1 The ropls package

The ropls R package implements the PCA, PLS(-DA) and OPLS(-DA) approaches with the original, NIPALS-based, versions of the algorithms (Wold, Sjostrom, and Eriksson 2001; Trygg and Wold 2002). It includes the R2 and Q2 quality metrics (Eriksson et al. 2001; Tenenhaus 1998), the permutation diagnostics (Szymanska et al. 2012), the computation of the VIP values (Wold, Sjostrom, and Eriksson 2001), the score and orthogonal distances to detect outliers (Hubert, Rousseeuw, and Vanden Branden 2005), as well as many graphics (scores, loadings, predictions, diagnostics, outliers, etc).

2 Context

2.1 Orthogonal Partial Least-Squares

Partial Least-Squares (PLS), which is a latent variable regression method based on covariance between the predictors and the response, has been shown to efficiently handle datasets with multi-collinear predictors, as in the case of spectrometry measurements (Wold, Sjostrom, and Eriksson 2001). More recently, Trygg and Wold (2002) introduced the Orthogonal Partial Least-Squares (OPLS) algorithm to model separately the variations of the predictors correlated and orthogonal to the response.

OPLS has a similar predictive capacity compared to PLS and improves the interpretation of the predictive components and of the systematic variation (Pinto, Trygg, and Gottfries 2012). In particular, OPLS modeling of single responses only requires one predictive component.

Diagnostics such as the Q2Y metrics and permutation testing are of high importance to avoid overfitting and assess the statistical significance of the model. The Variable Importance in Projection (VIP), which reflects both the loading weights for each component and the variability of the response explained by this component (Pinto, Trygg, and Gottfries 2012; Mehmood et al. 2012), can be used for feature selection (Trygg and Wold 2002; Pinto, Trygg, and Gottfries 2012).

2.2 OPLS software

OPLS is available in the SIMCA-P commercial software (Umetrics, Umea, Sweden; Eriksson et al. (2001)). In addition, the kernel-based version of OPLS (Bylesjo et al. 2008) is available in the open-source R statistical environment (R Development Core Team 2008), and a single implementation of the linear algorithm in R has been described (Gaude et al. 2013).

3 The sacurine metabolomics dataset

The sacurine metabolomics dataset will be used as a case study to describe the features from the ropls pacakge.

3.1 Study objective

The objective was to study the influence of age, body mass index (bmi), and gender on metabolite concentrations in urine, by analysing 183 samples from a cohort of adults with liquid chromatography coupled to high-resolution mass spectrometry (LC-HRMS; Thevenot et al. (2015)).

3.2 Pre-processing and annotation

Urine samples were analyzed by using an LTQ Orbitrap in the negative ionization mode. A total of 109 metabolites were identified or annotated at the MSI level 1 or 2. After retention time alignment with XCMS, peaks were integrated with Quan Browser. Signal drift and batch effect were corrected, and each urine profile was normalized to the osmolality of the sample. Finally, the data were log10 transformed (Thevenot et al. 2015).

3.3 Covariates

The volunteers’ age, body mass index (bmi), and gender were recorded.

4 Hands-on

4.1 Loading

We first load the ropls package:

library(ropls)

We then load the sacurine dataset which contains:

  1. The dataMatrix matrix of numeric type containing the intensity profiles (log10 transformed),

  2. The sampleMetadata data frame containg sample metadata,

  3. The variableMetadata data frame containg variable metadata

data(sacurine)
names(sacurine)
## [1] "dataMatrix"       "sampleMetadata"   "variableMetadata" "se"              
## [5] "eset"

