CNEr 1.30.0
Conserved noncoding elements (CNEs) are a pervasive class of elements clustering around genes with roles in development and differentiation in Metazoa (Woolfe et al. 2004). While many have been shown to act as long-range developmental enhancers (Sandelin et al. 2004), the source of their extreme conservation remains unexplained. To study the evolutionary dynamics of these elements and their relationship to the genes around which they cluster, it is essential to be able to produce genome-wide sets of these elements for a large number of species comparisons, each with multiple size and conservation thresholds.
This CNEr package aims to detect CNEs and visualise them along the genome. For performance reasons, the implementation of CNEs detection and corresponding I/O functions are primarily written as C extensions to R. We have used CNEr to produce sets of CNEs by scanning pairwise whole-genome net alignments with multiple reference species, each with two different window sizes and a range of minimum identity thresholds. Then, to pinpoint the boundaries of CNE arrays, we compute the CNE densities as the percentages of length covered by CNEs within a user specified window size. Finally, we describe a novel visualisation method using horizon plot tracks that shows a superior dynamic range to the standard density plots, simultaneously revealing CNE clusters characterized by vastly different levels of sequence conservation. Such CNE density plots generated using precise locations of CNEs can be used to identify genes involved in developmental regulation, even novel genes that are not annotated yet.
This section briefly demonstrates the pipeline of CNE identification and visualisation. More detailed usage of each step is described in following sections with a concise example of CNE identification and visualisation for the “barhl2” and “sox14” (chr6:24,000,000..27,000,000) loci in Zebrafish (danRer10) genome against Human (hg38).
The minimal input for CNEr includes the whole genome pairwise alignment of two assemblies, axt net files. UCSC already provides a set of precomputed axt files on http://hgdownload.soe.ucsc.edu/downloads.html for most of popular genomes. In case the axt net files are not available from UCSC, you can always generate the axt net files by following another vignette “Pairwise whole genome alignment” in this CNEr package.
Another essential information is the annotation of exons and repeats, which could be retrieved from various resources.
During the development of this package, there was no suitable class to store the axt alignments in Bioconductor.
Hence, we created two new S4 classes, Axt
and GRangePairs
, to easily manipulate the axt alignment files.
GRangePairs
is designed to hold a pair of GRanges
objects, which have the same length.
It builds on the Pairs
class of Bioconductor and inherits many useful methods from it.
This Axt
class inherits from GRangePairs
with no extra slots to hold the content from axt files, but many specific methods are created for Axt
.
The ranges of the target and the query organism are stored in two GRanges
objects with alignment sequences as metadata columns.
The Blastz scores and the widths of the alignments are stored in metadata columns of GRangePairs
.
For more information on the usage of these two classes, please refer to the documentation.
To read axt file into R,
CNEr provides readAxt
function for highly efficient reading.
This function is built on a backend C code of Kent’s utilities (W J Kent et al. 2002).
The axt alignment files can be either gzippped or in plain text file.
The alignments between two genomes can also be in one big file or in several files, such as “chr1.hg19.mm10.net.axt.gz”, “chr2.hg19.mm10.net.axt.gz”, etc.
library(CNEr)
## These axt files are specially prepared for the region
## (chr6:24,000,000..27,000,000)
axtFilesHg38DanRer10 <- file.path(system.file("extdata", package="CNEr"),
"hg38.danRer10.net.axt")
axtFilesDanRer10Hg38 <- file.path(system.file("extdata", package="CNEr"),
"danRer10.hg38.net.axt")
axtHg38DanRer10 <- readAxt(axtFilesHg38DanRer10)
## The number of axt files 1
## The number of axt alignments is 50
axtDanRer10Hg38 <- readAxt(axtFilesDanRer10Hg38)
