Quantifying drug response is the cornerstone of many pharmacological experiments ranging from pharmacogenomics studies to small-scale analyses of drug resistance. In general, cells are grown in the presence or absence of drugs for a few days and the endpoint cell count values (or a surrogate) is compared. From the relative cell count, metrics of drug sensitivity such as IC50 or Emax values are evaluated. In cases where the untreated control cells grow over the course of the assay, these traditional metrics are confounded by the number of divisions that take place over the course of an assay. In particular, for drugs that impact growth rate and block cell division, slow-growing cell lines will appear more resistant than fast-growing lines although the biological effect on a per-division basis may be the same.
Hafner et al. recently proposed alterative drug-response metrics based on growth rate inhibition (GR metrics) that are robust to differences in nominal division rate and assay duration. Using these metrics requires only to know the number of cells (or a surrogate) at the time of treatment; note that this value may also be inferred from the nominal division rate and the value of an untreated sample at the endpoint.
To facilitate the use of these GR metrics, we have developed an R package that provides functions to analyze and visualize drug response data with these new metrics across multiple conditions and cell lines.
The GRmetrics package can be installed through Bioconductor
if (!requireNamespace("BiocManager", quietly=TRUE))
install.packages("BiocManager")
BiocManager::install("GRmetrics")
#References: Hafner, M., Niepel, M. Chung, M. and Sorger, P.K., Growth Rate Inhibition Metrics Correct For Confounders In Measuring Sensitivity To Cancer Drugs. Nature Methods 13.6 (2016): 521-527. (http://dx.doi.org/10.1038/nmeth.3853)
Corresponding MATLAB and Python scripts available on repo:
https://github.com/sorgerlab/gr50_tools.
Note: Most, but not all of these scripts have been reproduced in this R package. Namely, this package does not contain code for “Case B” of the MATLAB scripts nor does it contain an R script to generate the example input data. The python script for generating the example data can be found in the “inst/scripts/” directory.
Browser interface and online tools: http://www.grcalculator.org
Much of the description below has been adapted from:
https://github.com/datarail/gr_metrics/blob/master/README.md.
#Input data The main function of the package is GRfit, which takes in a data frame containing information about concentration, cell counts over time, and additional grouping variables for a dose-response assay and calculates growth-rate inhibition (GR) metrics for each experiment in the dataset.
There are two cases of data input accepted by the GRfit function. They are described in detail below. Case “A” is the default option.
##Case A: a single file with control values assigned to treated measurements The control values (both control and time 0 cell counts) are pre-computed by the user and assigned to each treatment (row) in appropriate columns in the input file. Control cell counts should be in a column labeled cell_count__ctrl and the time 0 cell counts in a column labeled cell_count__time0.
An example input data frame for “Case A”, named “inputCaseA”, is contained within the package. To access it, use the following code:
library(GRmetrics)
data(inputCaseA)
The mandatory inputs for Case “A” are:
All other columns will be treated as additional keys on which the data will be grouped (e.g. cell_line, drug, time, replicate)
##Case C: a single file with control values stacked with treated measurements In the most general case, the control cell counts are in the same file and format as the treated cell counts. Control cell counts will be averaged (using a 50%-trimmed mean) and automatically matched to the treated cell counts based on the keys (columns in the data file). The control cell count values must have a value of 0 for concentration and a value for time that matches the treated measurements. The time 0 cell count values must have value of 0 for time. If the structure of the data is complex, the provided scripts may inappropriately match control and treated cell counts, so users instead should format their data as described in case A.
An example input data frame for “Case C”, named “inputCaseC”, is contained within the package. To access it, use the following code:
library(GRmetrics)
data(inputCaseC)
The mandatory inputs for Case “C” are:
All other columns will be treated as additional keys on which the data will be grouped (e.g. cell_line, drug, replicate)
##Functions The package contains 3 visualization functions: GRdrawDRC, GRscatter, and GRbox.
All of these functions take in an object created by GRfit as well as additional arguments. The results can be viewed in a static ggplot image or an interactive plotly (turned on/off by the plotly parameter).
The package also contains 4 accessor functions, which extract data from the SummarizedExperiment object created by GRfit. These functions are: GRgetMetrics, GRgetDefs, GRgetValues, and GRgetGroupVars.
