library(BiocStyle) BiocStyle::markdown()
Besides retrieving genomic and protein annotations, ensembldb
provides also
functionality to map between protein, transcript and genome coordinates. This
mapping relies on annotations of proteins (their sequences) to their encoding
transcripts which are stored in EnsDb
databases.
The available functions and their input and result objects are:
genomeToTranscript
: maps genomic coordinates to coordinates within the
transcript(s) encoded at the specified coordinates. The function takes a
GRanges
as input and returns an IRangesList
of length equal to the length
of the input object. Each IRanges
in the IRangesList
provides the
coordinates within the respective transcript.
genomeToProtein
: maps genomic coordinates to positions within the sequence
of the eventually encoded protein(s) in the genomic region. The function takes
a GRanges
as input and returns an IRangesList
of the same length, each
element (IRanges
) providing the coordinates within the respective protein's
sequence.
proteinToTranscript
: maps protein-relative coordinates to positions within
the encoding transcripts. Takes an IRanges
as input and returns an
IRangesList
of the same length with each element (IRanges
) providing the
coordinates within the transcript (relative to the first nucleotide of the
transcript).
proteinToGenome
: maps protein-relative coordinates to genomic region(s)
encoding the amino acid sequence. The function takes an IRanges
as input and
returns a list
of either GRanges
(if Ensembl protein identifiers are
provided in the input object) or GRangesList
(if the protein identifier
provided for the input range can be mapped to multiple Ensembl protein IDs).
transcriptToGenome
: maps coordinates within a transcript to genomic
coordinates. Takes an IRanges
as input and returns a GRangesList
(within-transcript coordinates can be mapped to several exons and hence
genomic locations). The returned GRangesList
has the same length than the
input IRanges
, with empty GRanges
for transcripts that can not be found in
the database (and thus can not be mapped to the genome) or for IRanges
that
define regions outside of the transcript's sequence.
transcriptToProtein
: maps regions within a transcript to the respective
amino acid residues in the encoded protein's sequence. The function takes an
IRanges
as input and returns an IRanges
of the same length.
transcriptToCds
: maps between transcript-relative and CDS-relative
coordinates (for protein-coding genes only).
cdsToTranscript
: maps between CDS-relative and transcript-relative
coordinates (for protein-coding genes only).
All functions, except proteinToGenome
and transcriptToGenome
return
IRanges
with negative coordinates if the mapping failed (e.g. because the
identifier is unknown to the database, or if, for mappings to and from protein
coordinates, the input coordinates are not within the coding region of a
transcript). proteinToGenome
and transcriptToGenome
return empty GRanges
if mappings fail.
Each protein encoding transcript is annotated by Ensembl to an unique
translation with an assigned Ensembl protein ID. In addition, Ensembl provides a
mapping from Uniprot identifiers to Ensembl protein IDs. This is however in many
cases an one-to-many mapping, i.e. a single Uniprot ID is assigned to multiple
Ensembl protein IDs. As an additional complication, the coding region might not
be complete for some transcripts and either their 3' or 5' ends (or both) are
not defined (or can not be mapped to the genome). In such cases, the length of
the CDS does not match the length of the annotated protein sequence. Reported
position mappings between proteins and transcripts might for that particular
cases not be correct. In such cases FALSE
is reported in a column named
"cds_ok"
in the results from functions mapping to and from protein
coordinates.
The cdsToTranscript
and transcriptToCds
functions are helpful to enable the
mapping of variants in genes that are usually provided as positions within the
gene's (actually transcript's) coding sequence. An example for such a mapping is
provided in section Mapping transcript coordinates to genomic coordinates
further below.
Below we load all required libraries and filter the EnsDb
database containing
the annotations from Ensembl release 86 to chromosome X. All genes of the
examples in this vignette are encoded on chromosome X and subsetting the EnsDb
to a single chromosome speeds all database queries considerably up.
library(ensembldb) library(EnsDb.Hsapiens.v86) edbx <- filter(EnsDb.Hsapiens.v86, filter = ~ seq_name == "X")
Below we define a genomic region on chromosome X for which we want to identify the transcripts that are eventually encoded by that position and determine the coordinates of the genomic region within these (relative to their first nucleotide).
gnm <- GRanges("X:107716399-107716401")
Before we map the coordinates we visualize the genomic region and all genes and transcripts overlapping it.
library(Gviz) ## Since we're using Ensembl chromosome names we have to set: options(ucscChromosomeNames = FALSE) ## Define a genome axis track gat <- GenomeAxisTrack(range = gnm) ## Get all genes in that region gnm_gns <- getGeneRegionTrackForGviz(edbx, filter = GRangesFilter(gnm)) gtx <- GeneRegionTrack(gnm_gns, name = "tx", geneSymbol = TRUE, showId = TRUE) ## Generate a higlight track ht <- HighlightTrack(trackList = list(gat, gtx), range = gnm) ## plot the region plotTracks(list(ht))
The genomic position overlaps two transcripts of the gene TSC22D3, encoded on
the reverse strand on chromosome X. Below we map this position to the
nucleotides within the encoded transcripts with the genomeToTranscript
function.