## The number of axt files 1
## The number of axt alignments is 352
## Axt class is shown in UCSC axt format
axtHg38DanRer10
## A Axt with 50 alignment pairs:
## 1 chr1 148165963 148166304 chr6 25825774 25826099 + 5310
## TCTCTCCCATCCCAACTGTTCTAAATGT-TCTTCCATTT...GCAGCTCTTTTCCAACCAAAACAACAGAAATTAAACTT
## TTTCTCTCCTGCTAGGTTTTATAAGAGTGTTTTTCAGTT...TCGGGTGCCTTTTCAGAGTAATGAGGGAAATTAAATTT
## 2 chr1 222131480 222131835 chr6 24819722 24820074 + 221
## CTTAATGTCTTTCTATCCAAAGTCATGCATTATATGTTA...TAATTGTGTTTAATATTTTTAATTAAATGGTCCTTTTA
## TTCGAATTTTTATTATTAAGATTCAAATATTATG-ATTG...TTACTGTATGTAACAGCATTTATTAAACTGTGTTATCA
## 3 chr10 65322021 65322919 chr6 26227619 26228468 + 946
## TTGCACTTTGAAGCCCAAACTTAGCAATAAATAAAAATA...TCTGTTACATTGAGCCATTTGTCTCACTTTTCATTAAT
## TTGTTTTTAAAAGACTAAATTTAACAATAAACTTAAATG...TTTTGAAAAGTAATTTTTTTGTATTTATATTCATTCAT
## 4 chr13 94750629 94751259 chr6 26600600 26601208 + 3302
## GCCTTCCCAGTTTCTCC-ACTCTCCCTCATTTTTTTCCC...GTCATAATATA---CATTTTTAAAATTAATTATCCATT
## GCTTTATCAGACTCTCCTAATGTCACCC---TCTCTCTC...GCCAAAAGATAGGGCATTCTAAAACTGTGTCACCCACT
## 5 chr13 94966940 94966991 chr6 26745445 26745499 + 711
## ATTCAGCTCTAAAGCACCTTTGACTTCTA---TTTCATTTTTTATTTTCCACTCA
## AGCCAGCGTGTATACCTAGCTGACATTTAGGTTTTTTTTTTTTTTTTGCCATTTA
## ... ... ... ... ... ... ... ...
## 46 chr6 61961895 61962455 chr6 24832605 24833189 + -3626
## AAACGGGATCATTCTGGCAG---CTGTGTTTAAAA----...TTTCAGTAGTTCCCAATCTATGGGCTGCACACTCTAAG
## AAAGGAAATAATTGTTGAAAGTACTGAATTTAAAGAAAT...ATTTATCTGTTTTGAACAAAT----TTAACA----AAA
## 47 chr6 131822466 131822664 chr6 25067163 25067383 + 1420
## AAAAATACTATCTATTGCAAA-----AAATTCAGAAAAT...CCTTT-----TTTCATTTATATTCCATTATGAAAGTTT
## AAATAGGCTATATATGTCATACTTTTAAACTTTTACAAA...TCTTTTTTTCTTTCATTTATGACATATTATAGTATTTT
## 48 chr7 16091079 16091261 chr6 24823861 24824043 + 1243
## TACAATTTAAAAACAGAAA-AGAAGGAAATGACATCTGT...AACACAAGACAAAAAGACAAAATATCACCTGGTGACAG
## TGCAATTTAAAAGTATAAATAAACAGACAATTTATCTAT...AAATAATGATATATAAACAAAATGTGACCTAATAACAG
## 49 chr8 111351278 111351934 chr6 25339132 25339742 + 3524
## TATAGCAGTGTGAAAATGAACTAATACACATACAA--AA...AGAAATAAAGATAGTATTTGAAGTTTAAACAGAGGAAG
## TATTATATTTGGGAACAGAACCAACAAAATTATGATGAT...ATTAATTAAAATAATATTTAAAATGAACAGATAGAAAG
## 50 chr8 111354557 111354869 chr6 25340098 25340413 + 722
## TTCTGATAAAC---TTCAGGGTTCCCATCTCAAGATCAA...AAAGGACAAATAAATAGGTGCTGAAGAGAAAAGCTAGA
## TGCTGATTAGCGCTCTCACGTTGCCTGCCATGAGATTAA...GAAGAAAAAATAAAGAGTGTCTGAAAGGAAAAACTAAA
axtDanRer10Hg38
## A Axt with 352 alignment pairs:
## 1 chr6 24000620 24001357 chr7 146767015 146767753 - -4315
## GCGGATTTATGTAGAAAGATTTTTGGGAGTATCATAAAT...AGAGCCACAATTCTCATTCAGCTATGTGTAGGGTTATT
## GAGGGCCAGTCTGGAAAGCTAACTAGGAGGATGCCAAAA...GAGAAAGGGATTCATAATGGAAACTGAGGGAGCTGCTT
## 2 chr6 24001358 24001524 chr9 17091651 17091817 - 8118
## ACCTTGTATTTAATTCCAGTTTTAAAATAGCCAAGGAAG...CCACTTTCATCCTGAGAACACTCATTACCTGCAGTTCA
## ACCTTGTACTTCAGGCCAGACTTGAAGTAGCCTAGGAAG...CCGCTCTCATCCTGGCTGCACTCATTGCCTACGGGACA
## 3 chr6 24001525 24001683 chr7 146767937 146768119 - -142
## AACA------GACACAGAGTATTG----CCAATATCTCA...---ACAGTACTTCTGTCAGTCTTATTTCTTTTATTTTG
## ATTATCAAGCAAGAGAAAGGATTAAGGCAGAATTTCTGA...TAATTAACAATTTTTTTAGTCTATTTTTTTTTTTTTTG
## 4 chr6 24001998 24002188 chr9 17092546 17092748 - 5826
## CTCACCCAGCCACATATGGACATTATAGGACGGAG----...ACCTGCATTCTGGAACTCCTTGTGAAAAACCATGATTC
## CTCACCCAGCCAGTAGTGGAGGTCATACTGCAGATTTCC...CCCTGCCTTGAGGAACTCGGGGTGTTCCACCACCATGC
## 5 chr6 24052977 24053618 chr1 156772050 156772641 - 15004
## AACAAAAGGAAGAAAGGGATAACCCTGTCCAG---TTCT...ATCCTTATGTGGGCTTAAAAAAAAAAAACACACTGGAA
## AAAAAATAAAGGAGTGGCATAAATTTTTCCAAAATGTTA...GTACCCTCAGAGTTTTGTAGAATATTAACACAATATAA
## ... ... ... ... ... ... ... ...
