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NOTE: This Documentation is also available as R Vignette.
chromoMap
provides interactive, configurable and elegant graphics visualization of chromosomes or chromosomal regions allowing users to map chromosome features (like genes,SNPs etc.) onto the chromosome and visualize the feature-associated data (like multi-omics data). Each chromosome is composed of genomic-windows(representing a specific range determined based on chromosome length) that, on hover, shows details about the annotations in that locus range. The plots can be saved as HTML documents that can be shared easily. In addition, you can include them in R Markdown or in R Shiny applications.
Some of the prominent features of the package are:
chromoMap-DiscreteColorMaps
.chromoMap-HeatMaps
(for chromsome heat-maps), chromoMap-Bar
(bar plots on chromosomes), chromoMap-Scatter
(scatter plot on chromosomes), and epi-tags
(condition-based tagging of chromosome genomic-windows).2-Dimensional Chromosome
plots.chromLinks plots
This vignette provide you with a description of how you can use the various features of chromoMap
to create fantastic annotation plots and visualizing the feature-associated data. If you, however, want to know more about the applications of the plot, please check the publication or contact me. I recommend using the RStudio
application since the interactive plots can be viewed beautifully in the application’s viewer pane and it allows you to export the plot either as static image or a stand-alone HTML web page.
chromoMap
You can install the package by just typing the following commands:
install.packages("chromoMap")
The chromoMap
can be used to visualize and annotate chromosomes of any living organism. It is because it renders the chromosome based on the co-ordinate information that you will provide as input. So, if you have the genomic co-ordinates of the organism, you can create chromoMaps for it.
The input data are tab-delimited text files (almost similar to the BED file format). It takes separate files for the chromosomes and the annotations. The input files should not have column headers (however, I have explained each column type below)
This file contains the co-ordinates of the chromosomes. The columns of this file(in order) are described below (all columns are mandatory unless specified optional):
I have developed algorithm that will include both start and end coordinates of chromosomes so that users can also be able to visualize a region of chromosome (not necessarily starting at 1). You can use your imagination to visualize anything that has coordinates( like RNA as well).
Your chromosome file should look like:Once you have chromosome co-ordinates in file, the next thing is to have data for annotation. annotation elements/features could be anything that has co-ordinates like genes,SNPS, etc., and associated data, like gene-expression, methylation etc. The annotation-data is also provided in the same format.
your annotation file should look like:
To prevent you from making some possible errors, here are a few points to care about while preparing files:
TIP: You can use MS excel to create your files and then use save as tab-delimited option.
For the plots in this vignette, I will be using synthetic chromosome and annotation files.
# chromosome files
chr_file_1 = "chr_file_without_centromere.txt"
chr_file_2 = "chr_file_with_centromere.txt"
# annotation files
anno_file_1 = "annotation_pos.txt"
anno_file_2 = "annotation_pos_and_neg.txt"
NOTE: I have used variables to assign file names. You can directly use the file names strings in the chromoMap( ) function.
Let’s have a look at the data in these files:
chromosome file:
head(read.table(chr_file_1,sep = "\t"))
#> V1 V2 V3
#> 1 chr1 1 1000
#> 2 chr2 1 700
Chromosome file with centromere:
head(read.table(chr_file_2,sep = "\t"))
#> V1 V2 V3 V4
#> 1 chr1 1 1000 500
#> 2 chr2 1 700 450
Annotation file with positive data.
head(read.table(anno_file_1,sep = "\t"))
#> V1 V2 V3 V4 V5
#> 1 An1 chr1 558 560 10
#> 2 An2 chr2 396 398 34
#> 3 An3 chr2 281 283 89
#> 4 An4 chr1 125 127 56
#> 5 An5 chr2 406 408 100
#> 6 An6 chr2 340 342 91
Annotation file with both positive and negative data.
head(read.table(anno_file_2,sep = "\t"))
#> V1 V2 V3 V4 V5
#> 1 An1 chr1 558 560 -64
#> 2 An2 chr2 396 398 29
#> 3 An3 chr2 281 283 -137
#> 4 An4 chr1 125 127 -129
#> 5 An5 chr2 406 408 -18
#> 6 An6 chr2 340 342 149
chromoMap
now supports passing R objects directly as input instead of filenames. The chromosome cordinate input (first argument) and annotations(second argument) can either be passed as a character vector
specifying the filenames or as a list of data.frames
with one data.frame per ploidy.
# passing data.frames directly instead of files
chromoMap(list(chr.data),list(anno.data))
# for polyploidy
chromoMap(list(chr.data1,chr.data2),
list(anno.data1,anno.data2),ploidy = 2)
Note: The format of the data is the same. column names or row names is irrelevant and can be anything but the order should be same as described above (for files).
chromoMap
Once you have your input files ready, begin creating chromosomes plots like a pro. The simple annotation plot can be created using the following command:
library(chromoMap)
chromoMap(chr_file_1,anno_file_1)
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 200
#> Visualizing..
This will create a plot with default properties.
that’s it! you have created a simple annotation plot. now hover over the annotated windows to see the magic. you should see a tooltip describing:
If you have added hyperlinks
to the elements, you can click the element labels in tooltip to access the web page.