## Map genomic coordinates to within-transcript coordinates gnm_tx <- genomeToTranscript(gnm, edbx)
As a result we get an IRangesList
object of length 1 (since we defined a
single genomic region as input). The IRanges
in the first element of our
result object provides the mapped coordinates within each transcript that is
encoded in the specified genomic region.
gnm_tx
The genomic region overlapped two transcripts and the transcript-relative
coordinates for both are reported. The ID of the transcripts are provided as the
names
of the IRanges
. The original genomic coordinates are listed in
additional metadata columns (which can be accessed with the mcols
method). Also the ID of the exon encoded at the genomic region and its
index/rank within the transcript is available in the "exon_id"
metadata
column.
To illustrate mapping of multiple genomic regions, we define below 2 genomic regions: twice the example region from above but once restricting to the reverse and once to the forward strand.
gnm_1 <- gnm strand(gnm_1) <- "-" gnm_2 <- gnm strand(gnm_2) <- "+" gnm <- c(gnm_1, gnm_2) genomeToTranscript(gnm, edbx)
The result for the first region is the same as above. The result for the second
region is an IRanges
with negative coordinates, since there is no transcript
encoded on the forward strand at the genomic position.
We can use the genomeToProtein
function to map genomic coordinates to
within-protein sequence coordinates. In addition to the genomeToTranscript
function, this function determines whether the transcript at the genomic
position encodes a protein, and if so, maps the genomic coordinates to
coordinates within the respective protein sequence. To this end, the
transcript-relative coordinates for the genomic region have to be located within
CDS of the transcript (excluding the stop codon, i.e. last 3 nucleotides of the
CDS, since they are not translated into an amino acid).
Below we define 4 genomic regions and map them to protein-relative coordinates: the first corresponds to the first 4 nucleotides of the CDS of ENST00000381578, the second to the last nucleotide of the CDS of the same transcript. The third region maps to the last nt before the stop codon of ENST00000381578 and the last region is located within an intron of the same transcript.
gnm <- GRanges("X", IRanges(start = c(630898, 644636, 644633, 634829), width = c(5, 1, 1, 3))) gnm_prt <- genomeToProtein(gnm, edbx)
The resulting object has the length 4, one IRanges
for each region in the
input GRanges
. The warning messages indicate that not all of the regions could
be mapped to within-protein coordinates. We explore now the results for each
input region separately.
gnm_prt[[1]]
The genomic region could be mapped to positions within the coding regions of 4
different transcripts, each of them being annotated to its own Ensembl protein
ID. The input region was mapped to the first 4 nucleotides of each transcripts'
CDS and was thus mapped to the amino acid residues 1 and 2 of the encoded
protein: the first 3 nucleotides to the first amino acid, the 4th to the second
amino acid. The encoding transcript ID, the exon ID, exon rank and the input
genomic region are provided as metadata columns in the result IRanges
. A
metadata column cds_ok
provides the additional information whether the length
of each transcripts' CDS matches the length of the encoded protein
sequence. This is an important information, as not all protein coding
transcripts in Ensembl have complete CDS, either because their 3' or their 5'
(or both) ends are incomplete (or could not be mapped/aligned to the
genome). Mappings to or from protein coordinates with a cds_ok
being FALSE
might not be correct and should be manually evaluated e.g. using the Ensembl
genome browser.
The second genomic region maps to last nucleotide of the CDS of ENST00000381578,
which is however part of the stop codon that is not translated. The coordinates
can therefore not be mapped to the protein sequence and an IRanges
with
negative start position is thus returned.
gnm_prt[[2]]
The third region can be mapped to the last nucleotide before the stop codon and was thus mapped to the last amino acid of the encoded protein.
gnm_prt[[3]]
This region maps however to coordinates within two transcripts, each with their own translation. Below we retrieve the protein sequences for both protein IDs to evaluate if it corresponds indeed to the last amino acid for the protein encoded by ENST00000381578.
prt <- proteins(edbx, filter = ProteinIdFilter(names(gnm_prt[[3]]))) nchar(prt$protein_sequence)
As expected, the position mapped to the last amino acid of the amino acid sequence associated with both protein IDs. In fact, these amino acid sequences are identical.
