (such as differential expression analyses) and
it may make sense to overwrite the result of clusterMetaclones manually;
for example, if a subclone defned on a mitochondrial mutation only should
be treated as part of a more clearly defined upstream clone for
differential expression analysis.
To overwrite the result of clusterMetaclones, first retrieve the
assignment of mutations to clones:
m2c <- mitoClone2:::getMut2Clone(P1)
print(m2c)
##To e.g. treat the mt:2537G>A and mt:14462:G>A mutations as a subclone
##distinct from CEBPA, we can assign them a new clonal identity
m2c[c("X2537GA","X14462GA")] <- as.integer(6)
P1.new <- mitoClone2:::overwriteMetaclones(P1, m2c)
plotClones(P1.new)
Session information
sessionInfo()
benstory/mitoClone2 documentation built on Oct. 30, 2024, 3:20 p.m.
R Package Documentation
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Note that we can't provide technical support on individual packages. You should contact the package authors for that.
Before you begin
library(mitoClone2)
You should have identified true somatic variants in the mitochondrial (and nuclear) genome. The remaining vignettes of this package document how to get there. Here, we start with count matrices of the alternative and the reference alleles, across a number of sites of interest. Such data is available from two patients (P1, P2) as part of this package. Only P1 is analyzed as part of this vignette but the commented code for P2 should be fully functional.
knitr::opts_chunk$set( collapse = TRUE, comment = "#>", tidy.opts=list(width.cutoff=70), tidy=TRUE )
load(system.file("data/M_P1.RData",package = "mitoClone2")) load(system.file("data/N_P1.RData",package = "mitoClone2")) P1 <- mutationCallsFromMatrix(as.matrix(M_P1), as.matrix(N_P1))
A first important step is to decide which mutations to include in the clustering. The default is to use all mutations that are covered in at least 20% of the cells, but this assignment can be changed manually.
Compute a phylogenetic tree
The next step is to run SCITE or
PhISCS to compute the most likely
phylogenetic tree. PhISCS is bundled in this package, but the package needs
to be run in an environment where gurobi and the
gurobipy python package are available. For example, you could set up a
conda environment that contains this package. SCITE does not require any
additional licenses but may need to be manually compiled.
## this next step takes approx 4.1 minutes to run tmpd <- tempdir() dir.create(paste0(tmpd,'/p1')) P1 <- varCluster(P1, tempfolder=paste0(tmpd,'/p1'),method='SCITE')
This step can take a while to run. It computes a likely phylogenetic tree of all the mutations. In the case of SCITE, multiple equally likely tree can be produced. In it's current state, this package simply selects the first tree from the list.
Identify clones and assign cells to clones
In many cases, the order of the leaves on these trees is arbitrary, because
mutations systematically co-occur. We therefore cluster the mutations into
clones. In detail, we take every every branch on the tree and then shuffle
the order of mutations in that branch while re-calculating the likelihood.
If swapping nodes leads to small changes in the likelihood, these nodes
are then merged into a "clone". The parameter min.lik that controls
the merging is set arbitrarily, see below for more information.
P1 <- clusterMetaclones(P1, min.lik = 1)
This step also assigns each cell to the most likely clone, and provides an
estimate of the likelihood. Refer to help(mutationCalls) for more info
on how these results are stored.
Finally, the clustering can be plotted.
plotClones(P1)
Parameter choice
The parameter min.lik that controls the merging is set arbitrarily. In
practice, the goal of these analyses is to group mutations into clones
for subsequent analyses (such as differential expression analyses) and
it may make sense to overwrite the result of clusterMetaclones manually;
for example, if a subclone defned on a mitochondrial mutation only should
be treated as part of a more clearly defined upstream clone for
differential expression analysis.
To overwrite the result of clusterMetaclones, first retrieve the
assignment of mutations to clones:
m2c <- mitoClone2:::getMut2Clone(P1) print(m2c) ##To e.g. treat the mt:2537G>A and mt:14462:G>A mutations as a subclone ##distinct from CEBPA, we can assign them a new clonal identity m2c[c("X2537GA","X14462GA")] <- as.integer(6) P1.new <- mitoClone2:::overwriteMetaclones(P1, m2c) plotClones(P1.new)
Session information
sessionInfo()
R Package Documentation
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We want your feedback!
Note that we can't provide technical support on individual packages. You should contact the package authors for that.
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