The goal of
proDA is to identify differentially abundant proteins in label-free
mass spectrometry data. The main challenge of this data are the many missing values.
The missing values don’t occur randomly but especially at low intensities. This
means that they cannot just be ignored. Existing methods have mostly focused on
replacing the missing values with some reasonable number (“imputation”) and then
run classical methods. But imputation is problematic because it obscures the
amount of available information. Which in turn can lead to over-confident
proDA on the other hand does not impute missing values, but constructs a
probabilistic dropout model. For each sample it fits a sigmoidal dropout
curve. This information can then be used to infer means across samples and the
associated uncertainty, without the intermediate imputation step.
supports full linear models with variance and location moderation.
For full details, please see our preprint:
Constantin Ahlmann-Eltze and Simon Anders: proDA: Probabilistic Dropout Analysis for Identifying Differentially Abundant Proteins in Label-Free Mass Spectrometry. biorXiv 661496 (Jun 2019)
proDA is implemented as an R package.
You can install it from Bioconductor by typing the following commands into R:
if(!requireNamespace("BiocManager", quietly = TRUE)) install.packages("BiocManager") BiocManager::install("proDA")
# install.packages("devtools") devtools::install_github("const-ae/proDA")
The pkgdown documentation for the package is available on https://const-ae.github.io/proDA/reference.
In the following section, I will give a very brief overview on the main
functionality of the
proDA package, aimed at experienced R users.
New users are advised to skip this “quickstart” and to go directly
to section 1.3, where I give a complete walkthrough and explain in
detail, what steps are necessary for the analysis of label-free mass
The three steps that are necessary to analyze the data are
# Load the package library(proDA) # Generate some dataset with known structure syn_dataset <- generate_synthetic_data(n_proteins = 100, n_conditions = 2) # The abundance matrix syn_dataset$Y[1:5, ] #> Condition_1-1 Condition_1-2 Condition_1-3 Condition_2-1 Condition_2-2 Condition_2-3 #> protein_1 19.17814 NA 18.89003 19.90698 NA 18.83656 #> protein_2 NA NA NA NA NA NA #> protein_3 23.89169 24.03214 23.73394 23.54467 23.57230 23.92561 #> protein_4 20.94756 21.03668 20.76283 20.51360 21.11377 20.66439 #> protein_5 19.44029 19.74747 19.29078 19.55662 19.28023 19.75506 # Assignment of the samples to the two conditions syn_dataset$groups #>  Condition_1 Condition_1 Condition_1 Condition_2 Condition_2 Condition_2 #> Levels: Condition_1 Condition_2 # Fit the probabilistic dropout model fit <- proDA(syn_dataset$Y, design = syn_dataset$groups) # Identify which proteins differ between Condition 1 and 2 test_diff(fit, `Condition_1` - `Condition_2`, sort_by = "pval", n_max = 5) #> # A tibble: 5 x 10 #> name pval adj_pval diff t_statistic se df avg_abundance n_approx n_obs #> <chr> <dbl> <dbl> <dbl> <dbl> <dbl> <dbl> <dbl> <dbl> <dbl> #> 1 protein_99 0.0000518 0.00518 -6.71 -18.4 0.365 4 22.4 4.96 5 #> 2 protein_91 0.000125 0.00624 -2.33 -14.7 0.158 4 20.4 6.00 6 #> 3 protein_100 0.00195 0.0649 4.74 7.23 0.657 4 20.5 3.07 3 #> 4 protein_96 0.00415 0.104 -1.69 -5.89 0.287 4 21.9 6.00 6 #> 5 protein_92 0.00674 0.135 0.933 5.15 0.181 4 20.6 6.00 6
Other helpful functions for quality control are
proDA is an R package that implements a powerful probabilistic dropout model
to identify differentially abundant proteins. The package was specifically designed
for label-free mass spectrometry data and in particular how to handle the many
many missing values.
