omu, a Metabolomics Analysis R Package
Connor R. Tiffany
5/2020
Introduction to omu
Omu is an R package that enables rapid analysis of Metabolomics data sets, and the creation of intuitive graphs. Omu can assign metabolite classes (Carbohydrates, Lipids, etc) as meta data, perform t tests, anovas and principle component analysis, and gather functional orthology and gene names from the KEGG database that are associated with the metabolites in a dataset. This package was developed with inexperienced R users in mind.
If your data do not yet have KEGG compound numbers you can acquire them by using the chemical translation service provided by the Fiehn lab here http://cts.fiehnlab.ucdavis.edu/
Data Analysis
Data Format
Included with Omu is an example metabolomics dataset of data from fecal samples collected from a two factor experiment with wild type c57B6J mice and c57B6J mice with a knocked out nos2 gene, that were either mock treated, or given streptomycin(an antibiotic), and a metadata file. To use Omu, you need a metabolomics count data frame in .csv format that resembles the example dataset, with the column headers Metabolite, KEGG, and then one for each of your samples. Row values are metabolite names in the Metabolite column, KEGG cpd numbers in the KEGG column, and numeric counts in the Sample columns.Additionally, for statistical analysis your data should already have undergone missing value imputation(eg. using random forest, k nearest neighbors, etc.). Here is a truncated version of the sample data in Omu as a visual example of this:
| Metabolite | KEGG | C289_1 |
|---|---|---|
| xylulose_NIST | C00312 | 2424 |
| xylose | C00181 | 56311 |
| xylonolactone_NIST | C02266 | 637 |
| xylonic_acid | C00502 | 545 |
The meta data file should have a Sample column, with row values being sample names, and then a column for each Factor in your dataset, with row values being groups within that factor. Here is a truncated version of the metadata that accompanies the above dataset:
| Sample | Background | Treatment | Grouped |
|---|---|---|---|
| C289_1 | WT | Mock | WTMock |
| C289_2 | WT | Mock | WTMock |
| C289_3 | WT | Mock | WTMock |
| C289_4 | WT | Mock | WTMock |
Getting Your Data into R
For end users metabolomics data, it is recommended to use the
read.metabo function to load it into R. This function is
simply a wrapper for read.csv, which ensures your data has
the proper class for KEGG_gather to work. For metadata,
read.csv should be used.
your_metabolomics_count_dataframe <- read.metabo(filepath = "path/to/your/data.csv")
your_metabolomics_metadata <- read.csv("path/to/your/metadata.csv")Assiging Hierarchical Class Data
Omu can assign hierarchical class data for metabolites, functional
orthologies, and organism identifiers associated with gene names. It
does this using data frames located in the system data of the
package(these can not be viewed or edited by the user, but the tables
are available on the Omu github page in .csv format). To assign
hierarchical class data, use the assign_hierarchy function
and pick the correct identifier, either “KEGG”, “KO_Number”,
“Prokaryote”, or “Eukaryote”. For example, using the
c57_nos2KO_mouse_countDF.RData that comes with the package, compound
hierarchy data can be assigned with the following code:
DF <- assign_hierarchy(count_data = c57_nos2KO_mouse_countDF, keep_unknowns = TRUE, identifier = "KEGG")The argument keep_unknowns = TRUE keeps compounds
without KEGG numbers, and compound hierarchy data was assigned by
providing “KEGG” for the identifier argument. The output DF
should look like this:
| Metabolite | KEGG | Class | Subclass_1 | Subclass_2 | Subclass_3 | Subclass_4 |
|---|---|---|---|---|---|---|
| xylulose_NIST | C00312 | Carbohydrates | Monosaccharides | Ketoses | none | none |
| xylose | C00181 | Carbohydrates | Monosaccharides | Aldoses | none | none |
| xylonolactone_NIST | C02266 | Carbohydrates | Lactones | none | none | none |
| xylonic_acid | C00502 | Carbohydrates | Monosaccharides | Sugar acids | none | none |
Machine Learning
PCA Plots
Omu supports multivariate statistical analysis and visualization in
the form of principle component analysis. To do this one only needs to
have their metabolomics count data and meta data in the proper format.
