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getSeq-methods: getSeq method for BSgenome objects

getSeq-methods: getSeq method for BSgenome objects
In Przemol/mirrors-bioc-BSgenome: Infrastructure for Biostrings-based genome data packages

Description Usage Arguments Details Value Note Author(s) See Also Examples

Description

A getSeq method for extracting a set of sequences (or subsequences) from a BSgenome object.

Usage

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## S4 method for signature 'BSgenome'
getSeq(x, names, start=NA, end=NA, width=NA,
                 strand="+", as.character=FALSE)

Arguments

x

A BSgenome object. See the available.genomes function for how to install a genome.

names

A character vector containing the names of the sequences in x where to get the subsequences from, or a GRanges object, or a GRangesList object, or a named RangesList object, or a named Ranges object. The RangesList or Ranges object must be named according to the sequences in x where to get the subsequences from.

If names is missing, then seqnames(x) is used.

See ?`BSgenome-class` for details on how to get the lists of single sequences and multiple sequences (respectively) contained in a BSgenome object.

start, end, width

Vector of integers (eventually with NAs) specifying the locations of the subsequences to extract. These are not needed (and it's an error to supply them) when names is a GRanges, GRangesList, RangesList, or Ranges object.

strand

A vector containing "+"s or/and "-"s. This is not needed (and it's an error to supply it) when names is a GRanges or GRangesList object.

as.character

TRUE or FALSE. Should the extracted sequences be returned in a standard character vector?

...

Additional arguments. (Currently ignored.)

Details

L, the number of sequences to extract, is determined as follow:

If names is neither a GRanges or GRangesList object, then the strand argument is also recycled to length L.

Here is how the names passed to the names argument are matched to the names of the sequences in BSgenome object x. For each name in names:

Value

Normally a DNAStringSet object (or character vector if as.character=TRUE).

With the 2 following exceptions:

  1. A DNAStringSetList object (or CharacterList object if as.character=TRUE) of the same shape as names if names is a GRangesList object.

  2. A DNAString object (or single character string if as.character=TRUE) if L = 1 and names is not a GRanges, GRangesList, RangesList, or Ranges object.

Note

Be aware that using as.character=TRUE can be very inefficient when extracting a "big" amount of DNA sequences (e.g. millions of short sequences or a small number of very long sequences).

Note that the masks in x, if any, are always ignored. In other words, masked regions in the genome are extracted in the same way as unmasked regions (this is achieved by dropping the masks before extraction). See ?`MaskedDNAString-class` for more information about masked DNA sequences.

Author(s)

H. Pages; improvements suggested by Matt Settles and others

See Also

getSeq, available.genomes, BSgenome-class, DNAString-class, DNAStringSet-class, MaskedDNAString-class, GRanges-class, GRangesList-class, RangesList-class, Ranges-class, grep

Examples

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## ---------------------------------------------------------------------
## A. SIMPLE EXAMPLES
## ---------------------------------------------------------------------

## Load the Caenorhabditis elegans genome (UCSC Release ce2):
library(BSgenome.Celegans.UCSC.ce2)

## Look at the index of sequences:
Celegans

## Get chromosome V as a DNAString object:
getSeq(Celegans, "chrV")
## which is in fact the same as doing:
Celegans$chrV

## Not run: 
  ## Never try this:
  getSeq(Celegans, "chrV", as.character=TRUE)
  ## or this (even worse):
  getSeq(Celegans, as.character=TRUE)

## End(Not run)

## Get the first 20 bases of each chromosome:
getSeq(Celegans, end=20)

## Get the last 20 bases of each chromosome:
getSeq(Celegans, start=-20)

## Get the "NM_058280_up_1000" sequence (belongs to the upstream1000
## multiple sequence) as a DNAString object:
s1 <- getSeq(Celegans, "NM_058280_up_1000")
stopifnot(identical(getSeq(Celegans, "NM_058280_up_5000", start=-1000), s1))

## Not run: 
  ## Fails because there is more than one sequence across
  ## Celegans$upstream1000, Celegans$upstream2000 and Celegans$upstream5000
  ## with "NM_058280" in its name:
  getSeq(Celegans, "NM_058280")

  ## Fails because there is no sequence named exactly "NM_058280":
  getSeq(Celegans, "^NM_058280$")

## End(Not run)

## ---------------------------------------------------------------------
## B. EXTRACTING SMALL SEQUENCES FROM DIFFERENT CHROMOSOMES
## ---------------------------------------------------------------------

myseqs <- data.frame(
  chr=c("chrI", "chrX", "chrM", "chrM", "chrX", "chrI", "chrM", "chrI"),
  start=c(NA, -40, 8510, 301, 30001, 9220500, -2804, -30),
  end=c(50, NA, 8522, 324, 30011, 9220555, -2801, -11),
  strand=c("+", "-", "+", "+", "-", "-", "+", "-")
)
getSeq(Celegans, myseqs$chr,
       start=myseqs$start, end=myseqs$end)
getSeq(Celegans, myseqs$chr,
       start=myseqs$start, end=myseqs$end, strand=myseqs$strand)