The result for the last region can not be mapped to any transcript-relative
coordinates and hence also not to any protein. As a result, an IRanges
with
negative coordinates is returned.
gnm_prt[[4]]
The proteinToTranscript
method allows to map protein-sequence relative
coordinates to the encoding region in the transcript. A protein identifier and
the coordinates within the protein sequence have to be provided with an
IRanges
object, the protein identifiers (ideally Ensembl protein IDs or also
Uniprot IDs) either provided as names
of the object, or in one of its metadata
columns. The function will first try to find the protein identifiers in the
database and, if found, map the provided coordinates to transcript-relative
positions.
In our first example we retrieve the transcript-relative coordinates of
positions 5 to 9 within the amino acid sequence of the gene GAGE10. Below we
first get the protein ID for this gene from the database and define then the
IRanges
with the protein sequence-internal coordinates.
GAGE10 <- proteins(edbx, filter = ~ genename == "GAGE10") GAGE10 ## Define the IRanges object. GAGE10_prt <- IRanges(start = 5, end = 9, names = GAGE10$protein_id)
Now we use the proteinToTranscript
function to map the coordinates. The
function also compares the length of the CDS with the length of the encoded
protein sequence and, if they are not matching, returns a FALSE
in the result
object's cds_ok
metadata column. In such cases (i.e. when the CDS of the
transcript is incomplete), the returned coordinates could be wrong.
GAGE10_tx <- proteinToTranscript(GAGE10_prt, edbx)
The result is a list
with the same length as the input IRanges
, each element
representing the mapping of the protein-relative coordinates to positions within
all encoding transcripts. Note that the transcript coordinates are relative to
the first nucleotide of the 5' UTR, not of the CDS.
GAGE10_tx
If Ensembl protein identifiers are used, the mapping between protein- and
transcript coordinates will always be 1:1. Many Uniprot identifiers are however
annotated to more than one Ensembl protein ID and the resulting IRanges
for
one input region might thus be of length larger than one. Below we define
regions in protein sequences identified by Uniprot IDs. In addition, to
illustrate a failing mapping, we add a region with an invalid ID.
ids <- c("O15266", "Q9HBJ8", "donotexistant") prt <- IRanges(start = c(13, 43, 100), end = c(21, 80, 100)) names(prt) <- ids prt_tx <- proteinToTranscript(prt, edbx, idType = "uniprot_id")
The region within the first protein with a Uniprot ID can be mapped to 4 different Ensembl protein IDs and the coordinates are thus mapped to regions within 4 transcripts.
prt_tx[[1]]
The Uniprot identifier for the second region can be mapped to a single Ensembl protein ID and we get thus coordinates within a single transcript.
prt_tx[[2]]
The last identifier can not be mapped to any Ensembl protein, and a region with negative coordinates is thus returned.
prt_tx[[3]]
The proteinToGenome
function allows to map coordinates within the amino acid
sequence of a protein to the corresponding DNA sequence on the genome. A protein
identifier and the coordinates of the sequence within its amino acid sequence
are required and have to be passed as an IRanges
object to the function. The
protein identifier can either be passed as names
of this object, or provided
in a metadata column (mcols
).
In our first example we map the positions 5 to 9 within the amino acid sequence of the protein ENSP00000385415 from gene GAGE10 to the genome.
## Define the IRanges object. GAGE10_prt <- IRanges(start = 5, end = 9, names = "ENSP00000385415")
We can now map the protein-relative coordinates to genomic coordinates. By
default, proteinToGenome
assumes the names of the provided
IRanges
object to be Ensembl protein identifiers.
GAGE10_gnm <- proteinToGenome(GAGE10_prt, edbx)
proteinToGenome
returns a list
, one element for each range in the input
IRanges
. We did only map a single range and hence the result is a list
of
length 1. The GRanges
object in the first element of GAGE10_gnm
represents
the coordinates of the DNA sequence encoding positions 5 to 9 in the protein.