## 348 chr6 26901575 26901753 chr2 241264446 241264624 + 5495
## ACCTGGGTGATGATTGAGGACTTCAGAGGTTTAATCTTA...ACACTGCTAGGGTCTCCTCCTGCAGCAGCTAATGAAGA
## ACCTGAGTGATGACAGAAGCCTTGATGGGTCGGATCTTG...GAATT--TAGAGTGGCA-ACTGGACCAGCCAACACAGA
## 349 chr6 26901818 26902021 chr2 241266790 241266977 + 4753
## TCACCTTTGACCTGCTCTGGCAGTAAGCCACTGCGATGC...ACAACGTTCGGCATATTTGTAAAGTTACAACCATAAAA
## TCACCTTTGATTTGTTGCGGAACCAGCCCACTTCGGTGT...ACAACCCTCAAT-TATCTATGAGATTGTTAACCTAAGA
## 350 chr6 26903886 26904002 chr2 241268465 241268573 + 4643
## GGTCAATCTTACCAGCTAAATGGTCAGTTACCAGATAAT...TTTGCCTAAAAACAAAACAGTAAATAAGAGAAGAAAAA
## GGTCAAACTTACCAGCAAAACGGTCAGTAGCCAGAAGGT...TTTGCT--GGTATGGGATGGGAAGTGGGAGAGGAGAGA
## 351 chr6 26996747 26997678 chr6 108023708 108024516 - 1325
## ATTGTAAATAATACACTGTGCATTACAAATGCATATCAT...TATTTCTTGTAGTCAAAAGCGGATGGGCAACTTCTTCT
## ATTATATATTATATATTGTACTACATATACATATATTAT...TATTTCTTG----CAATATCATATGCAAAATTCCTTAT
## 352 chr6 26999619 26999997 chr6 108026981 108027383 - 579
## TTTTTAACTGACAAGTGACACCAAGAATATTAAT-----...CTGCTGGCCATCTGTTTTTGAGTTTGCCAATCCAGCTT
## TTTCTGAGTCGCAAATAAAAAATAAAATATAAATGGGAA...CAGTTAACTATCTTTGGTTGGCTTAATGAATCCAGTTT
## Distribution of matched alignments; Given an Axt alignment, plot a heatmap with percentage of each matched alignment
matchDistribution(axtHg38DanRer10)
matchDistribution(axtDanRer10Hg38)
## Example of chr4 on hg19 and galGal3
## The synteny of human and zebrafish is not quite obvious on the dotplot.
library(BSgenome.Hsapiens.UCSC.hg19)
library(BSgenome.Ggallus.UCSC.galGal3)
fn <- file.path(system.file("extdata", package="CNEr"),
"chr4.hg19.galGal3.net.axt.gz")
axt <- readAxt(fn,
tAssemblyFn=file.path(system.file("extdata",
package="BSgenome.Hsapiens.UCSC.hg19"),
"single_sequences.2bit"),
qAssemblyFn=file.path(system.file("extdata",
package="BSgenome.Ggallus.UCSC.galGal3"),
"single_sequences.2bit"))
## The number of axt files 1
## The number of axt alignments is 14411
library(GenomeInfoDb)
syntenicDotplot(axt, firstChrs=c("chr4"), secondChrs="chr4", type="dot")
There are methods defined for handling Axt
objects, including subsetting, output to axt files.
More details can be found in the man page.
The gene annotation information, including exons and repeats, is used to filter out the undesired regions. Here we summarise a table of filtering information we used:
Assembly | Name | Exon | Repeat |
---|---|---|---|
hg38 | Human | RefSeq Genes, Ensembl Genes, UCSC Known Genes | RepeatMasker |
mm10 | Mouse | RefSeq Genes, Ensembl Genes, UCSC Known Genes | RepeatMasker |
xenTro3 | Frog | RefSeq Genes, Ensembl Genes | RepeatMasker |
tetNig2 | Tetraodon | Ensembl Genes | |
canFam3 | Dog | RefSeq Genes, Ensembl Genes | RepeatMasker |
galGal4 | Chicken | RefSeq Genes, Ensembl Genes | RepeatMasker |
danRer10 | Zebrafish | RefSeq Genes, Ensembl Genes | RepeatMasker |
fr3 | Fugu | RefSeq Genes | RepeatMasker |
anoCar2 | Lizard | Ensembl Genes | RepeatMasker |
equCab2 | Horse | RefSeq Genes, Ensembl Genes | RepeatMasker |
oryLat2 | Medaka | RefSeq Genes, Ensembl Genes | RepeatMasker |
monDom5 | Opossum | RefSeq Genes, Ensembl Genes | RepeatMasker |
gasAcu1 | Stickleback | RefSeq Genes, Ensembl Genes | RepeatMasker |
rn5 | Rat | RefSeq Genes, Ensembl Genes | RepeatMasker |
dm3 | D. melanogaster | RefSeq Genes, Ensembl Genes | RepeatMasker |
droAna2 | D. ananassae | RepeatMasker | |
dp3 | D. pseudoobscura | RepeatMasker | |
ce4 | C. elegans | RefSeq Genes | RepeatMasker |
cb3 | C. briggsae | RepeatMasker | |
caeRem2 | C. remanei | RepeatMasker | |
caePb1 | C. brenneri | RepeatMasker |
For the sake of simplicity, all the information listed above can be fetched easily with Bioconductor package rtracklayer, biomaRt and precompiled Bioconductor annotation packages. A few examples are given here:
## To fetch rmsk table from UCSC
library(rtracklayer)
mySession <- browserSession("UCSC")
genome(mySession) <- "hg38"
hg38.rmsk <- getTable(ucscTableQuery(mySession, track="RepeatMasker",
table="rmsk"))