It is recommended to deal with overdispersion of data prior to using
PCA_plot, by transformation via natural log, sqrt, etc.
A PCA plot can be made showing the relationship between Treatment groups in the package dataset:
c57_nos2KO_mouse_countDF_log <- c57_nos2KO_mouse_countDF
c57_nos2KO_mouse_countDF_log <- log(c57_nos2KO_mouse_countDF_log[,3:31])
c57_nos2KO_mouse_countDF_log <- cbind(c57_nos2KO_mouse_countDF[,1:2], c57_nos2KO_mouse_countDF_log)
PCA <- PCA_plot(count_data = c57_nos2KO_mouse_countDF_log, metadata = c57_nos2KO_mouse_metadata, variable = "Treatment", color = "Treatment", response_variable = "Metabolite")+ theme_bw() + theme(panel.grid = element_blank())This should make the following figure:
## Loading required package: ggplot2
Random Forest
Omu has a function, random_forest, which is a wrapper
built around the function randomForest from the R package
randomForest. The function returns a list which has the following
components: rf list from randomForest, training data, testing data,
metabolite metadata, and if a classificaton confusion matrices for the
training data and testing data. Variable importance plots and PCA plots
of the proximity matrix can be performed using
plot_variable_importance and plot_rf_PCA
respectively, which will produce ggplot2 objects. plot_rf_PCA is only
compatible with classification models. If you wish to tune
hyperparameters you will need to take the code and edit the function to
do so, and would only involve editing the line where randomForest is
called. Otherwise keep in mind that outside of the number of decision
trees to make, this funciton is running on default model parameters
which may not be sufficient for your data depending on your sample sizes
and ratio of observations to variables.
Modeling with Univariate Statistics
Prior to modeling the data, users can use the transform functions to
make their data more appropriate for the models.
transform_samples will perform column-wise transformations
across the datausing the supplied function. This is useful for
operations such as log transformation, or transforming by the square
root. transform metabolites transforms the data using the
supplied function across rows. This is useful for operations like
mean-centering and pareto scaling. Omu supports two univariate
statistical models, t test and anova, using the functions
omu_summary and anova_function respectively.
Both functions will output p values and adjusted p values, while
omu_summary will also output group means, standard error,
standard deviation, fold change, and log2foldchange. Both of these
models are useful for observing relationships between independent
variables in an experiment. The dataframe created using the
assign_hierarchy function can be used in the count_data
argument of omu_summary to run statistics on it. The output
of omu_summary will be needed in order to use the plotting
functions in Omu. The metadata that comes with the package,
c57_nos2KO_mouse_metadata, must be used for the
metadata argument. A comparison between the “Strep” group
within the “Treatment” factor against the “Mock” group can be done to
observe if antibiotic treatment of the mice had an effect on the
metabolome. The response_variable is the Metabolite column
of the data frame. The data can be log transformed using
log_transform = TRUE, and a p value adjustment method of
Benjamini & Hochberg with the argument p_adjust = "BH".
Alternatively, any adjustment method for the p.adjust
function that comes with R stats can be used. The test_type
argument is one of “students”, “welch”, or “mwu” for a students t test,
welch’s t test, or man whitney u test respectively. Paired tests for
each test type can be performed by setting the parameter
paired = TRUE. This parameter is set to FALSE by
default.
DF_stats <- omu_summary(count_data = DF, metadata = c57_nos2KO_mouse_metadata, numerator = "Strep", denominator = "Mock", response_variable = "Metabolite", Factor = "Treatment", log_transform = TRUE, p_adjust = "BH", test_type = "welch")The output should look like this:
## [1] "Number of zero values is below threshold across all metabolites."| Metabolite | Strep.mean | Mock.mean | Fold_Change | log2FoldChange | t_value |
|---|---|---|---|---|---|
| 1,2_anhydro_myo_inositol_NIST | 3077.154 | 1974.438 | 1.558496 | 0.6401546 | -1.2195381 |
| 1,5_anhydroglucitol | 13141.462 | 1640.125 | 8.012476 | 3.0022481 | -5.8626811 |
| 100253 | 1979.923 | 1930.500 | 1.025601 | 0.0364698 | 0.0410241 |
with columns of adjusted p values (“padj”), log2FoldChange, standard
error, and standard deviation for each of the metabolites. From here,
this data frame can be used to create bar plots, volcano plots, or pie
charts (see Data Visualization), or used in KEGG_gather to
get functional orthologies and gene info for the metabolites.