Tool-tip Toggle: On hover, the tooltip appear on the screen as long as your pointer is over the locus. It will disappear if you move the pointer away. You can click the locus to have a stable tooltip on screen. click again on same or other locus to hide it again.
If you are not satisfied with the default look of the plot(which I’m sure you wouldn’t), you can play around with some of the properties to style your plot described under the section ‘configuring chromoMap
’ in this vignette.
Now, let’s create one with centromeres.
library(chromoMap)
chromoMap(chr_file_2,anno_file_1)
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 200
#> Visualizing..
Biologically speaking, chromosomes occur in sets. So, just visualizing a set of chromosome(called as haploid) wouldn’t be sufficient in some scenarios. Hence, I added the feature of adding sets of chromosomes as seperate set of files. Don’t forget to set the ploidy
argument to the number of sets you are passing.
library(chromoMap)
chromoMap(c(chr_file_1,chr_file_1),c(anno_file_1,anno_file_2),
ploidy = 2)
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 2
#> Number of Chromosomes in set 1 : 2
#> Number of Chromosomes in set 2 : 2
#> Processing data..
#> Number of annotations in data set 1 : 200
#> Number of annotations in data set 2 : 200
#> Visualizing..
polyploidy turned out to be a powerful feature that can actually be used in multiple ways. The sets of chromsomes are rendered independent of each other and, hence, can differ in number and size. Using this feature you can visualize polyploid sets, haploid sets of different species on same plot, or even different samples of same species for comparison. Be creative to use this feature to your own requirement. Some interesting examples I have included in my paper.
I have provided two types of annotation algorithms that will visualize the annotations differently. Point annotation will annotate an element on a single locus, ignoring its size. While, the segment-annotation algorithm consider the size and visualize the annotation as a segment.
The default is point-annotation. To use segment annotation set the argument segment_annotation
to TRUE
. Segment annotations will be advantageous in cases like displaying gene structure.
chromoMap("chromosome_file.txt","annotation_file.txt",segment_annotation = T)
here’s a hypothetical example(exon regions of the genes g1,g2 and g3).
chromoMap
now supports construction of high resolution maps using by either scaling the number of windows per chromosome or by choosing arbitrary window size.
chromoMap
determines the number of genomic windows (and their size/range) constructed for each chromosome based on the length of the chromosomes. By default, 100 windows are created for the longest chromosome and all other chromosomes will have #windows based on the proportion of their length to the longest chromosome.
A new feature now allow to scale the number of windows which consequently reduces the genomic window size. The number of windows will be a multiple of 100 for the longest chromosome while the #windows for rest of chromosomes and the window size are algorithmically determined. Use the argument n_win.factor
to increase the scale as described below. Also, set the argument win.summary.display
to TRUE
to output window summary to console.
# default value
library(chromoMap)
chromoMap(chr_file_1,anno_file_1,
n_win.factor = 1,
win.summary.display=T)
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> ########### Window Summary ##########
#> Summary for Ploidy 1
#> Chr nwins min max
#> chr1 100 10 10
#> chr2 70 10 10
#> ####################################
#> Processing data..
#> Number of annotations in data set 1 : 200
#> Visualizing..
In the window summary, ‘nwin’ is number of windows while ‘min’ and ‘max’ is the minimum and maximum size of the window. In cases where chromsomes cannot be split into equal size windows, two window sizes differeing by 1nt are used (as in the following case).
Now, increasing the #windows 3 times #windows for the longest chromsome.
library(chromoMap)
chromoMap(chr_file_1,anno_file_1,
n_win.factor = 3,
win.summary.display = T)
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> ########### Window Summary ##########
#> Summary for Ploidy 1
#> Chr nwins min max
#> chr1 300 3 4
#> chr2 210 3 4
#> ####################################
#> Processing data..
#> Number of annotations in data set 1 : 200
#> Visualizing..
Alternately, users can now visualize the chromoMap
plots with a fixed window size. In order to use fixed-window method, set the fixed.window
argument to TRUE
and then specify the window.size
.
library(chromoMap)
chromoMap(chr_file_1,anno_file_1,
fixed.window = T,
window.size = 5,
win.summary.display = T)
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> ########### Window Summary ##########
#> Summary for Ploidy 1
#> Chr nwins min max
#> chr1 200 5 5
#> chr2 140 5 5
#> ####################################
#> Processing data..
#> Number of annotations in data set 1 : 200
#> Visualizing..
IMPORTANT In fixed window analysis, the last window of the chromosome will be removed if the chromosome cannot be equally divided using the given window size. Users can include the last window by setting the argument remove.last.window
to FALSE
. Note that in the case when last windows are included, the last windows may not be exactly to the scale.
Huge volume of biological data is being produced in today’s world. I thought it would be nice to visualize the data associated with the chromosome regions or elements/features. You can do this by creating data-based color annotation plots in chromoMap
. Before going forward let’s know about the data types chromoMap can handle. You can use either numeric data or character/categorical data for annotations. For the type of data type you are using, you need to set the argument data_type
to either numeric
or categorical
. Also, to use this category of plot, you need to set data_based_color_map
to TRUE
.Now let’s explore the various types of plots you can create using chromoMap
.