hg38.rmskGRanges <- GRanges(seqnames=hg38.rmsk$genoName,
## The UCSC coordinate is 0-based.
ranges=IRanges(start=hg38.rmsk$genoStart+1,
end=hg38.rmsk$genoEnd),
strand=hg38.rmsk$strand)
## To fetch ensembl gene exons from BioMart
library(biomaRt)
ensembl <- useMart(biomart="ENSEMBL_MART_ENSEMBL",
host="dec2015.archive.ensembl.org")
ensembl <- useDataset("hsapiens_gene_ensembl",mart=ensembl)
attributes <- listAttributes(ensembl)
exons <- getBM(attributes=c("chromosome_name", "exon_chrom_start",
"exon_chrom_end", "strand"),
mart=ensembl)
exonsRanges <- GRanges(seqnames=exons$chromosome_name,
ranges=IRanges(start=exons$exon_chrom_start,
end=exons$exon_chrom_end),
strand=ifelse(exons$strand==1L, "+", "-")
)
seqlevelsStyle(exonsRanges) <- "UCSC"
## Use the existing Bioconductor annotation package for hg38
library(TxDb.Hsapiens.UCSC.hg38.knownGene)
exonsRanges <- exons(TxDb.Hsapiens.UCSC.hg38.knownGene)
The regions to filter out can also be provided in a bed file.
To import the bed file into GRanges in R
,
rtracklayer provides a general function
import.bed
to do that.
Since only the chromosome names, start and end coordinates are used in CNEr,
we provide a more efficient readBed
function.
## Existing bed file for chr6:24,000,000..27,000,000 of Zebrafish danRer10
bedDanRer10Fn <- file.path(system.file("extdata", package="CNEr"),
"filter_regions.danRer10.bed")
danRer10Filter <- readBed(bedDanRer10Fn)
danRer10Filter
## GRanges object with 5996 ranges and 0 metadata columns:
## seqnames ranges strand
## <Rle> <IRanges> <Rle>
## [1] chr6 24000008-24000253 +
## [2] chr6 24000254-24000332 +
## [3] chr6 24000499-24000550 +
## [4] chr6 24000554-24000670 +
## [5] chr6 24000671-24000722 +
## ... ... ... ...
## [5992] chr6 26998029-26998373 +
## [5993] chr6 26998414-26998431 +
## [5994] chr6 26998432-26998526 +
## [5995] chr6 26998687-26998833 +
## [5996] chr6 26999116-26999802 +
## -------
## seqinfo: 1 sequence from an unspecified genome; no seqlengths
## Existing bed file for alignment region in Human hg38 against
## chr6:24,000,000..27,000,000 of danRer10
bedHg38Fn <- file.path(system.file("extdata", package="CNEr"),
"filter_regions.hg38.bed")
hg38Filter <- readBed(bedHg38Fn)
hg38Filter
## GRanges object with 413 ranges and 0 metadata columns:
## seqnames ranges strand
## <Rle> <IRanges> <Rle>
## [1] chr1 26817474-26819341 +
## [2] chr1 156772018-156772158 +
## [3] chr1 156772160-156772358 +
## [4] chr1 156772495-156772637 +
## [5] chr1 156774135-156774472 +
## ... ... ... ...
## [409] chr9 134045293-134045421 +
## [410] chr9 134048002-134048454 +
## [411] chr9 134051562-134051709 +
## [412] chr9 134052306-134052443 +
## [413] chr9 134053265-134053590 +
## -------
## seqinfo: 17 sequences from an unspecified genome; no seqlengths
CNE
classWe designed a CNE
class to store all metadata of running the pipeline for identifying a set of CNEs between two species, including the intermediate and final results.
CNE
can be created by providing the paths of the twoBit files of two assemblies, and
the paths of axt files, with each assembly as reference.
## Here we have the twoBit files from Bioconductor package
## BSgenome.Drerio.UCSC.danRer10 and BSgenome.Hsapiens.UCSC.hg38
cneDanRer10Hg38 <- CNE(
assembly1Fn=file.path(system.file("extdata",
package="BSgenome.Drerio.UCSC.danRer10"),
"single_sequences.2bit"),
assembly2Fn=file.path(system.file("extdata",
package="BSgenome.Hsapiens.UCSC.hg38"),
"single_sequences.2bit"),
axt12Fn=axtFilesDanRer10Hg38, axt21Fn=axtFilesHg38DanRer10,
cutoffs1=8L, cutoffs2=4L)
cneDanRer10Hg38
## An object of class "CNE"
## Slot "assembly1Fn":
## [1] "/home/biocbuild/bbs-3.14-bioc/R/library/BSgenome.Drerio.UCSC.danRer10/extdata/single_sequences.2bit"
##
## Slot "assembly2Fn":
## [1] "/home/biocbuild/bbs-3.14-bioc/R/library/BSgenome.Hsapiens.UCSC.hg38/extdata/single_sequences.2bit"
##
## Slot "axt12Fn":
## [1] "/tmp/Rtmp6K3T4P/Rinst3725642c4caf49/CNEr/extdata/danRer10.hg38.net.axt"
##
## Slot "axt21Fn":
## [1] "/tmp/Rtmp6K3T4P/Rinst3725642c4caf49/CNEr/extdata/hg38.danRer10.net.axt"
##
## Slot "window":
## [1] 50
##
## Slot "identity":
## [1] 50
##
## Slot "CNE12":
## GRangePairs object with 0 pairs and 0 metadata columns:
## first second
## <GRanges> <GRanges>
##
## Slot "CNE21":
## GRangePairs object with 0 pairs and 0 metadata columns:
## first second
## <GRanges> <GRanges>
##
## Slot "CNEMerged":
## GRangePairs object with 0 pairs and 0 metadata columns:
## first second
## <GRanges> <GRanges>
##
## Slot "CNEFinal":
## GRangePairs object with 0 pairs and 0 metadata columns:
## first second
## <GRanges> <GRanges>
##
## Slot "aligner":
## [1] "blat"
##
## Slot "cutoffs1":
## [1] 8
##
## Slot "cutoffs2":
## [1] 4
Note: the order of assemblies when creating CNE object is important.