An alternative option to omu_summary is the
omu_anova, which can be used to measure the variance of all
groups within a factor, or see if independent variables have an effect
on one another by modeling an interaction term (this only applies to
multi factorial datasets). This function also performs a tukeys test
following the anova, as well as calculating group means and fold changes
for each contrast in the tukeys test.omu_anova has five
arguments, three of which are required: count data, metadata, and a
model formula (see ?formula in R for more information on how model
formulas work). The function supports any number of factors, or
interactions a user wishes to include in their model, and will return a
list of dataframes, where each dataframe is one of the possible
contrasts in the users model, along with a data frame containing model
residuals for each response variable. When providing a formula for the
model argument, make sure to leave the left side blank, as the function
will supply the left side while running the model on each response
variable in the dataset.
DF_anova <- omu_anova(count_data = c57_nos2KO_mouse_countDF, metadata = c57_nos2KO_mouse_metadata, response_variable = "Metabolite", model = ~ Treatment")The output is similar to omu_summary so as to be compatible with graphing functions.
An alternative to doing an anova model with an interaction statement is to paste factor groups together using base R to make a new metadata column to be able to model the effect of treatment within mouse genetic backgrounds. For example, base R can be used to make a new “Grouped” Factor, with 4 levels; WTMock, WTStrep, Nos2Mock, and Nos2Strep.
c57_nos2KO_mouse_metadata$Grouped <- factor(paste0(c57_nos2KO_mouse_metadata$Background, c57_nos2KO_mouse_metadata$Treatment))This should produce a meta data file that looks like this :
| Sample | Background | Treatment | Grouped |
|---|---|---|---|
| C289_1 | WT | Mock | WTMock |
| C289_2 | WT | Mock | WTMock |
| C289_3 | WT | Mock | WTMock |
| C289_4 | WT | Mock | WTMock |
The function omu_summary can be used to model the effect
of strep treatment on the wild type mouse metabolome (excluding the
mutant background from the model), by using the “Grouped” column for the
Factor argument, WTStrep for the numerator
argument, and WTMock for the denominator argument:
DF_stats_grouped <- omu_summary(count_data = c57_nos2KO_mouse_countDF, metadata = c57_nos2KO_mouse_metadata, numerator = "WTStrep", denominator = "WTMock", response_variable = "Metabolite", Factor = "Grouped", log_transform = TRUE, p_adjust = "BH", test_type = "welch")Producing this data frame:
## [1] "Number of zero values is below threshold across all metabolites."| Metabolite | WTStrep.mean | WTMock.mean | Fold_Change | log2FoldChange | t_value |
|---|---|---|---|---|---|
| 1,2_anhydro_myo_inositol_NIST | 2470.750 | 2007.667 | 1.2306573 | 0.2994290 | -0.7164102 |
| 1,5_anhydroglucitol | 11699.625 | 1546.583 | 7.5648219 | 2.9193061 | -6.4189006 |
| 100253 | 1784.625 | 1929.000 | 0.9251555 | -0.1122322 | 1.0714548 |
Gathering Functional Orthology and Gene Data
To gather functional orthology and gene data, Omu uses an S3 method
called KEGG_gather, which retrieves data from the KEGG API
using the function keggGet from the package KEGGREST, and
cleans it up into a more readable format as new columns in the input
data frame. KEGG_gather can recognizes a second class assigned to the
data frame, which changes based on what metadata columns your data has
acquired. This means that one can simply use the function
KEGG_gather, regardless of what data you want to collect.