This type of plot can be used if your annotations are categorized into groups. This plot will assign distinct colors to each group. Your annotations file’s data column should have groups assigned to each element as character value.
IMPORTANT: the data_colors
argument will specify the color for each group and must be passed as a list() of vectors. If the ploidy is 2, two vectors will be passed in list. Hence, you must pass a vector for each ploidy in a list.
chromoMap("chromosome_file.txt","annotation_file.txt",
data_based_color_map = T,
data_type = "categorical",
data_colors = list(c("orange","yellow")))
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 20
#> Visualizing..
You can now manually set the order of categories by using the discrete.domain
argument which should be passed as vector with categories as character strings.(e.g discrete.domain
= c("type2","type1")
in above example.)
The best thing is, it can also create a legend for each group with labels used by you as group names. [see more under ‘legends’ section]
chromoMap-HeatMaps
are chromosome heatmaps that allow you to visualize feature associated numeric data as heat colors. In your annotations file, add numeric data in data column.
chromoMap(chr_file_1,anno_file_2,
data_based_color_map = T,
data_type = "numeric")
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 200
#> Visualizing..
data_colors
can be used to set the heat colors also. It should be passed as a list of vector(s) with a vector for each ploidy.
Well, remember that chromosomal locus in the plot is a range, and more than one elements can be annotated in that range. So, for the data assignment of the windows where multiple elements are mapped, there is an aggregation method that allows you to control how data is aggregated/summarized for a given locus. The data for each locus will be determined by aggregate_func
argument which can take avg
for average (default) ,sum
for summation of data values of all elements mapped on that locus, min
, max
,median
and count
.
So, if you want to use the sum function:
chromoMap("chromosome_file.txt","annotation_file.txt",
data_based_color_map = T,
data_type = "numeric",
aggregate_func = "sum")
You can use the different agregate functions for each ploidy by passing the argument as vector. Hence, for polyploidy, if only one value is passed, this value will be used for all sets.Otherwise, you can specify for each set as:
chromoMap(c("chromosome_file_set_1.txt","chromosome_file_set_2.txt")
,c("annotation_file_set_1.txt","annotation_file_set_2.txt"),
ploidy = 2, data_based_color_map = T,data_type = "numeric"
,aggregate_func = c("avg","sum"))
Note: If only one element is annotated per window, than the windows will take the element’s data value.
Please note that for construction of heatmaps, the domain (min-max) used for colors is based on the min-max values of the data. You can manually set the domain by using the numeric.domain
argument.It is a list of vectors where each vector specify the domain for the ploidy.
e.g numeric.domain
= list(c(0,100))
or for diploid use numeric.domain
= list(c(0,100),c(-60,60))
.
In addition to visualizing numeric data as heat colors on the chromosomes, chromoMap allows creating data charts over the annotated windows. chromoMap-Bar
plot can be used to visualize annotated data as barplots. You will need to use the plots
argument to specify the type of data charts you wish to visualize.
chromoMap(chr_file_1,anno_file_1,
data_based_color_map = T,
data_type = "numeric",
plots = "bar")
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 200
#> Visualizing..
The bars represents the aggregate_function
values for the windows. You can customize the chromoMap-Bar plots using various properties described under customizing Data-Plots
section.
You can also turn off the heatmap feature to selectively visualize the chromoMap-Bar
plots ( applicable for all of the plots discussed in the subsequent section). For that, set the heat_map
argument to FALSE
.
chromoMap(chr_file_1,anno_file_1,
data_based_color_map = T,
data_type = "numeric",
plots = "bar",
heat_map = F)
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 200
#> Visualizing..
chromoMap-Scatter
plots allows to visualize each value for a given annotated locus as scatter plot.
chromoMap(chr_file_1,anno_file_2,
data_based_color_map = T,
data_type = "numeric",
plots = "scatter")
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 200
#> Visualizing..
chromoMap-Scatter
plots are also interactive as the tooltips for a scatter shows the annotated element name and value.
This feature allows to filter numeric data based on the various mathematical conditions.
Tag-filters allows you to selectively tag a locus based on mathemetical condition on the data. If the condition is satisfied, the locus will be tagged. tag-filters are passed using the tag_filter
argument. The argument is a list of vectors where you can pass a vector for each ploidy. the vector specifies two values necessary to pass for a filter. The first value specifies the operation-type
and the second value specifies the operands
. Following table describes all possible operation-types along with usage example.