GAGE10_gnm
This GRanges
contains also useful additional information as metadata columns,
such as the ID of the encoding transcript (column "tx_id"
) the ID and index of
the exon within the protein region is encoded (columns "exon_id"
and
"exon_rank"
), the start and end coordinates from the input IRanges
object
(columns "protein_start"
and "protein_end"
) and a logical
indicating
whether the length of the encoding transcript's CDS matches the protein sequence
length ("cds_ok"
). Special care should be taken if a FALSE
is reported in
this last column. In such cases the returned genomic coordinates might not be
correct and they should be manually checked using the Ensembl genome browser.
The reason to use a list
as a result object and not, e.g. a GRangesList
, was
the one-to-many mappings between Uniprot identifiers and Ensembl protein IDs. To
illustrate this, we map positions within 3 proteins identified by their Uniprot
identifiers to genomic regions.
## Define the IRanges providing Uniprot IDs. uni_rng <- IRanges(start = c(2, 12, 8), end = c(2, 15, 17), names = c("D6RDZ7", "O15266", "H7C2F2")) ## We have to specify that the IDs are Uniprot IDs uni_gnm <- proteinToGenome(uni_rng, edbx, idType = "uniprot_id")
The length of the protein coding region of the encoding transcript for two of
the 3 proteins (D6RDZ7 and H7C2F2) do not match the length of the protein
sequence. For some transcripts the CDS is not complete (either at the 3', 5' or
both ends). Mapped coordinates might not be correct in such cases and it is
strongly suggested to manually check the mapped coordinates. The result from the
comparison of the protein sequence and the CDS length is provided in the
"cds_ok"
metadata column of the GRanges
with the genomic coordinates.
uni_gnm[[3]]
Mappings between Uniprot and Ensembl protein IDs can be one-to-many. In such
cases proteinToGenome
returns a GRangesList
with each element being the
coordinates calculated for each annotated Ensembl protein. In our example, each
of the first two proteins was annotated to 4 Ensembl proteins.
## To how many Ensembl proteins was each Uniprot ID mapped? lengths(uni_gnm)
Below we show the genomic coordinates for the within-protein positions calculated for all 4 Ensembl protein IDs for O15266.
uni_gnm[["O15266"]]
As a last example we fetch all protein domains for the gene SYP and map all of
them to the genome. To fetch protein domain information we select all columns
from the protein_domain table. In addition, we retrieve the result as a
AAStringSet
. Additional annotations will be available in the mcols
of this
result object.
SYP <- proteins(edbx, filter = ~ genename == "SYP", columns = c("protein_id", "tx_id", listColumns(edbx, "protein_domain")), return.type = "AAStringSet") SYP
Each protein sequence of the gene SYP has multiple protein domains annotated to
it, thus protein IDs and sequences are redundant in the AAStringSet
. We
restrict the result below to a single protein.
## How many proteins are annotated to SYP? unique(mcols(SYP)$protein_id) ## Reduce the result to a single protein SYP <- SYP[names(SYP) == "ENSP00000263233"] ## List the available protein domains and additional annotations mcols(SYP)
Next we create the IRanges
object, one range for each protein domain, and
perform the mapping of the protein domains to the genome. This time we provide
the protein identifiers with one of the metadata columns and pass the name of
this column with the id
parameter.
SYP_rng <- IRanges(start = mcols(SYP)$prot_dom_start, end = mcols(SYP)$prot_dom_end) mcols(SYP_rng) <- mcols(SYP) ## Map the domains to the genome. We set "id" to the name ## of the metadata columns containing the protein IDs SYP_gnm <- proteinToGenome(SYP_rng, edbx, id = "protein_id")
The function mapped each domain to the genome and returned a list
with the
mapping result for each as a GRanges
object. As an example we show the mapping
result for the second protein domain (PF01284).
SYP_gnm[[2]]
The protein domain is encoded by a sequence spanning exons 2 to 5 of the transcript ENST00000263233. Note that the gene is encoded on the reverse strand. The individual ranges are ordered by the index of the respective exon within the transcript.
At last we plot the encoding transcript and all of the mapped protein domains for the protein ENSP00000263233 of SYP.