For advanced users, additional methods and classes can be added to
KEGG_gather if something other than functional orthologies
and genes is desired. This can be done by altering the variables that
are fed into the internal make_omelette function and by
creating a new plate_omelette method that appropriately
cleans up the data.
It is recommended to subset the input data frame before using
KEGG_gather, as compounds can have multiple functional
orthologies associated with them. The data frame created from using
omu_summary can be subsetted to Organic acids only using
base R’s subset function. We can then subset based on
significance as well.
DF_stats_sub <- subset(DF_stats, Class=="Organic acids")
DF_stats_sub <- DF_stats_sub[which(DF_stats_sub[,"padj"] <= 0.05),]Now the data frame should contain only compounds that are Organic acids, and had adjusted p values lower than or equal to 0.05.
| Metabolite | log2FoldChange | padj | KEGG | C289_1 | Class | |
|---|---|---|---|---|---|---|
| 300 | 2,8_dihydroxyquinoline | -1.8223032 | 0.0012274 | C06342 | 10021 | Organic acids |
| 321 | 2_hydroxyglutaric_acid | -2.1012945 | 0.0276745 | C02630 | 3721 | Organic acids |
| 368 | 3_(3_hydroxyphenyl)propionic_acid | -7.1575036 | 0.0000000 | C11457 | 113181 | Organic acids |
| 369 | 3_(4_hydroxyphenyl)propionic_acid | -4.8857705 | 0.0000001 | C01744 | 78913 | Organic acids |
| 399 | 4_hydroxybutyric_acid | 0.6380038 | 0.0444984 | C00989 | 315 | Organic acids |
KEGG_gather can then be used to get the functional orthologies for these compounds.:
DF_stats_sub_KO <- KEGG_gather(DF_stats_sub)From here, the user can gather orthology metadata and gene metadata
from the KEGG API, using KEGG_gather again. Additionally,
assign_hierarchy can be used on Orthology identifiers and
organism identifiers for genes generated from KEGG_gather
to assign enzyme metadata and organism metadata respectively. This
metadata can then help the end user subset their data.frame to pathways
and/or organisms of interest related to metabolits that were
significantly different between treatment groups in their data for
hypothesis generation.
Data Visualization
Bar Plots
The plot_bar function can be used to make bar plots of
metabolite counts by their class meta data (from
assign_hierarchy). To make a bar plot, a data frame of the
number of significantly changed compounds by a hierarchy class must be
created. This can be done using the output from omu_summary
as an input for the function count_fold_changes, to make a
data frame with the number of compounds that significantly increased or
decreased per a hierarchy group. For this data frame, the argument
column = "Class" can be used to generate counts for the
Class level of compound hierarchy.
DF_stats_counts <- count_fold_changes(count_data = DF_stats, column = "Class", sig_threshold = 0.05)This should generate a data frame with 3 columns that show Class, number of compounds within that class that changed, and whether they increased or decreased.
| Class | Significant_Changes | color |
|---|---|---|
| Carbohydrates | 23 | Increase |
| Lipids | 3 | Increase |
| Organic acids | 9 | Increase |
| Peptides | 4 | Increase |
| Nucleic acids | 2 | Increase |
| Vitamins and Cofactors | 1 | Increase |
| Phytochemical compounds | 3 | Increase |
| Carbohydrates | -10 | Decrease |
| Lipids | -20 | Decrease |
| Organic acids | -11 | Decrease |
| Peptides | -13 | Decrease |
| Nucleic acids | -5 | Decrease |
| Vitamins and Cofactors | -1 | Decrease |
| Phytochemical compounds | -4 | Decrease |
This count data frame can be used as an input for the
plot_bar function:
library(ggplot2)
Class_Bar_Plot <- plot_bar(fc_data = DF_stats_counts, fill = c("dodgerblue2", "firebrick2"), outline_color = c("black", "black"), size = c(1,1)) + labs(x = "Class") + theme(panel.grid = element_blank())This should generate a plot that looks like this:
The argument fill is the color of the bars,
outline_color is the outline, and size is the
width of the bar outline. Colors are picked in alphanumeric order, so
the first item in each character vector corresponds to the “Decrease”
column and the second corresponds to the “Increase” column. The figure
is a ggplot2 object, so it is compatible with any ggplot2 themes you
wish to use to edit the appearance. An example of this is in the code
above:
labs(x = "Class") + theme(panel.grid = element_blank()),
and was used to clean up the figures appearance by giving it a
descriptive x axis label, and removing the grid lines from the
background.