In general, filters are specified as list(c("operation-type-label","operand1","operand2"))
operation type label | description | usage example |
---|---|---|
eq | equal | list(c(“eq”,5)) |
lt | less than | list(c(“lt”,-5)) |
gt | greater than | list(c(“gt”,6)) |
lte | less than equal | list(c(“lte”,6)) |
gte | greater than equal | list(c(“gte”,6)) |
gtalt | greater than AND less than | list(c(“gtalt”,5,-5)) |
gtolt | greater than OR less than | list(c(“gtolt”,5,-5)) |
gtealte | greater than equal AND less than equal | list(c(“gtealte”,5,-5)) |
gteolte | greater than equal OR less than equal | list(c(“gteolte”,5,-5)) |
For instance, to tag the windows with negative number values:
chromoMap(chr_file_1,anno_file_2,
data_based_color_map = T,
data_type = "numeric",
plots = "tags",
tag_filter = list(c("lt",0)))
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 200
#> Visualizing..
plot-filters are similar to tag-filters as they allow filtering of numeric data based on mathematical conditions, but they are visualized as condition-based coloring of chromoMap-Bar
and chromoMap-scatter
plots. The plot_filter
argument allows you to pass filter conditions. It is also a list of vector(s) similar to tag_filter
above, except that you have to pass an additional necessary option of color to it. If the condition is satisfied, this color value is assigned.
So, plot-filters are specified as list(c("operation-type-label","operand1","operand2","color-value"))
Here is an example of using plot-filter on chromoMap-Bar
plots. bars with value greater than and equal to are colored ‘green’.
chromoMap(chr_file_1,anno_file_1,
data_based_color_map = T,
data_type = "numeric",
plots = "bar",
plot_filter = list(c("gte",50,"green")))
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 200
#> Visualizing..
Similarly, it can be applied for chromoMap-Scatter
plots. The following example visualizes negative values as red on the scatter plot.
chromoMap(chr_file_1,anno_file_2,
data_based_color_map = T,
data_type = "numeric",
plots = "scatter",
plot_filter = list(c("lt",0,"red")))
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 200
#> Visualizing..
In order to visualize a second factor onto the scatter plot, you can now use a special plot_filter
option. The input data specifying the categories should be passed a secondary data column in addition to the primary data.
the input data file now looks like:
head(anno_file_3)
#> V1 V2 V3 V4 V5 V6
#> 1 An1 chr1 558 560 10 C
#> 2 An2 chr2 396 398 34 B
#> 3 An3 chr2 281 283 89 B
#> 4 An4 chr1 125 127 56 A
#> 5 An5 chr2 406 408 100 B
#> 6 An6 chr2 340 342 91 D
You can specify the colors of each category by using the ch2D.colors
argument. The legend is automatically displayed and can be adjusted with ch2D.lg_x
and ch2D.lg_y
arguments.
chromoMap(chr_file_1,anno_file_3,
data_based_color_map = T,
data_type = "numeric",
plots = "scatter",
plot_filter = list(c("col","byCategory")),
ch2D.colors = c("pink3","orange3","purple","blue2"))
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 200
#> Visualizing..
NOTE: As of now, only categorical data is supported as secondary data for this feature.
Users can now construct a new kind of plot called 2D-Chromosome
plots. The plot basically visualize annotations in 2D. The X-axis represent the chromosome split into genomic windows, while the y-axis visualize the annotations within the respective genomic windows with their positions relative to the start of the genomic windows.
2D-Chr plots can be constructed by simply using the chr.2D.plot
argument which takes Boolean value.
chromoMap(chr_file_1,anno_file_2,
chr.2D.plot = T)
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 200
#> Visualizing..
Not only that, you can visualize the feature-associated data as heat-maps.
You need to use the plot_filter
argument to create the heat-maps.
For numeric data, you need to pass a vector for plot_filter
specifying that you need to color by numeric data: c("col","byNumber")
. Please not as used previously, plot_filter
is a list which takes values per ploidy, that means that you can construct 2D-chr plot in as multiple-ploidy or even along with other types of plots like “scatter/bars”. You can use plot_height
to adjust the height of the plot.
chromoMap(chr_file_1,anno_file_2,
chr.2D.plot = T,
plot_filter = list(c("col","byNumber")))
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 200
#> Visualizing..
For numeric data, the legend can be adjusted using lg_x
or lg_y
arguments just as you adjust he legends for chromoMap-scatter/bar plots. Also, To change the colors use data_colors
argument.
You can also visualize categorical data as heatmap by using c("col","byCategory")
in plot_filter
. I am using the following data for anotation that has two groups “type1” and “type2”.
head(read.table(anno_file_cate))
#> V1 V2 V3 V4 V5
#> 1 An1 chr1 558 560 type2
#> 2 An2 chr2 396 398 type2
#> 3 An3 chr2 281 283 type1
#> 4 An4 chr1 125 127 type2
#> 5 An5 chr2 406 408 type1
#> 6 An6 chr2 340 342 type2
chromoMap(chr_file_1,anno_file_cate,
chr.2D.plot = T,
plot_filter = list(c("col","byCategory")),
ch2D.colors = c("red","blue"))
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 20
#> Visualizing..
For categorical data, you can use ch2D.lg_x
or ch2D.lg_y
to adjust the legends. You can use ch2D.colors
to manually set the colors for each category. Also ch2D.cat.order
to manually set the order of categories.