But all this is useless if you cannot load your data and get it into a shape that is useable. In the next section, I will explain how to load the abundance matrix and bring it into a useful form. The steps that I will go through are
proteinGroups.txtMaxQuant output table
NAs and take the
log2()of the data
I will now demonstrate how to load a MaxQuant output file. For more information about other approaches for loading the data, please take a look at the vignette on loading data.
MaxQuant is one of the most popular tools for handling raw MS data. It produces
a number of files. The important file that contains the protein intensities is
proteinGroups.txt. It is a large table with detailed information about
the identification and quantification process for each protein group (which I will
from now on just call “protein”).
This package comes with an example
proteinGroups.txt file, located in the
package folder. The file contains the reduced output from an experiment studying the different
DHHCs in Drosophila melanogaster.
system.file("extdata/proteinGroups.txt", package = "proDA", mustWork = TRUE) #>  "/tmp/RtmpVghisb/Rinstc555314b50183/proDA/extdata/proteinGroups.txt"
In this example, I will use the base R functions to load the data, because they don’t require any additional dependencies.
# Load the table into memory maxquant_protein_table <- read.delim( system.file("extdata/proteinGroups.txt", package = "proDA", mustWork = TRUE), stringsAsFactors = FALSE )
As I have mentioned, the table contains a lot of information (359 columns!!), but we are first of all interested in the columns which contain the measured intensities.
# I use a regular expression (regex) to select the intensity columns intensity_colnames <- grep("^LFQ\\.intensity\\.", colnames(maxquant_protein_table), value=TRUE) head(intensity_colnames) #>  "LFQ.intensity.CG1407.01" "LFQ.intensity.CG1407.02" "LFQ.intensity.CG1407.03" #>  "LFQ.intensity.CG4676.01" "LFQ.intensity.CG4676.02" "LFQ.intensity.CG4676.03" # Create the intensity matrix abundance_matrix <- as.matrix(maxquant_protein_table[, intensity_colnames]) # Adapt column and row maxquant_protein_table colnames(abundance_matrix) <- sub("^LFQ\\.intensity\\.", "", intensity_colnames) rownames(abundance_matrix) <- maxquant_protein_table$Protein.IDs # Print some rows of the matrix with short names so they fit on the screen abundance_matrix[46:48, 1:6] #> CG1407.01 CG1407.02 CG1407.03 CG4676.01 CG4676.02 CG4676.03 #> A0A0B4K6W1;P08970 713400 845440 0 0 1032600 0 #> A0A0B4K6W2;A0A0B4K7S0;P55824-3;P55824 5018800 4429500 2667200 0 8780200 1395800 #> A0A0B4K6X7;A1Z8J0 0 0 0 0 0 0
After extracting the bits from the table we most care about, we will have to modify it.
Firstly, MaxQuant codes missing values as
0. This is misleading, because the actual
abundance probably was not zero, but just some value too small to be detected by the mass spectrometer.
Accordingly, I will replace all
Secondly, the raw intensity values have a linear mean-variance relation. This is undesirable, because
a change of
x units can be a large shift if the mean is small or irrelevant if the mean is large.
Luckily, to make the mean and variance independent, we can just
log the intensities. Now a change
x units is as significant for highly abundant proteins, as it is for low abundant ones.
abundance_matrix[abundance_matrix == 0] <- NA abundance_matrix <- log2(abundance_matrix) abundance_matrix[46:48, 1:6] #> CG1407.01 CG1407.02 CG1407.03 CG4676.01 CG4676.02 CG4676.03 #> A0A0B4K6W1;P08970 19.44435 19.68934 NA NA 19.97785 NA #> A0A0B4K6W2;A0A0B4K7S0;P55824-3;P55824 22.25891 22.07871 21.34689 NA 23.06582 20.41266 #> A0A0B4K6X7;A1Z8J0 NA NA NA NA NA NA
Quality control (QC) is essential for a successful bioinformatics analysis, because any dataset shows some unwanted variation or could even contain more serious error like for example a sample swap.
