calculate_go_enrichment: Perform gene ontology enrichment analysis
In jpquast/protti: Bottom-Up Proteomics and LiP-MS Quality Control and Data Analysis Tools
View source: R/calculate_go_enrichment.R
calculate_go_enrichment R Documentation
Perform gene ontology enrichment analysis
Description
Analyses enrichment of gene ontology terms associated with proteins in the fraction of
significant proteins compared to all detected proteins. A two-sided Fisher's exact test is
performed to test significance of enrichment or depletion. GO annotations can be provided to
this function either through UniProt go_annotations_uniprot, through a table obtained
with fetch_go in the go_data argument or GO annotations are fetched automatically
by the function by providing ontology_type and organism_id.
Usage
calculate_go_enrichment(
data,
protein_id,
is_significant,
group = NULL,
y_axis_free = TRUE,
facet_n_col = 2,
go_annotations_uniprot = NULL,
ontology_type,
organism_id = NULL,
go_data = NULL,
plot = TRUE,
plot_style = "barplot",
plot_title = "Gene ontology enrichment of significant proteins",
barplot_fill_colour = c("#56B4E9", "#E76145"),
heatmap_fill_colour = protti::mako_colours,
heatmap_fill_colour_rev = TRUE,
label = TRUE,
enrichment_type = "all",
min_n_detected_proteins_in_process = 1,
plot_cutoff = "adj_pval top10"
)
Arguments
data
a data frame that contains at least the input variables.
protein_id
a character column in the data data frame that contains the protein
accession numbers.
is_significant
a logical column in the data data frame that indicates if the
corresponding protein has a significantly changing peptide. The input data frame may contain
peptide level information with significance information. The function is able to extract
protein level information from this.
group
optional, character column in the data data frame that contains information by
which the analysis should be grouped. The analysis will be performed separately for each of the
groups. This is most likely a column that labels separate comparisons of different conditions.
In protti the assign_missingness() function creates such a column automatically.
y_axis_free
a logical value that specifies if the y-axis of the plot should be "free"
for each facet if a grouping variable is provided. Default is TRUE. If FALSE is selected
it is easier to compare GO categories directly with each other.
facet_n_col
a numeric value that specifies the number of columns the faceted plot should have
if a column name is provided to group. The default is 2.
go_annotations_uniprot
recommended, a character column in the data data frame
that contains gene ontology annotations obtained from UniProt using fetch_uniprot.
These annotations are already separated into the desired ontology type so the argument
ontology_type is not required.
ontology_type
optional, character value specifying the type of ontology that should
be used. Possible values are molecular function (MF), biological process (BP), cellular component
(CC). This argument is not required if GO annotations are provided from UniProt in
go_annotations_uniprot. It is required if annotations are provided through go_data or
automatically fetched.
organism_id
optional, character value specifying an NCBI taxonomy identifier of an
organism (TaxId). Possible inputs include only: "9606" (Human), "559292" (Yeast) and "83333"
(E. coli). Is only necessary if GO data is not provided either by go_annotations_uniprot
or in go_data.
go_data
Optional, a data frame that can be obtained with fetch_go(). If you provide
data not obtained with fetch_go() make sure column names for protein ID (db_id) and GO ID
(go_id) are the same as for data obtained with fetch_go().
plot
a logical argument indicating whether the result should be plotted or returned as a table.
plot_style
a character argument that specifies the plot style. Can be either "barplot" (default)
or "heatmap". The "heatmap" plot is especially useful for the comparison of multiple groups. We recommend,
however, that you use it only with enrichment_type = "enriched" or enrichment_type = "deenriched,
because otherwise it is not possible to distinguish between enrichment and deenrichment in the plot.
plot_title
a character value that specifies the title of the plot. The default is "Gene ontology
enrichment of significant proteins".
barplot_fill_colour
a vector that contains two colours that should be used as the fill colours for
deenriched and enriched GO terms, respectively. If enrichment_type = "enriched" or "deenriched, please
still provide two values in the vector, the colour not used for the plot can be NA in this case. E.g.
c(NA, "red") for enrichment_type = "enriched".
heatmap_fill_colour
a vector that contains colours that should be used to create the gradient in the
heatmap plot. Default is mako_colours.
heatmap_fill_colour_rev
a logical value that specifies if the provided colours in heatmap_fill_colour
should be reversed in order. Default is TRUE.
label
a logical argument indicating whether labels should be added to the plot.