Also, although not recommended you can adjust height of annotation bars in 2D-Chr plots by using ann.h
argument.
chromLinks
plots can be used to visualize links or connections between any two features or windows. The two features can be located on the same chromosome or on different chromosomes from the same or different ploidies. The links data needs to be passed separately as a data.frame where each row represents a connection between two features and the columns represents:
The input data.frame should look like:
head(link_data)
#> V1 V2 V3 V4 V5
#> 1 An58 1 An194 1 100
#> 2 An98 1 An122 1 97
#> 3 An113 1 An132 1 95
#> 4 An119 1 An124 1 90
#> 5 An70 1 An120 1 80
#> 6 An105 1 An13 1 85
NOTE: The ploidy columns in the data represents the ploidy of the genomic feature. Since, chromoMap allows using duplicate names in different ploidies, it is important to specify correct ploidy for a given feature.
chromoMap
allows two ways to visualize the links between two features:
chromoMap
annotates the features by using either of the two annotation algorithms, namely, point-annotation and segment-annotation(discussed above). For the former type, links between two annotated features are visualized as edges
. To use the links-visualization feature, you need to set the show.links
argument to TRUE
and pass the links data.frame through the loci_links
argument.
chromoMap(chr_file, anno_file,
# main arguments
show.links = T,
loci_links = link_data[,c(1:4)],
links.colors = "red2",
#plot adjustments
ch_gap = 50,
y_chr_scale = 100,
top_margin = 100,
)
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 205
#> Visualizing..
The numeric or character data associated with the links can be color coded. You just need to pass the data as fifth column. The legends are automatically displayed. use links.lg_x
and links.lg_y
arguments to adjust the legends.
chromoMap(chr_file, anno_file,
# main arguments
show.links = T,
loci_links = link_data,
links.colors = c("red2","blue2"),
#plot adjustments
ch_gap = 50,
y_chr_scale = 100,
top_margin = 100,
links.lg_y = 300
)
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 205
#> Visualizing..
and also categorical data:
chromoMap(chr_file, anno_file,
# main arguments
show.links = T,
loci_links = link_data,
links.colors = c("red2","blue2","orange3","purple"),
#plot adjustments
ch_gap = 50,
y_chr_scale = 100,
top_margin = 100,
)
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 205
#> Visualizing..
there is also an option to visualize the arrow-heads on the links to signify direction. Use the directed.edges
boolean argument.
chromoMap(chr_file, anno_file,
# main arguments
show.links = T,
loci_links = link_data,
links.colors = c("red2","blue2","orange3","purple"),
directed.edges = T,
#plot adjustments
ch_gap = 50,
y_chr_scale = 100,
top_margin = 100,
)
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 205
#> Visualizing..
For segement-annotation plots, where features are usually large size and are annotated as segments of the chromosomes, the links are visualized as chords
.
chromoMap(chr_file, anno_file,
# main arguments
segment_annotation = T,
show.links = T,
loci_links = link_data,
links.colors = c("orange3","purple","green2"),
#plot adjustments
ch_gap = 50,
y_chr_scale = 100,
top_margin = 100,
)
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 3
#> Processing data..
#> Number of annotations in data set 1 : 6
#> Visualizing..
Note: the colors can be passed using the links.colors
argument that takes a character vector specifying color(s) for the links or data maps. For numeric data pass two colors and for categorical data pass as many colors as there are categories.
chromoMap
allows various options to customize and fine-tune your plots as desirable. This section covers all the customization options available.
You can configure the dimensions(width and height) of the plot by using the parameter canvas_width
and canvas_height
. From version 0.4.1 onwards, chromoMap automatically adjust the width and height to fit the plot and provide vertical and horizontal srolling in case of overflow.
chromoMap("chromosome_file.txt","annotation_file.txt",
canvas_width = 600,
canvas_height = 700)
When you use multiple ploidy, the plot might go off the margins. You can adjust the width and height to fit the plot to your need.
You can add a title to your plot by using title
argument.
chromoMap("chromosome_file.txt","annotation_file.txt",
title = "my first chromoMap plot")
You can also adjust the font-size of the title using the title_font_size
argument:
chromoMap("chromosome_file.txt","annotation_file.txt",
title = "my first chromoMap plot",
title_font_size = 12)
You can adjust the left and top margins through top_margin
and left_margin
.
chromoMap("chromosome_file.txt","annotation_file.txt",
top_margin = 25,
left_margin = 15)
You can change the color of each set of chromosome by using chr_color
property.
chromoMap("chromosome_file.txt","annotation_file.txt",
chr_color = c("orange"))
For polyploidy, if only one color is passed it will be taken for all sets of chromsomes. Otherwise, you can assign color to each set:
chromoMap(c("chromosome_file_set_1.txt","chromosome_file_set_2.txt")
,c("annotation_file_set_1.txt","annotation_file_set_2.txt"),
ploidy = 2,
chr_color = c("pink","blue"))
USEFUL TIPS :
For simple annotation plot, you can change the annotation color by using anno_col
argument.
chromoMap("chromosome_file.txt","annotation_file.txt",
anno_col = c("orange"))
For polyploidy, if you have passed one color value it will be taken for all the sets. Otherwise, you can pass distinct color values for each set:
chromoMap(c("chromosome_file_set_1.txt","chromosome_file_set_2.txt")
,c("annotation_file_set_1.txt","annotation_file_set_2.txt"),
ploidy = 2,
anno_col = c("pink","blue"))
NOTE: For data-based annotation plots(chromoMap-DiscreteColorMaps
or chromoMap-HeatMaps
), colors are controlled by data_colors
argument which is passed as a list of vector(s).