Often we start with normalizing the data to remove potential sample specific effects. But already this step is challenging, because the missing values cannot easily be corrected for. Thus, a first helpful plot is to look how many missing values are in each sample.
barplot(colSums(is.na(abundance_matrix)), ylab = "# missing values", xlab = "Sample 1 to 36")
We can see that the number of missing values differs substantially between samples (between 30% and 90%) in this dataset. If we take a look at the intensity distribution for each sample, we see that they differ substantially as well.
boxplot(abundance_matrix, ylab = "Intensity Distribution", xlab = "Sample 1 to 36")
Note that, the intensity distribution is shifted upwards for samples which also have a large number of missing values (for example the last one). This agrees with our idea that small values are more likely to be missing. On the other hand, this also demonstrates why normalization methods such as quantile normalization, which distort the data until all the distributions are equal, are problematic. I will apply the more “conservative” median normalization, which ignores the missing values and transforms the values so that the median difference between the sample and average across all other samples is zero.
normalized_abundance_matrix <- median_normalization(abundance_matrix)
An important tool to identify sample swaps and outliers in the dataset is to look at the sample distance matrix. It shows the distances of samples A to B, A to C, B to C and so on.
The base R
dist() function can not handle input data that contains missing values, so we might be
tempted to just replace the missing values with some realistic numbers and calculate the distance
completed dataset. But choosing a good replacement value is challenging and can also be misleading
because the samples with many missing values would be considered too close.
proDA provides the
dist_approx() function that takes either a fitted model (ie. the
proDA()) or a simple matrix (for which it internally calls
estimates the expected distance without imputing the missing values. In addition, it reports
the associated uncertainty with every estimate. The estimates for samples with many missing
values will be uncertain, allowing the data analyst to discount them.
da <- dist_approx(normalized_abundance_matrix)
dist_approx() returns two elements the
mean of the estimate and the associated
In the next step I will plot the heatmap for three different conditions, adding the 95% confidence
interval as text to each cell.
# This chunk only works if pheatmap is installed # install.packages("pheatmap") sel <- c(1:3, # CG1407 7:9, # CG59163 22:24)# CG6618 plot_mat <- as.matrix(da$mean)[sel, sel] # Remove diagonal elements, so that the colorscale is not distorted plot_mat[diag(9) == 1] <- NA # 95% conf interval is approx `sd * 1.96` uncertainty <- matrix(paste0(" ± ",round(as.matrix(da$sd * 1.96)[sel, sel], 1)), nrow=9) pheatmap::pheatmap(plot_mat, cluster_rows = FALSE, cluster_cols = FALSE, display_numbers= uncertainty, number_color = "black")
In the next step, we will fit the actual linear probabilistic dropout model to the normalized data. But before we start, I will create a data.frame that contains some additional information on each sample, in particular to which condition that sample belongs.
# The best way to create this data.frame depends on the column naming scheme sample_info_df <- data.frame(name = colnames(normalized_abundance_matrix), stringsAsFactors = FALSE) sample_info_df$condition <- substr(sample_info_df$name, 1, nchar(sample_info_df$name) - 3) sample_info_df$replicate <- as.numeric( substr(sample_info_df$name, nchar(sample_info_df$name) - 1, 20) ) sample_info_df #> # A tibble: 36 x 3 #> name condition replicate #> <chr> <chr> <dbl> #> 1 CG1407.01 CG1407 1 #> 2 CG1407.02 CG1407 2 #> 3 CG1407.03 CG1407 3 #> 4 CG4676.01 CG4676 1 #> 5 CG4676.02 CG4676 2 #> 6 CG4676.03 CG4676 3 #> 7 CG51963.01 CG51963 1 #> 8 CG51963.02 CG51963 2 #> 9 CG51963.03 CG51963 3 #> 10 CG5620A.01 CG5620A 1 #> # … with 26 more rows
Now we can call the
proDA() function to actually fit the model. We specify the
the formula notation, referencing the
condition column in the
sample_info_df data.frame that
we have just created. In addition, I specify that I want to use the
S2R condition as the reference
because I know that it was the negative control and this way automatically all coefficients
measure how much each condition differs from the negative control.
