This vignette describes how to use Olink® Analyze to evaluate a dataset for the presence of outliers. When performing statistical analyze it is important to establish the presence of any outlier samples in the data prior to statistical analysis. There are many reasons why a sample might be an outlier, it could be due to a data entry or measurement error (i.e. labeling a control sample as a disease sample), sampling problems or unusual conditions (i.e. contamination), or natural variation. In many parametric statistics tests the mean of each group is used to determine differences between groups. Since the mean is highly sensitive to outliers, it is important to examine datasets for outliers prior to analysis as these outliers could have a large influence on the statistical results.
In Olink Analyze, there are three visualization functions that can be
used to identify potential outlier samples. In this vignette, you will
learn how to use olink_pca_plot()
,
olink_dist_plot()
, and olink_qc_plot()
to
identify and remove outliers from a dataset.
For demonstration purposes two outlier datasets have been generated to demonstrate large outlier effects by adjusting the NPX values for specific Samples or groups.
# Create Datasets with outliers
outlier_data <- npx_data1 |>
dplyr::mutate(NPX = ifelse(SampleID == "A25", NPX + 4, NPX)) |>
dplyr::mutate(NPX = ifelse(SampleID == "A52", NPX - 4, NPX)) |>
dplyr::filter(!stringr::str_detect(SampleID, "CONTROL"))
group_data <- npx_data1 |>
dplyr::mutate(NPX = ifelse(Site == "Site_D", NPX + 3, NPX)) |>
dplyr::filter(!stringr::str_detect(SampleID, "CONTROL"))
Principal Component Analysis (PCA) is a dimensional reduction
technique. PCA plots can be particularly useful to visualize variability
within high dimensional data by plotting the data along the axes of
greatest variation. The first two principal components make up the
largest axes of variance between samples. In
olink_pca_plot()
samples are clustered together based on
similarities in overall expression patterns of the measured proteins.
These samples can be colored by any categorical variable to determine
which biological factors may be contributing to global effects across
the samples. PCA plots can be used to:
Identify individual outlier samples (Figure 1A)
Identify groups of outliers (Figure 1B)
Identify batch effects (see Bridging Vignette)
Regardless of what the PCA is being used for, PCA plots are great tools to get an overview of the data prior to analysis and pick up on any global trends. These samples are not necessarily outliers but might be indicative of a global difference between groups.
p1<- outlier_data |> olink_pca_plot(label_samples = T, quiet = T)
p2<- group_data |> olink_pca_plot(color_g = "Site", quiet = T)
ggpubr::ggarrange(p1[[1]], p2[[1]], nrow = 2, labels = "AUTO")
As shown above, PCA plots can be used to identify global differences in specific samples or sets of samples. Often times these samples can be attributed to natural variations, but sometimes these samples are outliers due to technical or sample specific issues. To determine if a sample is a true outlier and should be excluded, consider the following:
Did the sample pass QC? - Sometimes samples that are outliers and have a QC warnings may indicate sample or technical issues. For example, a buffer sample will often flag on QC and be plotted as an outlier as there are no proteins in the sample.
How far is the sample from other samples? - Samples variability within a specific group may be larger or there may be global variables within a group. In this case it is important to consider the sample within the context of the project.
Does the sample appear as an outlier by other plots? - If a sample is an outlier in the PCA, NPX distribution, and QC plots, that this might indicate a true outlier.
Is the sample an outlier on all panels? - Some samples may perform better on specific samples. In the next section we will explain how to view samples by panel.
PCA plots can be generated using olink_pca_plot()
and
specifying the color for each sample using the color_g
argument. By default the samples will be colored by QC_Warning. Prior to
generating the PCA plot, the duplicate SampleIDs (often Control samples)
will need to be renamed or filtered out.
OlinkAnalyze::npx_data1 |>
dplyr::filter(stringr::str_detect(SampleID, "CONTROL", negate = T)) |> # Filter duplicate SampleIDs
olink_pca_plot(color_g = "Treatment")
In this dataset there do not appear to be any outliers in the PCA plot.
When multiple panels are run, there is a chance a sample may be an
outlier on one panel. To get a global view of the samples per Panel, the
byPanel
argument can be specified.