Here we have danRer10 as assembly1 and hg38 as assembly2.
Then the axt12Fn
contains the axt alignment with assembly1 danRer10 as reference and axt21Fn
contains the alignment with assembly2 hg38 as reference.
The cutoffs1
and cutoffs2
are the maximal number of hits during the realignment in later steps.
Because zebrafish has undergone additional whole genome duplication compared to human, the cutoffs of zebrafish also doubles the cutoffs of human.
In this section, we will go through the details of CNE identification.
Detecting CNEs highly relies on the whole-genome pairwise net alignments. To correct the bias of a chosen genome (which bias?) and capture the duplicated CNEs during genome evolution, we scan two sets of nets for each pairwise comparison, one as reference from each of the genomes.
We identify CNEs by scanning the alignments for regions with at least I identities over C alignment columns. Because different genes and loci may favor various similarity scores, we usually scan at two diffrent window sizes 30 and 50 with several similarity criterias (I/C) range from 70% to 100%.
identities <- c(45L, 48L, 49L)
windows <- c(50L, 50L, 50L)
## Here danRer10Filter is tFilter since danRer10 is assembly1
cneListDanRer10Hg38 <- ceScan(x=cneDanRer10Hg38, tFilter=danRer10Filter,
qFilter=hg38Filter,
window=windows, identity=identities)
## The number of axt files 1
## The number of axt alignments is 352
## The number of axt files 1
## The number of axt alignments is 50
At this stage, a list of CNE
is returned from ceScan
, which contains the preliminary two sets of CNEs from a pair of axt alignments.
We can examine the intermediate CNEs by
## CNEs from the alignments with danRer10 as reference
CNE12(cneListDanRer10Hg38[["45_50"]])
## GRangePairs object with 74 pairs and 2 metadata columns:
## first second | score
## <GRanges> <GRanges> | <numeric>
## [1] chr6:26746284-26746334:+ chr3:137269941-137269991:+ | 90.20
## [2] chr6:26745047-26745455:+ chr3:137264717-137265124:+ | 95.11
## [3] chr6:26708061-26708129:+ chr3:137294941-137295008:- | 91.30
## [4] chr6:26699009-26699078:+ chr3:137329801-137329870:- | 92.86
## [5] chr6:26699080-26699274:+ chr3:137329608-137329799:- | 90.26
## ... ... ... . ...
## [70] chr6:24605694-24605830:+ chr1:90841095-90841232:- | 92.75
## [71] chr6:24605831-24605936:+ chr1:90840976-90841082:- | 90.65
## [72] chr6:24606573-24606626:+ chr1:90840328-90840381:- | 90.74
## [73] chr6:24599740-24599806:+ chr1:90856700-90856765:- | 92.54
## [74] chr6:24580009-24580099:+ chr1:90944046-90944137:- | 90.22
## cigar
## <character>
## [1] 51M
## [2] 218M1I190M
## [3] 47M1I21M
## [4] 70M
## [5] 82M1I96M2I14M
## ... ...
## [70] 128M1D9M
## [71] 99M1D7M
## [72] 54M
## [73] 33M1I33M
## [74] 12M1D79M
## CNEs from the alignments with hg38 as reference
CNE21(cneListDanRer10Hg38[["45_50"]])
## GRangePairs object with 4 pairs and 2 metadata columns:
## first second | score
## <GRanges> <GRanges> | <numeric>
## [1] chr3:137523038-137523102:+ chr6:26638744-26638808:+ | 87.69
## [2] chr3:137523122-137523187:+ chr6:26638826-26638891:+ | 89.39
## [3] chr3:137269941-137269991:+ chr6:26746284-26746334:+ | 90.20
## [4] chr3:137264717-137265124:+ chr6:26745047-26745455:+ | 95.11
## cigar
## <character>
## [1] 65M
## [2] 66M
## [3] 51M
## [4] 218M1D190M
In the result table, even though the strand for query element can be negative, the coordinate for that query element is already on the positive strand.
It is essential to scan two sets of pairwise net alignments with each assembly as reference, in order not to miss any duplicated elements in either lineage. This is particularly important for the comparison between teleost fishes and other vertebrates, because one (for instance, the case of zebrafish) or two (the case of common carp) extra whole genome duplications occured.
As we perform two rounds of CNE detection with each genome as reference, some conserved elements overlap on both genomes and should be removed. Elements, however, that overlap only on one of the genomes are kept, so that duplicated elements remain distinct.
cneMergedListDanRer10Hg38 <- lapply(cneListDanRer10Hg38, cneMerge)
Some CNEs might be unannotated repeats. To remove them, currently we use blat (W James Kent 2002) to realign each sequence of CNEs against the respective genomes. When the number of matches exceeds a certain threshold, for instance 8, that CNE will be discarded.