fit <- proDA(normalized_abundance_matrix, design = ~ condition, col_data = sample_info_df, reference_level = "S2R") fit #> Parameters of the probabilistic dropout model #> #> The dataset contains 36 samples and 122 proteins #> 59.7% of the values are missing #> #> Experimental design: y~condition #> The model has successfully converged. #> #> The inferred parameters are: #> location_prior_mean: 19.5 #> location_prior_scale: 8.37 #> location_prior_df: 3 #> variance_prior_scale: 0.283 #> variance_prior_df: 1.64 #> dropout_curve_position: 19.9, 19, 20.1, 22.8, ... #> dropout_curve_scale: -0.816, -0.601, -1.02, -1.31, ...
proDAFit object prints a number of useful information about the convergence of the model,
the size of the dataset, the number of missing values, and the inferred hyper parameters.
To make it easy to find available methods on the
proDAFit object, the
$-operator is overloaded
and shows a list of possible functions:
# Equivalent to feature_parameters(fit) fit$feature_parameters #> # A tibble: 122 x 4 #> n_approx df s2 n_obs #> <dbl> <dbl> <dbl> <dbl> #> 1 12.0 0.001 3808. 5 #> 2 12.0 0.001 2439. 1 #> 3 19.3 8.93 4.07 14 #> 4 12.0 0.001 850. 6 #> 5 17.4 7.04 0.470 17 #> 6 12.0 0.001 2472. 1 #> 7 12.0 0.001 2410. 1 #> 8 28.9 18.6 0.217 29 #> 9 12.0 0.001 1798. 4 #> 10 12.0 0.001 1881. 4 #> # … with 112 more rows
proDAFit object is implemented as a subclass of
This means it can be subsetted, which is for example useful for calculating the distance
of a subset of proteins and samples.
# This chunk only works if pheatmap is installed # install.packages("pheatmap") pheatmap::pheatmap(dist_approx(fit[1:20, 1:3], by_sample = FALSE)$mean)
Lastly, we will use a Wald test to identify in which proteins a coefficient is significantly different
from zero. The
test_diff() function takes first the fit object produced by
proDA() and a
contrast argument. This can either be a string or an expression if we want to test more complex
combinations. For example
conditionCG1407 - (conditionCG6017 + conditionCG5880) / 2 would test
for the difference between CG1407 and the average of CG6017 and CG5880.
test_diff() also supports likelihood ratio F-tests. In that case instead of the
argument specify the
# Test which proteins differ between condition CG1407 and S2R # S2R is the default contrast, because it was specified as the `reference_level` test_res <- test_diff(fit, "conditionCG1407") test_res #> # A tibble: 122 x 10 #> name pval adj_pval diff t_statistic se df avg_abundance n_approx n_obs #> <chr> <dbl> <dbl> <dbl> <dbl> <dbl> <dbl> <dbl> <dbl> <dbl> #> 1 Q8IP47;Q9VJP8;Q9V43… 0.904 0.964 -0.132 -0.122 1.08 24 18.9 12.0 5 #> 2 A0A023GPV6;A8JV04;Q… 0.923 0.964 -0.0992 -0.0978 1.01 24 18.4 12.0 1 #> 3 A0A023GQA5;P24156 0.0356 0.265 -2.92 -2.23 1.31 24 19.3 19.3 14 #> 4 Q1RKY1;A0A0B4LG19;A… 0.667 0.964 0.632 0.435 1.45 24 18.7 12.0 6 #> 5 A0A0B4JD00;A8DY69;I… 0.919 0.964 0.0691 0.103 0.670 24 20.0 17.4 17 #> 6 A0A0B4JCT8;Q9V780 0.923 0.964 -0.0994 -0.0980 1.01 24 18.5 12.0 1 #> 7 A0A0B4LHQ4;A0A0B4JD… 0.923 0.964 -0.0990 -0.0977 1.01 24 18.4 12.0 1 #> 8 A0A0B4JCW4;Q9VHJ8;Q… 0.643 0.964 -0.197 -0.469 0.419 24 21.9 28.9 29 #> 9 Q9VDV4;A0A0B4JCY1;Q… 0.295 0.860 1.95 1.07 1.82 24 18.7 12.0 4 #> 10 A0A0B4JCY6;Q7KSF4;A… 0.598 0.964 -0.783 -0.535 1.46 24 19.0 12.0 4 #> # … with 112 more rows
This walkthrough ends with the identification which proteins are differentially abundant. But for a real dataset, now the actual analysis only just begins. A list of significant proteins is hardly ever a publishable result, one often needs to make sense what the relevant underlying biological mechanisms are. But for this problem other tools are necessary, which depend on the precise question associated with the biological problem at hand.