## ---------------------------------------------------------------------
## C. USING A GRanges OBJECT
## ---------------------------------------------------------------------

gr1 <- GRanges(seqnames=c("chrI", "chrI", "chrM"),
               ranges=IRanges(start=101:103, width=9))
gr1  # all strand values are "*"
getSeq(Celegans, gr1)  # treats strand values as if they were "+"

strand(gr1)[] <- "-"
getSeq(Celegans, gr1)

strand(gr1)[1] <- "+"
getSeq(Celegans, gr1)

strand(gr1)[2] <- "*"
if (interactive())
  getSeq(Celegans, gr1)  # Error: cannot mix "*" with other strand values

gr2 <- GRanges(seqnames=c("chrM", "NM_058280_up_1000"),
               ranges=IRanges(start=103:102, width=9))
gr2
if (interactive()) {
  ## Because the sequence names are supplied via a GRanges object, they
  ## are not treated as regular expressions:
  getSeq(Celegans, gr2)  # Error: sequence NM_058280_up_1000 not found
}

## ---------------------------------------------------------------------
## D. USING A GRangesList OBJECT
## ---------------------------------------------------------------------

gr1 <- GRanges(seqnames=c("chrI", "chrII", "chrM", "chrII"),
               ranges=IRanges(start=101:104, width=12),
               strand="+")
gr2 <- shift(gr1, 5)
gr3 <- gr2
strand(gr3) <- "-"

grl <- GRangesList(gr1, gr2, gr3)
getSeq(Celegans, grl)

## ---------------------------------------------------------------------
## E. EXTRACTING A HIGH NUMBER OF RANDOM 40-MERS FROM A GENOME
## ---------------------------------------------------------------------

extractRandomReads <- function(x, density, readlength)
{
    if (!is.integer(readlength))
        readlength <- as.integer(readlength)
    start <- lapply(seqnames(x),
                    function(name)
                    {
                      seqlength <- seqlengths(x)[name]
                      sample(seqlength - readlength + 1L,
                             seqlength * density,
                             replace=TRUE)
                    })
    names <- rep.int(seqnames(x), elementLengths(start))
    ranges <- IRanges(start=unlist(start), width=readlength)
    strand <- strand(sample(c("+", "-"), length(names), replace=TRUE))
    gr <- GRanges(seqnames=names, ranges=ranges, strand=strand)
    getSeq(x, gr)
}

## With a density of 1 read every 100 genome bases, the total number of
## extracted 40-mers is about 1 million:
rndreads <- extractRandomReads(Celegans, 0.01, 40)

## Notes:
## - The short sequences in 'rndreads' can be seen as the result of a
##   simulated high-throughput sequencing experiment. A non-realistic
##   one though because:
##     (a) It assumes that the underlying technology is perfect (the
##         generated reads have no technology induced errors).
##     (b) It assumes that the sequenced genome is exactly the same as
##         the reference genome.
##     (c) The simulated reads can contain IUPAC ambiguity letters only
##         because the reference genome contains them. In a real
##         high-throughput sequencing experiment, the sequenced genome
##         of course doesn't contain those letters, but the sequencer
##         can introduce them in the generated reads to indicate
##         ambiguous base-calling.
## - Those reads are coming from the plus and minus strands of the
##   chromosomes.
## - With a density of 0.01 and the reads being only 40-base long, the
##   average coverage of the genome is only 0.4 which is low. The total
##   number of reads is about 1 million and it takes less than 10 sec.
##   to generate them.
## - A higher coverage can be achieved by using a higher density and/or
##   longer reads. For example, with a density of 0.1 and 100-base reads
##   the average coverage is 10. The total number of reads is about 10
##   millions and it takes less than 1 minute to generate them.
## - Those reads could easily be mapped back to the reference by using
##   an efficient matching tool like matchPDict() for performing exact
##   matching (see ?matchPDict for more information). Typically, a
##   small percentage of the reads (4 to 5% in our case) will hit the
##   reference at multiple locations. This is especially true for such
##   short reads, and, in a lower proportion, is still true for longer
##   reads, even for reads as long as 300 bases.

## ---------------------------------------------------------------------
## F. SEE THE BSgenome CACHE IN ACTION
## ---------------------------------------------------------------------

options(verbose=TRUE)
first20 <- getSeq(Celegans, end=20)
first20
gc()
stopifnot(length(ls(Celegans@.seqs_cache)) == 0L)
## One more gc() call is needed in order to see the amount of memory in
## used after all the chromosomes have been removed from the cache:
gc()

Przemol/mirrors-bioc-BSgenome documentation built on May 8, 2019, 3:46 a.m.

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