OlinkAnalyze::npx_data2 |>
dplyr::filter(stringr::str_detect(SampleID, "CONTROL", negate = T)) |> # Filter out control SampleIDs
olink_pca_plot(byPanel = TRUE) # Specify by panel
The PCA plots will be saved in a list of ggplot objects and each can
be viewed individually using [[n]]
syntax as shown
below.
pca_plots<-OlinkAnalyze::npx_data2|> # Save the PCA plot to a variable
dplyr::filter(stringr::str_detect(SampleID, "CONTROL", negate = T)) |> # Filter duplicate SampleIDs
olink_pca_plot(byPanel = TRUE, quiet = TRUE) # By panel
# quiet argument suppresses export
pca_plots[[1]] #Cardiometabolic PCA
pca_plots[[2]] #Inflammation PCA
The plots above show an example where there are not any clear outliers in the PCA. For the purposes of this vignette, we have also generated data where 2 samples appear as outliers.
However from this plot, we can not identify which two samples are outliers. In the next section we will go over how to label outliers in the plot.
There are two ways to label the samples in the PCA plot. The first
way is to use the label_samples
argument. This argument
will label all samples by replacing the dot with the SampleID.
outlier_data |>
dplyr::filter(stringr::str_detect(SampleID, "CONTROL", negate = T)) |> # Filter duplicate SampleIDs
olink_pca_plot(label_samples = TRUE)
Here we can see that samples A25 and A52 appear as outliers. This
method can be useful when there is clear separation in samples. However
it can be difficult to identify additional trends when all samples are
labeled. In this case the samples must also be visually identified as
opposed to programmatically extracted from the plot. For a cleaner plot
with only the outliers labeled, we can use outlierDefX
,
outlierDefY
, outlierLines
, and
label_outliers
. These arguments will plot lines at a number
of standard deviations from the mean of the plotted PC and label the
samples outside of these lines. The values of outlierDefX
and outlierDefY
will need to be generated by the users and
may require some manual adjustment to determine the correct number to
highlight the outliers.
outlier_data |>
dplyr::filter(stringr::str_detect(SampleID, "CONTROL", negate = T)) |> # Filter duplicate SampleIDs
olink_pca_plot(outlierDefX = 3, outlierDefY = 3,
outlierLines = TRUE, label_outliers = TRUE)
To remove the lines and just keep the outliers labelled,
outlierLines
can be set to False.
outlier_data |>
dplyr::filter(stringr::str_detect(SampleID, "CONTROL", negate = T)) |> # Filter duplicate SampleIDs
olink_pca_plot(outlierDefX = 3, outlierDefY = 3,
outlierLines = FALSE, label_outliers = TRUE)
Once the correct outliers have been highlighted in the graph, we can then programmatically extract the outlier SampleIDs using dplyr.
outliers_pca_labeled <- outlier_data |>
dplyr::filter(stringr::str_detect(SampleID, "CONTROL", negate = T)) |> # Filter duplicate SampleIDs
olink_pca_plot(outlierDefX = 3, outlierDefY = 3, outlierLines = FALSE,
label_outliers = TRUE, quiet = TRUE)
outliers_pca_labeled[[1]]$data |>
dplyr::filter(Outlier == TRUE) |>
dplyr::select(SampleID) |>
dplyr::distinct()
#> SampleID
#> 1 A25
#> 2 A52
NPX distribution plots generated by olink_dist_plot
consist of box and whisker plots of NPX distribution for each sample.
These boxplots can be used to determine if a sample has an unusually
large or small distribution or if a samples NPX distribution is shifted
compared to other samples in the study. When used in combination with
PCA and QC plots, NPX distribution plots can give an additional
dimension of data to help identify outlier samples or global trends
within groups of samples.
In NPX distribution plot an outlier may show one of the following characteristics:
If we look at a subset of the outlier data from the PCA example, we can see that A25 and A52 have shifted NPX distributions, which in combination with the PCA plot, suggest that these samples may be potential outliers. If there are many samples in a project, it can be helpful to look at a subset of the samples at a time as shown below.
outlier_data |>
dplyr::filter(SampleID %in% c("A25", "A52", "A1", "A2", "A3", "A5", "A15", "A16", "A18", "A19", "A20"))|>
olink_dist_plot()
NPX distribution plots can also be useful in identifying group
trends, such as a difference in site D as shown in the figure below. The
color of the bars can be altered using the color_g
argument.
group_data |>
dplyr::filter(Site %in% c("Site_A", "Site_D")) |> # Only visualizing 2 sites to see all samples
olink_dist_plot(color_g = "Site")
In this case, the shift in NPX distribution could be biologically meaningful or could indicate a sample or technical issue. There are several biological cases where the total protein concentration in a sample may be larger in one group than another. However, in some cases the difference in protein concentration can also lead to skewed results, in which case it may be helpful to normalize the data for the changes in protein concentration by performing a median adjustment as shown below.