sessionInfo() #> R version 4.1.0 (2021-05-18) #> Platform: x86_64-pc-linux-gnu (64-bit) #> Running under: Ubuntu 20.04.2 LTS #> #> Matrix products: default #> BLAS: /home/biocbuild/bbs-3.13-bioc/R/lib/libRblas.so #> LAPACK: /home/biocbuild/bbs-3.13-bioc/R/lib/libRlapack.so #> #> locale: #>  LC_CTYPE=en_US.UTF-8 LC_NUMERIC=C LC_TIME=en_GB #>  LC_COLLATE=C LC_MONETARY=en_US.UTF-8 LC_MESSAGES=en_US.UTF-8 #>  LC_PAPER=en_US.UTF-8 LC_NAME=C LC_ADDRESS=C #>  LC_TELEPHONE=C LC_MEASUREMENT=en_US.UTF-8 LC_IDENTIFICATION=C #> #> attached base packages: #>  stats graphics grDevices utils datasets methods base #> #> other attached packages: #>  proDA_1.6.0 BiocStyle_2.20.0 #> #> loaded via a namespace (and not attached): #>  SummarizedExperiment_1.22.0 xfun_0.23 bslib_0.2.5.1 #>  lattice_0.20-44 colorspace_2.0-1 vctrs_0.3.8 #>  htmltools_0.5.1.1 stats4_4.1.0 yaml_2.2.1 #>  utf8_1.2.1 rlang_0.4.11 jquerylib_0.1.4 #>  pillar_1.6.1 BiocGenerics_0.38.0 RColorBrewer_1.1-2 #>  matrixStats_0.58.0 GenomeInfoDbData_1.2.6 lifecycle_1.0.0 #>  stringr_1.4.0 MatrixGenerics_1.4.0 zlibbioc_1.38.0 #>  munsell_0.5.0 gtable_0.3.0 evaluate_0.14 #>  Biobase_2.52.0 knitr_1.33 IRanges_2.26.0 #>  ps_1.6.0 GenomeInfoDb_1.28.0 parallel_4.1.0 #>  fansi_0.4.2 highr_0.9 Rcpp_1.0.6 #>  scales_1.1.1 BiocManager_1.30.15 DelayedArray_0.18.0 #>  S4Vectors_0.30.0 magick_2.7.2 jsonlite_1.7.2 #>  XVector_0.32.0 digest_0.6.27 stringi_1.6.2 #>  bookdown_0.22 GenomicRanges_1.44.0 grid_4.1.0 #>  cli_2.5.0 tools_4.1.0 bitops_1.0-7 #>  magrittr_2.0.1 sass_0.4.0 RCurl_1.98-1.3 #>  tibble_3.1.2 crayon_1.4.1 pkgconfig_2.0.3 #>  ellipsis_0.3.2 pheatmap_1.0.12 Matrix_1.3-3 #>  rmarkdown_2.8 extraDistr_1.9.1 rstudioapi_0.13 #>  R6_2.5.0 compiler_4.1.0