Do you think chromosomes appear too thin or too short for your annotations? well, you can adjust these parameters by using chr_width
and chr_length
arguments.
chromoMap("chromosome_file.txt","annotation_file.txt",
chr_width = 4,
chr_length = 5)
the spacing between chromosomes can be adjusted with ch_gap
argument.
chromoMap("chromosome_file.txt","annotation_file.txt",
ch_gap = 6)
The curves appearing at the telo-meres (chromosome end windows) and in centromere locus can also be adjusted using the chr_curve
argument.
chromoMap("chromosome_file.txt","annotation_file.txt",
chr_curve = 5)
TIP: setting this property to 0 will remove the curves that render the chromosomes as rectangles.
You can adjust the y or vertical position of the chromosome scale using the y_chr_scale
argument.
Well, the chromosome text will be taken from file you have provided. The only thing I thought might be useful is to enable or disable text individually for each ploidy. This is done by using chr_text
parameter.
chromoMap("chromosome_file.txt","annotation_file.txt",
chr_text = F)
For multiple ploidy pass a vector:
chromoMap(c("chromosome_file_set_1.txt","chromosome_file_set_2.txt")
,c("annotation_file_set_1.txt","annotation_file_set_2.txt"),
ploidy = 2,
chr_text = c(T,F))
you can adjust the text font size using text_font_size
parameter.
You can now disable/enable interactivity for chromosomes by using the interactivity
argument.
chromoMap("chromosome_file.txt","annotation_file.txt",
interactivity = F)
You can change the ‘suffix’ value used in the chromosome scale. By default it uses ‘bp’ but you can set to any other value or remove it by passing empty string ““.
chromoMap("chromosome_file.txt","annotation_file.txt",
scale.suffix = "cM")
You can set the number of ticks for chr scale using chr.scale.ticks
argument.
You can choose to show/hide the chromosomes for each ploidy by using the display.chr
argument. It can be different for different ploidy like you can pass c(F,T)
to this argument indicating that you only want to hide the first ploidy chromosomes. NOTE that plots will still be visible and you can adjust the plots with plot_shift
argument.
chromoMap("chromosome_file.txt","annotation_file.txt",
display.chr = c(F))
You can display guides in the background using the guides
argument. Guides will help separate each genomic window. You can also set the color by guides_color
.
chromoMap("chromosome_file.txt","annotation_file.txt",
guides = T,
guides_color = "black")
The id
argument allows to uniquely identify the plot. This feature is important when including multiple chromoMap plots in a single HTML document (like RMarkdown) as it prevent from any conflicts.
chromoMap("chromosome_file.txt","annotation_file.txt",
id="my_plot_1")
As a test feature, chromoMap
now automatically assigns random color values if the colors are not passed manually. the color values are randomly selected and change every time you plot. I would still recommend using the manual color assignments.
Also, now you can use R color names such as ‘red3’ as color inputs.
chromoMap-Bar
, chromoMap-Scatter
, and epi-tag
plots can be customized as desired.
You can add a horizontal reference line to the data-plots. Set the ref_line
argument to TRUE
. The reference line is attached to the axis-scale. By default, the line is attached at the beginning of the axis(position:0). You can adjust the refl_pos
argument to bring the line to desirable position.
TIP:For the line to be at the middle of axis, set refl_pos
argument to exactly half of plot_height
.
chromoMap(chr_file_1,anno_file_1,
data_based_color_map = T,
data_type = "numeric",
plots = "bar",
ref_line = T,
refl_pos = 15)
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 200
#> Visualizing..
Reference line in scatter plot:
chromoMap(chr_file_1,anno_file_2,
data_based_color_map = T,
data_type = "numeric",
plots = "scatter",
ref_line = T,
refl_pos = 20)
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 200
#> Visualizing..
You can change the color and stroke-size of the reference line using refl_color
and refl_stroke_w
arguments respectively.
Change the plot height using plot_height
parameter.
chromoMap(chr_file_1,anno_file_2,
data_based_color_map = T,
data_type = "numeric",
plots = "scatter",
plot_height = 50)
Change the plot colors (bar and scatter colors) using the plot_color
parameter.
chromoMap(chr_file_1,anno_file_2,
data_based_color_map = T,
data_type = "numeric",
plots = "scatter",
plot_color = "orange")
For the epi-tag plots, you need to use tagColor
argument that will change the tag-head colors.
chromoMap(chr_file_1,anno_file_2,
data_based_color_map = T,
data_type = "numeric",
plots = "tags",
tagColor = "orange")
You can change the range of y-axis of the plots using plot_y_domain
argument. It is passed as list of vector(s), a vector for each ploidy. You can also change the number of ticks of the scale using the plot_ticks
argument.