# Calculate SampleID Median NPX
median_NPX<-group_data |>
dplyr::group_by(SampleID) |>
dplyr::summarise(Median_NPX = median(NPX))
# Adjust by sample median
adjusted_data <- group_data |>
dplyr::inner_join(median_NPX, by = "SampleID")|>
dplyr::mutate(NPX = NPX - Median_NPX)
adjusted_data|>
dplyr::filter(Site %in% c("Site_A", "Site_D")) |> # Only visualizing 2 sites to see all samples
olink_dist_plot(color_g = "Site")
Often there are too many samples to identify outliers using
olink_dist_plot()
. In this case,
olink_qc_plot()
offers an alternative way to visualize the
NPX distribution per sample. In this plot, the sample median and sample
interquartile range (IQR) are plotted to visualize where the sample is
centered and how much variability is within the sample.
olink_qc_plot()
contains similar features to
olink_pca_plot()
and can be used in a similar way. These
samples can be colored by any categorical variable to determine which
biological factors may be contributing to global effects across the
samples or individual sample outlier. QC plots can be used to identify
individual outlier samples or identify groups of outliers. In the QC
plot an outlier may show one or more of the following
characteristics:
Using the outlier data from the previous plots, we can see that sample A52 has a lower sample median and sample A25 has a higher sample median in both panels. Sample A48 has the highest IQR of all samples in the Inflammation panel. However, we can see many other samples approaching the line threshold line (default of 3 standard deviation from the mean IQR or sample median), suggesting that this sample may not be a true outlier.
With a standard deviation of 3 and assuming a normal distribution of samples, it is expected that over 99% of the data will lie within 3 standard deviations from the mean, however depending on the groups and samples within the study, there may be global shifts which will result in one or more samples outside of the 3 SD line. These lines should be used as guidelines and not strict thresholds of outliers.
Similar to what was shown in the NPX distribution plot example, the QC plot can also be used to see changes in specific groups. In the example below, the samples are colored by site and Site D appears to have samples with higher sample median.
To change the threshold and outliers that are labeled, we can use
median_outlierDef
, IQR_outlierDef
,
outlierLines
, and label_outliers
. These
arguments will plot lines at a number of standard deviations from the
mean of the sample median or IQR and label the samples outside of these
lines. The values of median_outlierDef
and
IQR_outlierDef
default to 3 and may require some manual
adjustment to determine the correct number to highlight the
outliers.
outlier_data |>
olink_qc_plot(median_outlierDef = 2, IQR_outlierDef = 4,
outlierLines = TRUE, label_outliers = TRUE)
To remove the lines and just keep the outliers labelled
outlierLines
can be set to False.
outlier_data |>
olink_qc_plot(median_outlierDef = 2, IQR_outlierDef = 4,
outlierLines = FALSE, label_outliers = TRUE)
Once the correct outliers have been highlighted in the graph, we can then programmatically extract the outlier SampleIDs using dplyr.
outliers_qc_labeled <- outlier_data |>
olink_qc_plot(median_outlierDef = 2, IQR_outlierDef = 4,
outlierLines = FALSE, label_outliers = TRUE)
outliers_qc_labeled$data |>
dplyr::filter(Outlier == TRUE) |>
dplyr::select(SampleID) |>
dplyr::distinct()
#> # A tibble: 2 × 1
#> SampleID
#> <chr>
#> 1 A25
#> 2 A52
After reviewing these plots, a list of potential outliers may be generated. Whether or not these outliers should be excluded depends on how different from the other samples the potential outliers appear and if the outliers can be traced to a biological, sample specific, or technical issue. An outlier could also be specific to a particular panel, in which case the outlier either be excluded from just the panel on which it is an outlier or excluded from all panels.
In the case of a biological issue, it may be useful to keep the potential outlier within the study as the sample has biological meaning, however additional normalization may be needed. For example, in a diabetes study, patients with severe diabetes may have higher protein in their urine as compared to control subject. In this case it could be useful to normalize based on total protein concentration or median NPX to set all values within the context of the study. Another example is in the case of multiple batches, one batch may appear to cluster differently from another batch. In this case additional normalization such as bridging is needed to bridge the studies to the same scale.
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