This step can be very time-consuming when the number of CNEs is large. Other alignment methods could also be considered, for example Bowtie2 or BWA (provided that they are installed on the user’s machine)
cneFinalListDanRer10Hg38 <- lapply(cneMergedListDanRer10Hg38, blatCNE)
As the computation of CNEs from the whole pipeline and the preparation of annotation package can be very time-consuming, for a smoother visualisation experience, we decided to use a local SQLite database in order to store CNEs.
Since the CNEs data.frame
is a table, it can be imported into a SQL table.
To speed up the query from the SQL database,
the bin indexing system is adopted.
For more information, please refer to the paper (W J Kent et al. 2002)
and genomewiki.
## on individual tables
dbName <- tempfile()
data(cneFinalListDanRer10Hg38)
tableNames <- paste("danRer10", "hg38", names(cneFinalListDanRer10Hg38),
sep="_")
for(i in 1:length(cneFinalListDanRer10Hg38)){
saveCNEToSQLite(cneFinalListDanRer10Hg38[[i]], dbName, tableNames[i],
overwrite=TRUE)
}
When querying results from the local SQLite database based on the chr,
coordinates and other criterias,
a GRanges
object is returned.
chr <- "chr6"
start <- 24000000L
end <- 27000000L
minLength <- 50L
tableName <- "danRer10_hg38_45_50"
fetchedCNERanges <- readCNERangesFromSQLite(dbName, tableName, chr,
start, end, whichAssembly="first",
minLength=minLength)
fetchedCNERanges
## GRangePairs object with 70 pairs and 0 metadata columns:
## first second
## <GRanges> <GRanges>
## [1] chr6:26708061-26708129 chr3:137294941-137295008
## [2] chr6:26699009-26699078 chr3:137329801-137329870
## [3] chr6:26699080-26699274 chr3:137329608-137329799
## [4] chr6:26688342-26688673 chr3:137406806-137407138
## [5] chr6:26677966-26678081 chr3:137467520-137467634
## ... ... ...
## [66] chr6:24580009-24580099 chr1:90944046-90944137
## [67] chr6:26638744-26638808 chr3:137523038-137523102
## [68] chr6:26638826-26638891 chr3:137523122-137523187
## [69] chr6:26746284-26746334 chr3:137269941-137269991
## [70] chr6:26745047-26745455 chr3:137264717-137265124
As the lengths of CNEs (Salerno, Havlak, and Miller 2006) and the distances between consecutive elements (Polychronopoulos, Sellis, and Almirantis 2014) exhibit power-law distributions, we implemented a function that might be useful in showing interesting patterns in the distribution of the identified elements.
dbName <- file.path(system.file("extdata", package="CNEr"),
"danRer10CNE.sqlite")
tAssemblyFn <- file.path(system.file("extdata",
package="BSgenome.Drerio.UCSC.danRer10"),
"single_sequences.2bit")
qAssemblyFn <- file.path(system.file("extdata",
package="BSgenome.Hsapiens.UCSC.hg38"),
"single_sequences.2bit")
cneGRangePairs <- readCNERangesFromSQLite(dbName=dbName,
tableName="danRer10_hg38_45_50",
tAssemblyFn=tAssemblyFn,
qAssemblyFn=qAssemblyFn)
plotCNEWidth(cneGRangePairs)
CNEs tend to form clusters. A quick check of the genomic distribution of CNEs is available.
plotCNEDistribution(first(cneGRangePairs))
For visualisation in other Genome Browser, we provide functions to generate the CNE in bed files and CNE density in bedGraph files. For example, to get the first 1000 coordinates of CNEs:
makeCNEDensity(cneGRangePairs[1:1000])
To visualise CNEs alongside other gene annotations, we choose to use the Bioconductor package Gviz in this vignette. Gviz, based on the grid graphics scheme, is a very powerful package for plotting data and annotation information along genomic coordinates. The functionality of integrating publicly available genome annotation data, such as UCSC or Ensembl, significantly reduced the burden of preparing annotations for common assemblies. Since the Bioconductor release 2.13 of Gviz, it provides the data track in horizon plot, which exactly meets our needs for visualisation of CNEs density plots. For more detailed usage, please check the vignette or manual of Gviz.
Another option for visualisation is the package ggbio,
which is based on ggplot2.
The advantage of ggbio is the simplicity of
adding any customised ggplot2 style track
into the plot without tuning the coordinate systems.
The densities generated in the following section can be easily plot in the
horizon plot.
A short straightforward tutorial regarding horizon plot
in ggplot2
format
is available from
http://timelyportfolio.blogspot.co.uk/2012/08/horizon-on-ggplot2.html.
For the example case of hg38 vs danRer10 in this vignette, we choose danRer10 as the reference and show the range of developmental gene barhl2 and sox14.
library(Gviz)
library(biomaRt)
genome <- "danRer10"
axisTrack <- GenomeAxisTrack()
cpgIslands <- UcscTrack(genome=genome, chromosome=chr,
track="cpgIslandExt", from=start, to=end,
trackType="AnnotationTrack", start="chromStart",
end="chromEnd", id="name", shape="box",
showId=FALSE,
fill="#006400", name="CpG",
background.title="brown")
refGenes <- UcscTrack(genome=genome, chromosome=chr,
track="refGene", from=start, to=end,
trackType="GeneRegionTrack", rstarts="exonStarts",
rends="exonEnds", gene="name2", symbol="name2",
transcript="name", strand="strand", fill="#8282d2",
name="refSeq Genes", collapseTranscripts=TRUE,
showId=TRUE, background.title="brown")
ensembl <- useMart(biomart="ENSEMBL_MART_ENSEMBL",
host="dec2015.archive.ensembl.org")
ensembl <- useDataset("drerio_gene_ensembl",mart=ensembl)
biomTrack <- BiomartGeneRegionTrack(genome=genome, chromosome=chr,
biomart=ensembl,
start=start , end=end, name="Ensembl Genes")
library(Gviz)
plotTracks(list(axisTrack, cpgIslands, refGenes),
collapseTranscripts=TRUE, shape="arrow",
transcriptAnnotation="symbol")
It is also possible to plot the annotation from an ordinary R
object,
such as data.frame
, GRanges
, IRanges
or even from a local file.