Load example data (Case A)
data(inputCaseA)
head(inputCaseA)
## cell_line agent perturbation replicate time concentration cell_count
## 1 MCF10A drugA 0 1 48 0.001000 1131
## 2 MCF10A drugA 0 1 48 0.003162 1205
## 3 MCF10A drugA 0 1 48 0.010000 1021
## 4 MCF10A drugA 0 1 48 0.031620 743
## 5 MCF10A drugA 0 1 48 0.100000 459
## 6 MCF10A drugA 0 1 48 0.316200 318
## cell_count__ctrl cell_count__time0
## 1 1212.5 299.5
## 2 1212.5 299.5
## 3 1212.5 299.5
## 4 1212.5 299.5
## 5 1212.5 299.5
## 6 1212.5 299.5
Calculate GR values and solve for GR metrics parameters (i.e. fit curves)
drc_output = GRfit(inputCaseA, groupingVariables = c('cell_line','agent'))
See overview of output data (SummarizedExperiment object)
drc_output
## class: SummarizedExperiment
## dim: 19 12
## metadata(2): '' ''
## assays(1): ''
## rownames(19): ctrl_cell_doublings GR50 ... pval_rel_cell
## flat_fit_rel_cell
## rowData names(2): Metric Description
## colnames(12): BT20 drugA BT20 drugB ... MCF7 drugC MCF7 drugD
## colData names(6): cell_line agent ... experiment concentration_points
Review output table of GR metrics parameters
head(GRgetMetrics(drc_output))
## cell_line agent fit_GR fit_rel_cell experiment
## BT20 drugA BT20 drugA sigmoid sigmoid BT20 drugA
## BT20 drugB BT20 drugB flat flat BT20 drugB
## BT20 drugC BT20 drugC sigmoid sigmoid BT20 drugC
## BT20 drugD BT20 drugD sigmoid sigmoid BT20 drugD
## MCF10A drugA MCF10A drugA sigmoid sigmoid MCF10A drugA
## MCF10A drugB MCF10A drugB sigmoid sigmoid MCF10A drugB
## concentration_points ctrl_cell_doublings GR50 GRmax
## BT20 drugA 9 1.256578 0.09080477 0.03305683
## BT20 drugB 9 1.256578 Inf 0.99059876
## BT20 drugC 9 1.256578 0.24800535 -0.71018761
## BT20 drugD 9 1.256578 0.02215168 -0.05039563
## MCF10A drugA 9 2.121869 0.03964474 -0.06533159
## MCF10A drugB 9 2.121869 1.73502021 0.05502585
## GR_AOC GEC50 GRinf h_GR r2_GR
## BT20 drugA 0.50926262 0.08715113 0.02267627 1.1301507 0.968621411
## BT20 drugB 0.02209509 0.00000000 0.99059876 0.0100000 -0.004378014
## BT20 drugC 0.56226401 0.58512184 -0.78533762 1.0999555 0.977472706
## BT20 drugD 0.67647820 0.02363744 -0.04032884 1.1948823 0.976877384
## MCF10A drugA 0.62559226 0.04496553 -0.06702646 0.9988893 0.986610798
## MCF10A drugB 0.22076112 2.41460135 -0.18764462 0.9641436 0.971364003
## pval_GR flat_fit_GR IC50 Emax AUC EC50
## BT20 drugA 2.096868e-80 NA 0.55085523 0.4482145 0.7052483 0.08039928
## BT20 drugB 1.000000e+00 0.9757885 Inf 0.9864435 0.9847035 0.00000000
## BT20 drugC 4.938309e-88 NA 0.56550564 0.1029963 0.6905482 0.49386992
## BT20 drugD 1.967703e-87 NA 0.09308940 0.4062678 0.6118821 0.02197710
## MCF10A drugA 2.731585e-66 NA 0.05331866 0.2166405 0.5080238 0.03076491
## MCF10A drugB 9.815911e-55 NA 2.27507203 0.2721915 0.8128093 1.56574961
## Einf h r2_rel_cell pval_rel_cell flat_fit_rel_cell
## BT20 drugA 0.44184478 1.117968 0.88748193 5.185369e-51 NA
## BT20 drugB 0.98644353 0.010000 -0.01158457 1.000000e+00 0.9834633
## BT20 drugC 0.07154552 1.140094 0.98373427 1.575768e-95 NA
## BT20 drugD 0.41098367 1.195509 0.88438881 2.182698e-50 NA
## MCF10A drugA 0.21427553 1.017582 0.94713334 2.048170e-45 NA
## MCF10A drugB 0.15621884 1.002558 0.96108795 4.497222e-50 NA
View descriptions of each GR metric (or goodness of fit measure)