We attach sacurine to the search path and display a summary of the content of the dataMatrix, sampleMetadata and variableMetadata with the view method from the ropls package:

attach(sacurine)
view(dataMatrix)
##        dim  class    mode typeof   size NAs  min mean median max
##  183 x 109 matrix numeric double 0.2 Mb   0 -0.3  4.2    4.3   6
##        (2-methoxyethoxy)propanoic acid isomer (gamma)Glu-Leu/Ile ...
## HU_011                            3.019766011        3.888479324 ...
## HU_014                             3.81433889        4.277148905 ...
## ...                                       ...                ... ...
## HU_208                            3.748127215        4.523763202 ...
## HU_209                            4.208859398        4.675880567 ...
##        Valerylglycine isomer 2  Xanthosine
## HU_011             3.889078716 4.075879575
## HU_014             4.181765852 4.195761901
## ...                        ...         ...
## HU_208             4.634338821 4.487781609
## HU_209              4.47194762 4.222953354

view(sampleMetadata)
##      age     bmi gender
##  numeric numeric factor
##  nRow nCol size NAs
##   183    3 0 Mb   0
##         age   bmi gender
## HU_011   29 19.75      M
## HU_014   59 22.64      F
## ...     ...   ...    ...
## HU_208   27 18.61      F
## HU_209 17.5 21.48      F
## 1 data.frame 'factor' column(s) converted to 'numeric' for plotting.

view(variableMetadata)
##  msiLevel      hmdb chemicalClass
##   numeric character     character
##  nRow nCol size NAs
##   109    3 0 Mb   0
##                                        msiLevel      hmdb chemicalClass
## (2-methoxyethoxy)propanoic acid isomer        2                  Organi
## (gamma)Glu-Leu/Ile                            2                  AA-pep
## ...                                         ...       ...           ...
## Valerylglycine isomer 2                       2           AA-pep:AcyGly
## Xanthosine                                    1 HMDB00299        Nucleo
## 2 data.frame 'character' column(s) converted to 'numeric' for plotting.

Note:

  1. the view method applied to a numeric matrix also generates a graphical display

  2. the view method can also be applied to an ExpressionSet object (see below)

4.2 Principal Component Analysis (PCA)

We perform a PCA on the dataMatrix matrix (samples as rows, variables as columns), with the opls method:

sacurine.pca <- opls(dataMatrix)

A summary of the model (8 components were selected) is printed:

## PCA
## 183 samples x 109 variables
## standard scaling of predictors
##       R2X(cum) pre ort
## Total    0.501   8   0

In addition the default summary figure is displayed:

Figure 1: PCA summary plot. Top left overview: the scree plot (i.e., inertia barplot) suggests that 3 components may be sufficient to capture most of the inertia; Top right outlier: this graphics shows the distances within and orthogonal to the projection plane (Hubert, Rousseeuw, and Vanden Branden 2005): the name of the samples with a high value for at least one of the distances are indicated; Bottom left x-score: the variance along each axis equals the variance captured by each component: it therefore depends on the total variance of the dataMatrix X and of the percentage of this variance captured by the component (indicated in the labels); it decreases when going from one component to a component with higher indice; Bottom right x-loading: the 3 variables with most extreme values (positive and negative) for each loading are black colored and labeled.

Note:

  1. Since dataMatrix does not contain missing value, the singular value decomposition was used by default; NIPALS can be selected with the algoC argument specifying the algorithm (Character),

  2. The predI = NA default number of predictive components (Integer) for PCA means that components (up to 10) will be computed until the cumulative variance exceeds 50%. If the 50% have not been reached at the 10th component, a warning message will be issued (you can still compute the following components by specifying the predI value).

Let us see if we notice any partition according to gender, by labeling/coloring the samples according to gender (parAsColFcVn) and drawing the Mahalanobis ellipses for the male and female subgroups (parEllipseL).

genderFc <- sampleMetadata[, "gender"]
plot(sacurine.pca,
     typeVc = "x-score",
     parAsColFcVn = genderFc)

Figure 2: PCA score plot colored according to gender.