Default is TRUE.
enrichment_type
a character argument that is either "all", "enriched" or "deenriched". This
determines if the enrichment analysis should be performed in order to check for both enrichemnt and
deenrichemnt or only one of the two. This affects the statistics performed and therefore also the displayed
plot.
min_n_detected_proteins_in_process
is a numeric argument that specifies the minimum number of
detected proteins required for a GO term to be displayed in the plot. The default is 1, meaning
no filtering of the plotted data is performed. This argument does not affect any computations or
the returned data if plot = FALSE. This argument is useful in order to remove terms that were only
detected in for example 1 protein. Even though these terms are sometimes significant, they are not
really relevant.
plot_cutoff
a character value indicating if the plot should contain the top n (e.g. top10) most
significant proteins (p-value or adjusted p-value), or if a significance cutoff should be used
to determine the number of GO terms in the plot. This information should be provided with the
type first followed by the threshold separated by a space. Example are
plot_cutoff = "adj_pval top10", plot_cutoff = "pval 0.05" or
plot_cutoff = "adj_pval 0.01". The threshold can be chosen freely. The default value is
"adj_pval top10".
Value
A bar plot or heatmap (depending on plot_style). By default the bar plot displays negative log10
adjusted p-values for the top 10 enriched or deenriched gene ontology terms. Alternatively, plot cutoffs
can be chosen individually with the plot_cutoff argument. Bars are colored according to the direction
of the enrichment (enriched or deenriched). If a heatmap is returned, terms are organised on the y-axis, while
the colour of each tile represents the negative log10 adjusted p-value (default). If a group column
is provided the x-axis contains all groups. If plot = FALSE, a data frame is returned. P-values are adjusted with
Benjamini-Hochberg.
Examples
# Load libraries
library(dplyr)
library(stringr)
# Create example data
# Contains artificial de-enrichment for ribosomes.
uniprot_go_data <- fetch_uniprot_proteome(
organism_id = 83333,
columns = c(
"accession",
"go_f"
)
)
if (!is(uniprot_go_data, "character")) {
data <- uniprot_go_data %>%
mutate(significant = c(
rep(TRUE, 1000),
rep(FALSE, n() - 1000)
)) %>%
mutate(significant = ifelse(
str_detect(
go_f,
pattern = "ribosome"
),
FALSE,
significant
)) %>%
mutate(group = c(
rep("A", 500),
rep("B", 500),
rep("A", (n() - 1000) / 2),
rep("B", round((n() - 1000) / 2))
))
# Plot gene ontology enrichment
calculate_go_enrichment(
data,
protein_id = accession,
go_annotations_uniprot = go_f,
is_significant = significant,
plot = TRUE,
plot_cutoff = "pval 0.01"
)
# Plot gene ontology enrichment with group
calculate_go_enrichment(
data,
protein_id = accession,
go_annotations_uniprot = go_f,
is_significant = significant,
group = group,
facet_n_col = 1,
plot = TRUE,
plot_cutoff = "pval 0.01"
)
# Plot gene ontology enrichment with group in a heatmap plot
calculate_go_enrichment(
data,
protein_id = accession,
group = group,
go_annotations_uniprot = go_f,
is_significant = significant,
min_n_detected_proteins_in_process = 15,
plot = TRUE,
label = TRUE,
plot_style = "heatmap",
enrichment_type = "enriched",
plot_cutoff = "pval 0.01"
)
# Calculate gene ontology enrichment
go_enrichment <- calculate_go_enrichment(
data,
protein_id = accession,
go_annotations_uniprot = go_f,
is_significant = significant,
plot = FALSE,
)
head(go_enrichment, n = 10)
}
jpquast/protti documentation built on June 9, 2024, 10:40 a.m.
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View source: R/calculate_go_enrichment.R
| calculate_go_enrichment | R Documentation |
Perform gene ontology enrichment analysis
Description
Analyses enrichment of gene ontology terms associated with proteins in the fraction of
significant proteins compared to all detected proteins. A two-sided Fisher's exact test is
performed to test significance of enrichment or depletion. GO annotations can be provided to
this function either through UniProt go_annotations_uniprot, through a table obtained
with fetch_go in the go_data argument or GO annotations are fetched automatically
by the function by providing ontology_type and organism_id.