chromoMap(chr_file_1,anno_file_2,
data_based_color_map = T,
data_type = "numeric",
plots = "scatter",
plot_ticks = 3,
plot_y_domain = list(c(-5,5)))
You can now set y-axis labels for the plots for each ploidy by using plot.y.labels
argument. Adjust the x nd y position of the labels by using plot.y.lab.x
and plot.y.lab.y
argument respectively. Set the size with plot.y.lab.size
.
vertical grid lines can be used to highlight specific regions of the chromosomes. You can add any number of grid-lines to the plot. Set the vertical_grid
argument to TRUE
. You can add multiple grid lines by specifying a vector of positions(in bp) within the max range of the plot(depicted by the horizontal chromosome scale). The following example demonstrate the use of grid lines where 5 grid lines are added at random genomic positions 1,54,100,420, and 621(the entire scale is 1k bp wide). The plot also demonstrate the use of other customization options.
chromoMap(c(chr_file_1,chr_file_1),c(anno_file_1,anno_file_2),
ploidy = 2
data_based_color_map = T,
data_type = "numeric",
plots = c("bar","scatter"),
plot_height = 40,
plot_color = c("green","red"),
ref_line = T,
refl_pos = 20,
#gridline arguments
vertical_grid = T,
grid_array = c(1,54,100,420,621))
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 2
#> Number of Chromosomes in set 1 : 2
#> Number of Chromosomes in set 2 : 2
#> Processing data..
#> Number of annotations in data set 1 : 200
#> Number of annotations in data set 2 : 200
#> Visualizing..
You can also add text/labels for individual grid line. the text will added at the top end of the grid-line and needs to be passed as an array(vector) of texts for each corresponding position passed in grid_array
. Use the grid_text
argument to pass the text, grid_text_size
to specify the text font-size, grid_text_y
to adjust the vertical position of the texts, and grid_color
to change color of grid-lines.
chromoMap(c(chr_file_1,chr_file_1),c(anno_file_1,anno_file_2),
ploidy = 2
data_based_color_map = T,
data_type = "numeric",
plots = c("bar","scatter"),
plot_height = 40,
plot_color = c("green","red"),
ref_line = T,
refl_pos = 20,
#gridline arguments
vertical_grid = T,
grid_array = c(1,54,100,420,621),
grid_text = c("","","mark 1","region 1",""))
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 2
#> Number of Chromosomes in set 1 : 2
#> Number of Chromosomes in set 2 : 2
#> Processing data..
#> Number of annotations in data set 1 : 200
#> Number of annotations in data set 2 : 200
#> Visualizing..
Note: for the grid-lines for which no text was displayed an empty string ""
is added corresponding to the grid-line position. The length of grid_array
and grid_text
should match.
chromoMap
now supports a quick zoom-in feature that allow the users to zoom in on a specific region of interest on any chromosome. The region information is passed with the region
argument which is a character vector containing region(s) in the following format:
c("<chromsome name>:<ploidy>:<region start>:<region stop>")
eg. c(“chr1:1:5142689:6478512”)
chromoMap(chr_file_1,anno_file_2,
data_based_color_map = T,
data_type = "numeric",
plots = "scatter",
#highlighting a region on chr1
vertical_grid = T,
grid_array = c(550,754))
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 200
#> Visualizing..
chromoMap(chr_file_1,anno_file_2,
data_based_color_map = T,
data_type = "numeric",
plots = "scatter",
#zoom in
region = c("chr1:1:550:754"))
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> WARNING: 80 out-of-bound annotations are removed in chromosome set 1 .
#> Number of annotations in data set 1 : 120
#> Visualizing..
Note: the scale of the chromosomes will be updated based on their new length. The region zoom could have been done by modifying the chromosome range in the input chromosome files but this argument provides a quick option to view a region of interest without changing the master chromosome data.
multiple regions can also be passed as:
chromoMap(chr_file_1,anno_file_2,
data_based_color_map = T,
data_type = "numeric",
plots = "scatter",
#zoom in
region = c("chr1:1:550:754","chr2:1:221:450"))
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> WARNING: 138 out-of-bound annotations are removed in chromosome set 1 .
#> Number of annotations in data set 1 : 62
#> Visualizing..
legends are provided for data-based annotation plots (chromoMap-DiscreteColorMaps
and chromoMap-HeatMaps
). It is hidden by default. Use legend
option to enable it.
chromoMap("chromosome_file.txt","annotation_file.txt",
data_based_color_map = T,
data_type = "categorical",
legend = T)
For polyploidy, you can enable or disable the legend independently for each set.
chromoMap(c("chromosome_file_set_1.txt","chromosome_file_set_2.txt")
,c("annotation_file_set_1.txt","annotation_file_set_2.txt"),
ploidy = 2,
data_based_color_map = T,
data_type = "numeric",
legend = c(F,T))
I know, the legends in your plot are present weirdly?. I have made the postion of legends independent of the plot and hence you can position it anywhere in the plot you want using the y and x direction length. Consider the orgin to be the bottom right corner of the plot now tweak the lg_x
and/or lg_y
arguments to adjust the positioning of the legend.
chromoMap("chromosome_file.txt","annotation_file.txt",
data_based_color_map = T,
data_type = "categorical",
legend = T, lg_x = 100,
lg_y = 250)
For numeric-data plots like scatter/bar use plot.legend.labels
for each ploidy. For categorical data legends, use cat.legend.label
. Note that for categorical data plots, only one legend is shown with all categories.