Note:

  1. The plotting parameter to be used As Colors (Factor of character type or Vector of numeric type) has a length equal to the number of rows of the dataMatrix (ie of samples) and that this qualitative or quantitative variable is converted into colors (by using an internal palette or color scale, respectively). We could have visualized the age of the individuals by specifying parAsColFcVn = sampleMetadata[, "age"].

  2. The displayed components can be specified with parCompVi (plotting parameter specifying the Components: Vector of 2 integers)

  3. The labels and the color palette can be personalized with the parLabVc and parPaletteVc parameters, respectively:

plot(sacurine.pca,
     typeVc = "x-score",
     parAsColFcVn = genderFc,
     parLabVc = as.character(sampleMetadata[, "age"]),
     parPaletteVc = c("green4", "magenta"))

4.3 Partial least-squares: PLS and PLS-DA

For PLS (and OPLS), the Y response(s) must be provided to the opls method. Y can be either a numeric vector (respectively matrix) for single (respectively multiple) (O)PLS regression, or a character factor for (O)PLS-DA classification as in the following example with the gender qualitative response:

sacurine.plsda <- opls(dataMatrix, genderFc)
## PLS-DA
## 183 samples x 109 variables and 1 response
## standard scaling of predictors and response(s)
##       R2X(cum) R2Y(cum) Q2(cum) RMSEE pre ort pR2Y  pQ2
## Total    0.275     0.73   0.584 0.262   3   0 0.05 0.05

Figure 3: PLS-DA model of the gender response. Top left: inertia barplot: the graphic here suggests that 3 orthogonal components may be sufficient to capture most of the inertia; Top right: significance diagnostic: the R2Y and Q2Y of the model are compared with the corresponding values obtained after random permutation of the y response; Bottom left: outlier diagnostics; Bottom right: x-score plot: the number of components and the cumulative R2X, R2Y and Q2Y are indicated below the plot.

Note:

  1. When set to NA (as in the default), the number of components predI is determined automatically as follows (Eriksson et al. 2001): A new component h is added to the model if:
  • \(R2Y_h \geq 0.01\), i.e., the percentage of Y dispersion (i.e., sum of squares) explained by component h is more than 1 percent, and

  • \(Q2Y_h=1-PRESS_h/RSS_{h-1} \geq 0\) for PLS (or 5% when the number of samples is less than 100) or 1% for OPLS: \(Q2Y_h \geq 0\) means that the predicted residual sum of squares (\(PRESS_h\)) of the model including the new component h estimated by 7-fold cross-validation is less than the residual sum of squares (\(RSS_{h-1}\)) of the model with the previous components only (with \(RSS_0\) being the sum of squared Y values).

  1. The predictive performance of the full model is assessed by the cumulative Q2Y metric: \(Q2Y=1-\prod\limits_{h=1}^r (1-Q2Y_h)\). We have \(Q2Y \in [0,1]\), and the higher the Q2Y, the better the performance. Models trained on datasets with a larger number of features compared with the number of samples can be prone to overfitting: in that case, high Q2Y values are obtained by chance only. To estimate the significance of Q2Y (and R2Y) for single response models, permutation testing (Szymanska et al. 2012) can be used: models are built after random permutation of the Y values, and \(Q2Y_{perm}\) are computed. The p-value is equal to the proportion of \(Q2Y_{perm}\) above \(Q2Y\) (the default number of permutations is 20 as a compromise between quality control and computation speed; it can be increased with the permI parameter, e.g. to 1,000, to assess if the model is significant at the 0.05 level),

  2. The NIPALS algorithm is used for PLS (and OPLS); dataMatrix matrices with (a moderate amount of) missing values can thus be analysed.

We see that our model with 3 predictive (pre) components has significant and quite high R2Y and Q2Y values.