Usage
calculate_go_enrichment(
data,
protein_id,
is_significant,
group = NULL,
y_axis_free = TRUE,
facet_n_col = 2,
go_annotations_uniprot = NULL,
ontology_type,
organism_id = NULL,
go_data = NULL,
plot = TRUE,
plot_style = "barplot",
plot_title = "Gene ontology enrichment of significant proteins",
barplot_fill_colour = c("#56B4E9", "#E76145"),
heatmap_fill_colour = protti::mako_colours,
heatmap_fill_colour_rev = TRUE,
label = TRUE,
enrichment_type = "all",
min_n_detected_proteins_in_process = 1,
plot_cutoff = "adj_pval top10"
)
Arguments
data |
a data frame that contains at least the input variables. |
protein_id |
a character column in the |
is_significant |
a logical column in the |
group |
optional, character column in the |
y_axis_free |
a logical value that specifies if the y-axis of the plot should be "free"
for each facet if a grouping variable is provided. Default is |
facet_n_col |
a numeric value that specifies the number of columns the faceted plot should have if a column name is provided to group. The default is 2. |
go_annotations_uniprot |
recommended, a character column in the |
ontology_type |
optional, character value specifying the type of ontology that should
be used. Possible values are molecular function (MF), biological process (BP), cellular component
(CC). This argument is not required if GO annotations are provided from UniProt in
|
organism_id |
optional, character value specifying an NCBI taxonomy identifier of an
organism (TaxId). Possible inputs include only: "9606" (Human), "559292" (Yeast) and "83333"
(E. coli). Is only necessary if GO data is not provided either by |
go_data |
Optional, a data frame that can be obtained with |
plot |
a logical argument indicating whether the result should be plotted or returned as a table. |
plot_style |
a character argument that specifies the plot style. Can be either "barplot" (default)
or "heatmap". The "heatmap" plot is especially useful for the comparison of multiple groups. We recommend,
however, that you use it only with |
plot_title |
a character value that specifies the title of the plot. The default is "Gene ontology enrichment of significant proteins". |
barplot_fill_colour |
a vector that contains two colours that should be used as the fill colours for
deenriched and enriched GO terms, respectively. If |
heatmap_fill_colour |
a vector that contains colours that should be used to create the gradient in the
heatmap plot. Default is |
heatmap_fill_colour_rev |
a logical value that specifies if the provided colours in |
label |
a logical argument indicating whether labels should be added to the plot. Default is TRUE. |
enrichment_type |
a character argument that is either "all", "enriched" or "deenriched". This determines if the enrichment analysis should be performed in order to check for both enrichemnt and deenrichemnt or only one of the two. This affects the statistics performed and therefore also the displayed plot. |
min_n_detected_proteins_in_process |
is a numeric argument that specifies the minimum number of
detected proteins required for a GO term to be displayed in the plot. The default is 1, meaning
no filtering of the plotted data is performed. This argument does not affect any computations or
the returned data if |
plot_cutoff |
a character value indicating if the plot should contain the top n (e.g. top10) most
significant proteins (p-value or adjusted p-value), or if a significance cutoff should be used
to determine the number of GO terms in the plot. This information should be provided with the
type first followed by the threshold separated by a space. Example are
|
Value
A bar plot or heatmap (depending on plot_style). By default the bar plot displays negative log10
adjusted p-values for the top 10 enriched or deenriched gene ontology terms. Alternatively, plot cutoffs
can be chosen individually with the plot_cutoff argument. Bars are colored according to the direction
of the enrichment (enriched or deenriched). If a heatmap is returned, terms are organised on the y-axis, while
the colour of each tile represents the negative log10 adjusted p-value (default). If a group column
is provided the x-axis contains all groups. If plot = FALSE, a data frame is returned. P-values are adjusted with
Benjamini-Hochberg.
Examples
# Load libraries
library(dplyr)
library(stringr)
# Create example data
# Contains artificial de-enrichment for ribosomes.
uniprot_go_data <- fetch_uniprot_proteome(
organism_id = 83333,
columns = c(
"accession",
"go_f"
)
)
if (!is(uniprot_go_data, "character")) {
data <- uniprot_go_data %>%
mutate(significant = c(
rep(TRUE, 1000),
rep(FALSE, n() - 1000)
)) %>%
mutate(significant = ifelse(
str_detect(
go_f,
pattern = "ribosome"
),
FALSE,
significant
)) %>%
mutate(group = c(
rep("A", 500),
rep("B", 500),
rep("A", (n() - 1000) / 2),
rep("B", round((n() - 1000) / 2))
))
# Plot gene ontology enrichment
calculate_go_enrichment(
data,
protein_id = accession,
go_annotations_uniprot = go_f,
is_significant = significant,
plot = TRUE,
plot_cutoff = "pval 0.01"
)
# Plot gene ontology enrichment with group
calculate_go_enrichment(
data,
protein_id = accession,
go_annotations_uniprot = go_f,
is_significant = significant,
group = group,
facet_n_col = 1,
plot = TRUE,
plot_cutoff = "pval 0.01"
)
# Plot gene ontology enrichment with group in a heatmap plot
calculate_go_enrichment(
data,
protein_id = accession,
group = group,
go_annotations_uniprot = go_f,
is_significant = significant,
min_n_detected_proteins_in_process = 15,
plot = TRUE,
label = TRUE,
plot_style = "heatmap",
enrichment_type = "enriched",
plot_cutoff = "pval 0.01"
)
# Calculate gene ontology enrichment
go_enrichment <- calculate_go_enrichment(
data,
protein_id = accession,
go_annotations_uniprot = go_f,
is_significant = significant,
plot = FALSE,
)
head(go_enrichment, n = 10)
}
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