library(Gviz) ## Define a genome axis track gat <- GenomeAxisTrack() ## Get the transcript ID: txid <- SYP_gnm[[1]]$tx_id[1] ## Get a GRanges for the transcript trt <- getGeneRegionTrackForGviz(edbx, filter = TxIdFilter(txid)) ## Define a GRanges for the mapped protein domains and add ## metadata columns with the grouping of the ranges and the ## IDs of the corresponding protein domains, so they can be ## identified in the plot dmns <- unlist(GRangesList(SYP_gnm)) dmns$grp <- rep(1:length(SYP_rng), lengths(SYP_gnm)) dmns$id <- rep(mcols(SYP_rng)$protein_domain_id, lengths(SYP_gnm)) ## Since we're using Ensembl chromosome names we have to set options(ucscChromosomeNames = FALSE) ## Plotting the transcript and the mapped protein domains. plotTracks(list(gat, GeneRegionTrack(trt, name = "tx"), AnnotationTrack(dmns, group = dmns$grp, id = dmns$id, groupAnnotation = "id", just.group = "above", shape = "box", name = "Protein domains")), transcriptAnnotation = "transcript")
Coordinates within transcript sequences can be mapped to genomic coordinates
with the transcriptToGenome
function. In the example below we map coordinates
within 2 transcript to the genome.
rng_tx <- IRanges(start = c(501, 1), width = c(5, 5), names = c("ENST00000486554", "ENST00000381578")) rng_gnm <- transcriptToGenome(rng_tx, edbx)
The function returns a GRangesList
with the GRanges
in each element
containing the genomic coordinates to which the positions could be mapped (or an
empty GRanges
if the transcript identifier can not be found in the database or
the input range is not within the transcript's sequence). The length of each
GRanges
depends on the number of exons the region in the transcript spans.
rng_gnm
The region in the first transcript (ENST00000486554) is mapped to two genomic regions, because part of it is located in the first, and part in the second exon of the transcript. All 5 nucleotides of the second region are within the transcript's first exon and are thus mapped to only a single genomic region.
Next we map variants in the gene PKP2 to the corresponding genomic
coordinates. The variants are PKP2 c.1643DelG and c.1881DelC and the
positions we are looking for are thus nucleotides 1643 and 1881 within the
CDS of the gene/transcript. Looking up the available transcripts for this
gene we identified ENST00000070846 as the representative transcript for the
gene. Since the positions are not relative to the transcription start site we
can not use the transcriptToGenome
function for the mapping, but we have to
map the cds-relative positions first to transcript-relative coordinates. We do
this below using the cdsToTranscript
function.
## Define the position within the CDS of the transcript pkp2_cds <- IRanges(start = c(1643, 1881), width = c(1, 1), name = rep("ENST00000070846", 2)) ## Convert cds-relative to transcript-relative coordinates pkp2 <- cdsToTranscript(pkp2_cds, EnsDb.Hsapiens.v86) pkp2
With the coordinates being now relative to the first nucleotide of the
transcript we can use the transcriptToGenome
function for the final mapping of
the position to the genome.
pkp2_gnm <- transcriptToGenome(pkp2, EnsDb.Hsapiens.v86) pkp2_gnm
To verify that the nucleotides at the positions are indeed G and C as stated in the definition of the variant (c.1643DelG and c.1881DelC) we extract below the nucleotide at the identified genomic position. We thus load the package providing the genome sequence for GRCh38 on which Ensembl release 86 is based.
library(BSgenome.Hsapiens.NCBI.GRCh38) getSeq(BSgenome.Hsapiens.NCBI.GRCh38, pkp2_gnm)
The transcriptToProtein
function can be used to map coordinates within a
transcript to the corresponding coordinates within the encoded protein. Note
that only regions within protein coding transcripts can be mapped and that
coordinates within the transcript are assumed to be relative to the first
nucleotide of the transcript (not of the CDS).
Below we define regions within several transcripts and map these to the corresponding amino acid residues in the protein.
rng_tx <- IRanges(start = c(501, 1, 200), width = c(5, 5, 4), names = c("ENST00000486554", "ENST00000381578", "ENST00000431238")) rng_prt <- transcriptToProtein(rng_tx, edbx)
The mapping did throw several warnings. The region within transcript ENST00000431238 can not be mapped to protein coordinates, because the transcript does not encode a protein. Transcript ENST00000381578 encodes a protein, but the specified nucleotides 1 to 5 are located in the 5' UTR of the transcript and can therefore also not be mapped. Finally, the CDS of the transcript ENST00000486554 is not complete and, while the coordinates were mapped to protein residues, they might not be correct.
rng_prt
For transcript coordinates that could not be mapped, negative coordinates are
returned (see lines/elements 2 and 3 above). The first region could be mapped,
but the returned protein-relative coordinates might be wrong, because the CDS of
the transcript is incomplete (hence a FALSE
is reported in metadata column
"cds_ok"
). In fact, only the 3' end of the CDS is incomplete for this
transcript and the returned coordinates are thus correct.
sessionInfo()
Add the following code to your website.
For more information on customizing the embed code, read Embedding Snippets.