Usually the gff file containing the gene annotation can be processed by
Gviz directly.
For more details, please look into the vignette of Gviz.
dbName <- file.path(system.file("extdata", package="CNEr"),
"danRer10CNE.sqlite")
genome <- "danRer10"
windowSize <- 200L
minLength <- 50L
cneDanRer10Hg38_21_30 <-
CNEDensity(dbName=dbName,
tableName="danRer10_hg38_21_30",
whichAssembly="first", chr=chr, start=start,
end=end, windowSize=windowSize,
minLength=minLength)
cneDanRer10Hg38_45_50 <-
CNEDensity(dbName=dbName,
tableName="danRer10_hg38_45_50",
whichAssembly="first", chr=chr, start=start,
end=end, windowSize=windowSize,
minLength=minLength)
cneDanRer10Hg38_49_50 <-
CNEDensity(dbName=dbName,
tableName="danRer10_hg38_49_50",
whichAssembly="first", chr=chr, start=start,
end=end, windowSize=windowSize,
minLength=minLength)
cneDanRer10AstMex102_48_50 <-
CNEDensity(dbName=dbName,
tableName="AstMex102_danRer10_48_50",
whichAssembly="second", chr=chr, start=start,
end=end, windowSize=windowSize,
minLength=minLength)
cneDanRer10CteIde1_75_75 <-
CNEDensity(dbName=dbName,
tableName="cteIde1_danRer10_75_75",
whichAssembly="second", chr=chr, start=start,
end=end, windowSize=windowSize,
minLength=minLength)
dTrack1 <- DataTrack(range=cneDanRer10Hg38_21_30,
genome=genome, type="horiz",
horizon.scale=max(cneDanRer10Hg38_21_30$score)/3,
fill.horizon=c("#B41414", "#E03231", "#F7A99C",
"yellow", "orange", "red"),
name="human 21/30", background.title="brown")
dTrack2 <- DataTrack(range=cneDanRer10Hg38_45_50,
genome=genome, type="horiz",
horizon.scale=max(cneDanRer10Hg38_45_50$score)/2,
fill.horizon=c("#B41414", "#E03231", "#F7A99C",
"yellow", "orange", "red"),
name="human 45/50", background.title="brown")
dTrack3 <- DataTrack(range=cneDanRer10Hg38_49_50,
genome=genome, type="horiz",
horizon.scale=max(cneDanRer10Hg38_21_30$score)/3,
fill.horizon=c("#B41414", "#E03231", "#F7A99C",
"yellow", "orange", "red"),
name="human 49/50", background.title="brown")
dTrack4 <- DataTrack(range=cneDanRer10AstMex102_48_50,
genome=genome, type="horiz",
horizon.scale=max(cneDanRer10Hg38_21_30$score)/3,
fill.horizon=c("#B41414", "#E03231", "#F7A99C",
"yellow", "orange", "red"),
name="blind cave fish 48/50", background.title="brown")
dTrack5 <- DataTrack(range=cneDanRer10CteIde1_75_75,
genome=genome, type="horiz",
horizon.scale=max(cneDanRer10CteIde1_75_75$score)/3,
fill.horizon=c("#B41414", "#E03231", "#F7A99C",
"yellow", "orange", "red"),
name="grass carp 75/75", background.title="brown")
ht <- HighlightTrack(trackList=list(refGenes, dTrack5, dTrack4,
dTrack1, dTrack2, dTrack3),
start=c(24200000, 25200000, 26200000),
end=c(25100000, 26150000, 27000000),
chromosome =chr)
plotTracks(list(axisTrack, cpgIslands, ht),
collapseTranscripts=TRUE, shape="arrow",
transcriptAnnotation="symbol",
from=24000000, to=27000000)
From this horizon plot and when comparing Zebrafish with Human as a reference genome, we notice that the genes barhl2, lmo4b and sox14 are surrounded by the density peaks of CNEs.
CNEr efficiently identifies CNEs
and handles the corresponding objects conveniently in R.
Horizon plot shows a superior dynamic range to the standard density plots,
simultaneously revealing CNE clusters characterized
by vastly different levels of sequence conservation.
Such CNE density plots generated using precise locations of CNEs
can be used to identify genes involved in developmental regulation,
even for novel genes that are not yet annotated.