Pie Charts
It is also possible to make a pie_chart from our counts data frame
instead of a bar plot. First, a frequency data frame (percentage values)
must be made from the count data frame using the ra_table
function:
DF_ra <- ra_table(fc_data = DF_stats_counts, variable = "Class")This should generate a data frame with percentages of compounds that increased significantly, decreased significantly, or changed significantly (either increased of decreased):
| Class | Significant_Changes | Decrease | Increase |
|---|---|---|---|
| Carbohydrates | 30.275229 | 15.6250 | 51.111111 |
| Lipids | 21.100917 | 31.2500 | 6.666667 |
| Nucleic acids | 6.422018 | 7.8125 | 4.444444 |
| Organic acids | 18.348624 | 17.1875 | 20.000000 |
| Peptides | 15.596330 | 20.3125 | 8.888889 |
| Phytochemical compounds | 6.422018 | 6.2500 | 6.666667 |
| Vitamins and Cofactors | 1.834862 | 1.5625 | 2.222222 |
This frequency data frame can be used in the pie_chart
function:
Pie_Chart <- pie_chart(ratio_data = DF_ra, variable = "Class", column = "Decrease", color = "black")This should make a pie chart showing the percent of compounds that decreased per class level:
Volcano Plots
Omu can generate volcano plots using the output from
omu_summary and the function plot_volcano.
This function gives the user the option to highlight data points in the
plot by their hierarchy meta data (i.e. Class, Subclass_1, etc.) For
example, a Volcano plotcan be made that highlights all of the compounds
that are either Organic acids or Carbohydrates with the argument
strpattern = c("Organic acids", "Carbohydrates").
fill determines the color of the points, color
determines the outline color of the points, alpha sets the
level of transparency (with 1 being completely opaque),
size sets the size of the points, and shape
takes integers that correspond to ggplot2 shapes. For fill, color,
alpha, and shape the character vectors must be a length of n +1, with n
being the number of meta data levels that are going to be highlighted.
When picking color, fill, alpha, and shape, the values are ordered
alphanumerically, and anything not listed in the “strpattern” argument
is called “NA”. If the strpattern argument is not used, all
points below the chosen sig_threshold value will be filled
red. If sig_threshold is not used, a dashed line will be
drawn automatically for an adjusted p value of 0.05:
Volcano_Plot <- plot_volcano(count_data = DF_stats, size = 2, column = "Class", strpattern = c("Organic acids, Carbohydrates"), fill = c("firebrick2","white","dodgerblue2"), color = c("black", "black", "black"), alpha = c(1,1,1), shape = c(21,21,21)) + theme_bw() + theme(panel.grid = element_blank())This will give us the following plot:
PCA Plots
Omu also supports multivariate statistical analysis and visualization
in the form of principle component analysis. To do this one only needs
to have their metabolomics count data and meta data in the proper
format. It is recommended to deal with overdispersion of data prior to
using PCA_plot, by transformation via natural log, sqrt,
etc.
A PCA plot can be made showing the relationship between Treatment groups in the package dataset:
c57_nos2KO_mouse_countDF_log <- c57_nos2KO_mouse_countDF
c57_nos2KO_mouse_countDF_log <- log(c57_nos2KO_mouse_countDF_log[,3:31])
c57_nos2KO_mouse_countDF_log <- cbind(c57_nos2KO_mouse_countDF[,1:2], c57_nos2KO_mouse_countDF_log)
PCA <- PCA_plot(count_data = c57_nos2KO_mouse_countDF_log, metadata = c57_nos2KO_mouse_metadata, variable = "Treatment", color = "Treatment", response_variable = "Metabolite")+ theme_bw() + theme(panel.grid = element_blank())This should make the following figure:
Heatmaps
Heatmaps can be generated using plot_heatmap on a
dataframe that has not been transformed by omu_summary or
omu_anova. It gives the user the option of aggregating
their metabolite data by metabolite Class or Subclass with the argument
aggregate_by. If unused, the heatmap will include every
individual metabolite in the users count data. log transformation is
recommended but optional, and if TRUE will transform the data by the
natural log.