View(GRgetDefs(drc_output))
Review output table of GR values
head(GRgetValues(drc_output))
## cell_line agent perturbation replicate time concentration cell_count
## 1 MCF10A drugA 0 1 48 0.001000 1131
## 2 MCF10A drugA 0 1 48 0.003162 1205
## 3 MCF10A drugA 0 1 48 0.010000 1021
## 4 MCF10A drugA 0 1 48 0.031620 743
## 5 MCF10A drugA 0 1 48 0.100000 459
## 6 MCF10A drugA 0 1 48 0.316200 318
## cell_count__ctrl cell_count__time0 log10_concentration GRvalue
## 1 1212.5 299.5 -3.0000000 0.93219264
## 2 1212.5 299.5 -2.5000381 0.99385806
## 3 1212.5 299.5 -2.0000000 0.83663626
## 4 1212.5 299.5 -1.5000381 0.56891172
## 5 1212.5 299.5 -1.0000000 0.23569217
## 6 1212.5 299.5 -0.5000381 0.03015641
## rel_cell_count ctrl_cell_doublings experiment
## 1 0.9327835 2.017357 MCF10A drugA
## 2 0.9938144 2.017357 MCF10A drugA
## 3 0.8420619 2.017357 MCF10A drugA
## 4 0.6127835 2.017357 MCF10A drugA
## 5 0.3785567 2.017357 MCF10A drugA
## 6 0.2622680 2.017357 MCF10A drugA
View grouping variables used for calculation
GRgetGroupVars(drc_output)
## [1] "cell_line" "agent"
You can also export your results. Here are two examples:
# Write GR metrics parameter table to tab-separated text file
write.table(GRgetMetrics(drc_output), file = "filename.tsv", quote = FALSE,
sep = "\t", row.names = FALSE)
# Write original data plus GR values to comma-separated file
write.table(GRgetValues(drc_output), file = "filename.csv", quote = FALSE,
sep = ",", row.names = FALSE)
#Visualizations You can draw GR dose-response curves with plotly or with ggplot2. You can also specify the range of the graph.
# Draw dose-response curves
GRdrawDRC(drc_output)
## Warning: `gather_()` was deprecated in tidyr 1.2.0.
## Please use `gather()` instead.
## This warning is displayed once every 8 hours.
## Call `lifecycle::last_lifecycle_warnings()` to see where this warning was generated.
GRdrawDRC(drc_output, experiments = c('BT20 drugA', 'MCF10A drugA',
'MCF7 drugA'))
GRdrawDRC(drc_output, experiments = c('BT20 drugA', 'MCF10A drugA',
'MCF7 drugA'),
min = 10^(-4), max = 10^2)
GRdrawDRC(drc_output, plotly = FALSE)
You can also draw scatterplots and boxplots of GR metrics with plotly or ggplot2. Here is an example using example data in the format of Case C.
## Case C (scatterplot and boxplot examples)
data(inputCaseC)
head(inputCaseC)
## cell_line agent perturbation replicate time concentration cell_count
## 1 MCF10A - 0 NaN 0 0 294
## 2 MCF10A - 0 NaN 0 0 318
## 3 MCF10A - 0 NaN 0 0 287
## 4 MCF10A - 0 NaN 0 0 296
## 5 MCF10A - 0 NaN 0 0 291
## 6 MCF10A - 0 NaN 0 0 286
output1 = GRfit(inputData = inputCaseC, groupingVariables =
c('cell_line','agent', 'perturbation', 'replicate', 'time'), case = "C")
# Draw scatterplots
GRscatter(output1, 'GR50', 'agent', c('drugA','drugD'), 'drugB')
## Coordinate system already present. Adding new coordinate system, which will replace the existing one.
GRscatter(output1, 'GR50', 'agent', c('drugA','drugD'), 'drugB',
plotly = FALSE)