The following is the session info that generated this vignette:
sessionInfo()
## R version 4.1.1 (2021-08-10)
## Platform: x86_64-pc-linux-gnu (64-bit)
## Running under: Ubuntu 20.04.3 LTS
##
## Matrix products: default
## BLAS: /home/biocbuild/bbs-3.14-bioc/R/lib/libRblas.so
## LAPACK: /home/biocbuild/bbs-3.14-bioc/R/lib/libRlapack.so
##
## locale:
## [1] LC_CTYPE=en_US.UTF-8 LC_NUMERIC=C
## [3] LC_TIME=en_GB LC_COLLATE=C
## [5] LC_MONETARY=en_US.UTF-8 LC_MESSAGES=en_US.UTF-8
## [7] LC_PAPER=en_US.UTF-8 LC_NAME=C
## [9] LC_ADDRESS=C LC_TELEPHONE=C
## [11] LC_MEASUREMENT=en_US.UTF-8 LC_IDENTIFICATION=C
##
## attached base packages:
## [1] grid stats4 stats graphics grDevices utils datasets
## [8] methods base
##
## other attached packages:
## [1] Gviz_1.38.0 BSgenome.Ggallus.UCSC.galGal3_1.4.0
## [3] BSgenome.Hsapiens.UCSC.hg19_1.4.3 BSgenome_1.62.0
## [5] rtracklayer_1.54.0 Biostrings_2.62.0
## [7] XVector_0.34.0 GenomicRanges_1.46.0
## [9] GenomeInfoDb_1.30.0 IRanges_2.28.0
## [11] S4Vectors_0.32.0 BiocGenerics_0.40.0
## [13] CNEr_1.30.0 BiocStyle_2.22.0
##
## loaded via a namespace (and not attached):
## [1] backports_1.2.1 Hmisc_4.6-0
## [3] BiocFileCache_2.2.0 plyr_1.8.6
## [5] lazyeval_0.2.2 splines_4.1.1
## [7] BiocParallel_1.28.0 ggplot2_3.3.5
## [9] digest_0.6.28 ensembldb_2.18.0
## [11] htmltools_0.5.2 magick_2.7.3
## [13] GO.db_3.14.0 fansi_0.5.0
## [15] magrittr_2.0.1 checkmate_2.0.0
## [17] memoise_2.0.0 cluster_2.1.2
## [19] tzdb_0.1.2 readr_2.0.2
## [21] annotate_1.72.0 matrixStats_0.61.0
## [23] R.utils_2.11.0 vroom_1.5.5
## [25] prettyunits_1.1.1 jpeg_0.1-9
## [27] colorspace_2.0-2 blob_1.2.2
## [29] rappdirs_0.3.3 xfun_0.27
## [31] dplyr_1.0.7 crayon_1.4.1
## [33] RCurl_1.98-1.5 jsonlite_1.7.2
## [35] VariantAnnotation_1.40.0 survival_3.2-13
## [37] glue_1.4.2 gtable_0.3.0
## [39] zlibbioc_1.40.0 DelayedArray_0.20.0
## [41] scales_1.1.1 DBI_1.1.1
## [43] Rcpp_1.0.7 xtable_1.8-4
## [45] progress_1.2.2 htmlTable_2.3.0
## [47] foreign_0.8-81 bit_4.0.4
## [49] Formula_1.2-4 htmlwidgets_1.5.4
## [51] httr_1.4.2 RColorBrewer_1.1-2
## [53] ellipsis_0.3.2 pkgconfig_2.0.3
## [55] XML_3.99-0.8 R.methodsS3_1.8.1
## [57] farver_2.1.0 nnet_7.3-16
## [59] sass_0.4.0 dbplyr_2.1.1
## [61] utf8_1.2.2 tidyselect_1.1.1
## [63] labeling_0.4.2 rlang_0.4.12
## [65] reshape2_1.4.4 AnnotationDbi_1.56.0
## [67] munsell_0.5.0 tools_4.1.1
## [69] cachem_1.0.6 cli_3.0.1
## [71] generics_0.1.1 RSQLite_2.2.8
## [73] evaluate_0.14 stringr_1.4.0
## [75] fastmap_1.1.0 yaml_2.2.1
## [77] knitr_1.36 bit64_4.0.5
## [79] purrr_0.3.4 KEGGREST_1.34.0
## [81] AnnotationFilter_1.18.0 R.oo_1.24.0
## [83] poweRlaw_0.70.6 pracma_2.3.3
## [85] xml2_1.3.2 biomaRt_2.50.0
## [87] compiler_4.1.1 rstudioapi_0.13
## [89] filelock_1.0.2 curl_4.3.2
## [91] png_0.1-7 tibble_3.1.5
## [93] bslib_0.3.1 stringi_1.7.5
## [95] highr_0.9 GenomicFeatures_1.46.0
## [97] lattice_0.20-45 ProtGenerics_1.26.0
## [99] Matrix_1.3-4 vctrs_0.3.8
## [101] pillar_1.6.4 lifecycle_1.0.1
## [103] BiocManager_1.30.16 jquerylib_0.1.4
## [105] data.table_1.14.2 bitops_1.0-7
## [107] R6_2.5.1 BiocIO_1.4.0
## [109] latticeExtra_0.6-29 bookdown_0.24
## [111] gridExtra_2.3 dichromat_2.0-0
## [113] assertthat_0.2.1 SummarizedExperiment_1.24.0
## [115] rjson_0.2.20 GenomicAlignments_1.30.0
## [117] Rsamtools_2.10.0 GenomeInfoDbData_1.2.7
## [119] parallel_4.1.1 hms_1.1.1
## [121] rpart_4.1-15 rmarkdown_2.11
## [123] MatrixGenerics_1.6.0 biovizBase_1.42.0
## [125] Biobase_2.54.0 base64enc_0.1-3
## [127] restfulr_0.0.13
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