To avoid an overly noisy plot, its recommended that you either subset to metabolites within a class of interest, or aggregate metabolites by a class of interest. For example, using the data frame from the start of our analysis with compound hierarchy assigned:
DF <- assign_hierarchy(count_data = c57_nos2KO_mouse_countDF, keep_unknowns = TRUE, identifier = "KEGG")
heatmap_class <- plot_heatmap(count_data = DF, metadata = c57_nos2KO_mouse_metadata, Factor = "Treatment", response_variable = "Metabolite", log_transform = TRUE, high_color = "goldenrod2", low_color = "midnightblue", aggregate_by = "Class") + theme(axis.text.x = element_text(angle = 30, hjust=1, vjust=1, size = 6), axis.text.y = element_text(size = 6))
This code should generate the following heatmap:
We can subset the data to a Class of interest, such as Carbohydrates, and then either plot all individual carbohydrates or aggregate them by a subclass:
DF <- assign_hierarchy(count_data = c57_nos2KO_mouse_countDF, keep_unknowns = TRUE, identifier = "KEGG")
DF_carbs <- subset(DF, Class == "Carbohydrates")
heatmap_carbs <- plot_heatmap(count_data = DF_carbs, metadata = c57_nos2KO_mouse_metadata, Factor = "Treatment", response_variable = "Metabolite", log_transform = TRUE, high_color = "goldenrod2", low_color = "midnightblue") + theme(axis.text.x = element_text(angle = 30, hjust=1, vjust=1, size = 6))
DF_carbs <- subset(DF, Class == "Carbohydrates")
heatmap_carbs_sc2 <- plot_heatmap(count_data = DF_carbs, metadata = c57_nos2KO_mouse_metadata, Factor = "Treatment", response_variable = "Metabolite", log_transform = TRUE, high_color = "goldenrod2", low_color = "midnightblue", aggregate_by = "Subclass_2") + theme(axis.text.x = element_text(angle = 30, hjust=1, vjust=1, size = 6), axis.text.y = element_text(size = 6))
Boxplots
Boxplots of metabolite abundance by experiment group can be generated
using the function plot_boxplot with a count data frame
that has not been transformed by omu_summary or
omu_anova. The function will produce a boxplot of every
metabolite in your dataframe, so it may be best to subset the dataframe
by compound class, similar to what we did with
plot_heatmap. Like plot_heatmap, it also
provides the option to aggregate by compound class or subclass. If
log_transform = TRUE the data will be transformed by the
natural log.
DF_carbs_trunc <- DF_carbs[1:10,]
boxplot_carbs <- plot_boxplot(count_data = DF_carbs_trunc, metadata = c57_nos2KO_mouse_metadata, log_transform = TRUE, Factor = "Treatment", response_variable = "Metabolite", fill_list = c("darkgoldenrod1", "dodgerblue2"))
Alternatively, we could aggregate the dataset containing
carbohydrates only by Subclass_2, or aggregate the full
dataset by Class.
boxplot_carbs_sc2 <- plot_boxplot(count_data = DF_carbs, metadata = c57_nos2KO_mouse_metadata, log_transform = TRUE, Factor = "Treatment", response_variable = "Metabolite", fill_list = c("darkgoldenrod1", "dodgerblue2"), aggregate_by = "Subclass_2")
boxplot_class <- plot_boxplot(count_data = DF, metadata = c57_nos2KO_mouse_metadata, log_transform = TRUE, Factor = "Treatment", response_variable = "Metabolite", fill_list = c("darkgoldenrod1", "dodgerblue2"), aggregate_by = "Class")