## Coordinate system already present. Adding new coordinate system, which will replace the existing one.
# Draw boxplots
GRbox(output1, metric ='GRinf', groupVariable = 'cell_line',
pointColor = 'agent')
GRbox(output1, metric ='GRinf', groupVariable = 'cell_line',
pointColor = 'agent',
factors = c('BT20', 'MCF10A'))
GRbox(output1, metric ='GRinf', groupVariable = 'cell_line',
pointColor = 'agent',
factors = c('BT20', 'MCF10A'), plotly = FALSE)
GRbox(output1, metric ='GR50', groupVariable = 'cell_line',
pointColor = 'agent', wilA = 'BT20', wilB = c('MCF7', 'MCF10A'),
plotly = FALSE)
#GR metric details We have developed scripts to calculate normalized growth rate inhibition (GR) values and corresponding metrics (GR50, GRmax, …) based on cell counts measured in dose-response experiments. Users provide a tab-separated data file in which each row represents a separate treatment condition and the columns specify the keys that define the treatment condition (e.g. cell line, drug or other perturbagen, perturbagen concentration, treatment time, replicate) and the measured cell counts (or surrogate). The experimentally measured cell counts that are required for GR metric calculation are as follows: - measured cell counts after perturbagen treatment (cell_count, x(c)) - measured cell counts of control (e.g. untreated or DMSO-treated) wells on the same plate (cell_count__ctrl, x_ctrl) - measured cell counts from an untreated sample grown in parallel until the time of treatment (cell_count__time0, x_0)
The provided GR scripts compute over the user’s data to calculate GR values individually for each treatment condition (cell line, time, drug, concentration, …) using the formula:
GR(c) = 2 ^ ( log2(x(c)/x_0) / log2(x_ctrl/x_0) ) - 1
Based on a set of GR values across a range of concentrations, the data are fitted with a sigmoidal curve:
GR(c) = GRinf + (1-GRinf)/(1 + (c/(GEC50))^Hill )
The following GR metrics are calculated:
GR50, the concentration at which the effect reaches a GR value of 0.5 based on interpolation of the fitted curve.
GRmax, the effect at the highest tested concentration. Note that GRmax can differ from GRinf if the dose-response does not reach its plateau value. For robustness, we take this as the minimum mean GR value at the two highest concentrations.
GR_AOC, the area over the dose-response curve, which is the integral of 1-GR(c) over the range of concentrations tested, normalized by the range of concentration.
GEC50, the drug concentration at half-maximal effect, which reflects the potency of the drug.
GRinf, GR(c->inf), which reflects asymptotic drug efficacy.
h_GR, The Hill coefficient of the fitted (GR) curve, which reflects how steep the dose response curve is
r2_GR, The coefficient of determination - essentially how well the (GR) curve fits to the data points
pval_GR, The p-value of the F-test comparing the fit of the (GR) curve to a horizontal line fit
flat_fit_GR, For data that doesn’t significantly fit better to a curve than a horizontal line fit (p > 0.05), the y value (GR) of the flat line
The following traditional metrics are calculated:
IC50, The concentration at which relative cell count = 0.5
Emax, The maximal effect of the drug (minimal relative cell count value). For robustness, we take this as the minimum mean relative cell count at the two highest concentrations.
AUC, The ‘Area Under the Curve’ - The area below the fitted (traditional) dose response curve
EC50, The concentration at half-maximal effect (not growth rate normalized)
Einf, The asymptotic effect of the drug (not growth rate normalized)
h, The Hill coefficient of the fitted (traditional) dose response curve, which - reflects how steep the dose response curve is
r2_rel_cell, The coefficient of determination - essentially how well the (traditional) curve fits to the data points
pval_rel_cell, The p-value of the F-test comparing the fit of the (traditional) curve to a horizontal line fit
flat_fit_rel_cell, For data that doesn’t significantly fit better to a curve than a horizontal line fit (p > 0.05), the y value (relative cell count) of the flat line
In addition to the metrics, the scripts report the r-squared of the fit and evaluate the significance of the sigmoidal fit based on an F-test. If the fit is not significant (p > 0.05), the sigmoidal fit is replaced by a constant value (flat fit). This can be circumvented by using the “force” option in the GRfit function. Additional information and considerations are described in the supplemental material of the manuscript referred above.