This feature I added at the end thought might be useful in some scenarios. This will show the labels (element names) on top of locus. It is disabled by default, to enable it use label
argument.
chromoMap("chromosome_file.txt","annotation_file.txt",
labels=T)
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 20
#> Visualizing..
You can change the labels angle and font-size using label_angle
and label_font
arguments respectively.
chromoMap("chromosome_file.txt","annotation_file.txt",
labels=T,
label_font = 12,
label_angle = -65)
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 20
#> Visualizing..
TIP: To make the labels non-overlapping, tweak the chromosome length and width properties like shown in the following example.
chromoMap("chromosome_file.txt","annotation_file.txt",
labels=T,
label_angle = -65,
chr_length = 6,
chr_width = 25,
canvas_width = 800)
#> ********************************** __ __ ************
#> ** __**|__ * __* __ * __ __ * __ *| | |* __ * __ **
#> **|__**| |*| *|__|*| | |*|__|*| | |*|_ |*|__|**
#> ***********************************************| **
#> *****************************************************
#> OUTPUT:
#> Number of Chromosome sets: 1
#> Number of Chromosomes in set 1 : 2
#> Processing data..
#> Number of annotations in data set 1 : 20
#> Visualizing..
This feature will allow you to add hyperlinks with elements. Add hyperlinks in annotations file and don’t forget to use hlinks
argument to enable it.
chromoMap("chromosome_file.txt","annotation_file.txt",
hlinks=T)
The RStudio
allows the option to export the graphics, shown in its viewer’s pane ,as either a static image or a web page. Use this feature to either save chromoMaps as static images and include them into your documents or papers, or export interactive plots as standalone-html to include them as supplementary materials in publications.
From version 0.4.1, chromoMap has an in-built exporting options that provide buttons to export the plot as either PNG or SVG. In order to use it, set the export.options
argument to TRUE
. You will see export buttons at the bottom of plot.
IMPORTANT The buttons might not work in RStudios’ viewer pane. you can first export the plot as “WEB Page/HTML” and then view it in a broweser like Chrome.
You can include chromoMaps in Shiny application by using the function chromoMapOutput()
in the UI part of the code and renderChromoMap()
in the server part of the code.
library(shiny)
library(chromoMap)
# Define UI for application that draws chromoMap
ui <- fluidPage(
# Application title
titlePanel("An example of chromoMap in Shiny"),
# you can use GUI controls for your chromoMap
sidebarLayout(
sidebarPanel(
#some code
),
# Show a plot of the generated distribution
mainPanel(
chromoMapOutput("myChromoMap")
)
)
)
# Define server logic required to draw chromoMap
server <- function(input, output) {
output$myChromoMap <- renderChromoMap({
chromoMap("chromosome_file.txt","annotation_file.txt")
})
}
# Run the application
shinyApp(ui = ui, server = server)
The chromoMap package is distributed under GPL-3 (GNU GENERAL PUBLIC LICENSE version 3).
You are welcome to send feedback or bug reports through e-mail lakshayanan15@gmail.com
chromoMap
is now published in BMC Bioinformatics journal. Please visit the site for citing options.
sessionInfo()
#> R version 4.1.3 (2022-03-10)
#> Platform: aarch64-apple-darwin20 (64-bit)
#> Running under: macOS Monterey 12.2.1
#>
#> Matrix products: default
#> BLAS: /Library/Frameworks/R.framework/Versions/4.1-arm64/Resources/lib/libRblas.0.dylib
#> LAPACK: /Library/Frameworks/R.framework/Versions/4.1-arm64/Resources/lib/libRlapack.dylib
#>
#> locale:
#> [1] C/en_US.UTF-8/en_US.UTF-8/C/en_US.UTF-8/en_US.UTF-8
#>
#> attached base packages:
#> [1] stats graphics grDevices utils datasets methods base
#>
#> other attached packages:
#> [1] knitr_1.37 chromoMap_4.1.1
#>
#> loaded via a namespace (and not attached):
#> [1] digest_0.6.29 R6_2.5.1 jsonlite_1.7.2 magrittr_2.0.1
#> [5] evaluate_0.14 highr_0.9 rlang_0.4.12 stringi_1.7.6
#> [9] jquerylib_0.1.4 bslib_0.3.1 rmarkdown_2.11 tools_4.1.3
#> [13] stringr_1.4.0 htmlwidgets_1.5.4 xfun_0.29 yaml_2.2.1
#> [17] fastmap_1.1.0 compiler_4.1.3 htmltools_0.5.2 sass_0.4.0
These binaries (installable software) and packages are in development.
They may not be fully stable and should be used with caution. We make no claims about them.
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