4.4 Orthogonal partial least squares: OPLS and OPLS-DA

To perform OPLS(-DA), we set orthoI (number of components which are orthogonal; Integer) to either a specific number of orthogonal components, or to NA. Let us build an OPLS-DA model of the gender response.

sacurine.oplsda <- opls(dataMatrix, genderFc,
                        predI = 1, orthoI = NA)
## OPLS-DA
## 183 samples x 109 variables and 1 response
## standard scaling of predictors and response(s)
##       R2X(cum) R2Y(cum) Q2(cum) RMSEE pre ort pR2Y  pQ2
## Total    0.275     0.73   0.602 0.262   1   2 0.05 0.05

Figure 4: OPLS-DA model of the gender response.

Note:

  1. For OPLS modeling of a single response, the number of predictive component is 1,

  2. In the (x-score plot), the predictive component is displayed as abscissa and the (selected; default = 1) orthogonal component as ordinate.

Let us assess the predictive performance of our model. We first train the model on a subset of the samples (here we use the odd subset value which splits the data set into two halves with similar proportions of samples for each class; alternatively, we could have used a specific subset of indices for training):

sacurine.oplsda <- opls(dataMatrix, genderFc,
                        predI = 1, orthoI = NA,
                        subset = "odd")
## OPLS-DA
## 92 samples x 109 variables and 1 response
## standard scaling of predictors and response(s)
##       R2X(cum) R2Y(cum) Q2(cum) RMSEE RMSEP pre ort
## Total     0.26    0.825   0.608 0.213 0.341   1   2

We first check the predictions on the training subset:

trainVi <- getSubsetVi(sacurine.oplsda)
confusion_train.tb <- table(genderFc[trainVi], fitted(sacurine.oplsda))
confusion_train.tb
##    
##      M  F
##   M 50  0
##   F  0 42

We then compute the performances on the test subset:

confusion_test.tb <- table(genderFc[-trainVi],
                           predict(sacurine.oplsda, dataMatrix[-trainVi, ]))
confusion_test.tb
##    
##      M  F
##   M 43  7
##   F  7 34

As expected, the predictions on the test subset are (slightly) lower. The classifier however still achieves 85% of correct predictions.

4.5 Comments

4.5.1 Overfitting

Overfitting (i.e., building a model with good performances on the training set but poor performances on a new test set) is a major caveat of machine learning techniques applied to data sets with more variables than samples. A simple simulation of a random X data set and a y response shows that perfect PLS-DA classification can be achieved as soon as the number of variables exceeds the number of samples, as detailed in the example below, adapted from Wehrens (2011):

Figure 5: Risk of PLS overfitting. In the simulation above, a random matrix X of 20 observations x 200 features was generated by sampling from the uniform distribution \(U(0, 1)\). A random y response was obtained by sampling (without replacement) from a vector of 10 zeros and 10 ones. Top left, top right, and bottom left: the X-score plots of the PLS modeling of y by the (sub)matrix of X restricted to the first 2, 20, or 200 features, are displayed (i.e., the observation/feature ratios are 0.1, 1, and 10, respectively). Despite the good separation obtained on the bottom left score plot, we see that the Q2Y estimation of predictive performance is low (negative); Bottom right: a significant proportion of the models trained after random permutations of the labels have a higher Q2Y value than the model trained with the true labels, confirming that PLS cannot specifically model the y response with the X predictors, as expected.

This simple simulation illustrates that PLS overfit can occur, in particular when the number of features exceeds the number of observations. It is therefore essential to check that the \(Q2Y\) value of the model is significant by random permutation of the labels.

4.5.2 VIP from OPLS models

The classical VIP metric is not useful for OPLS modeling of a single response since (Galindo-Prieto, Eriksson, and Trygg 2014; Thevenot et al. 2015): 1. VIP values remain identical whatever the number of orthogonal components selected, 2. VIP values are univariate (i.e., they do not provide information about interactions between variables). In fact, when features are standardized, we can demonstrate a mathematical relationship between VIP and p-values from a Pearson correlation test (Thevenot et al. 2015), as illustrated by the figure below:

ageVn <- sampleMetadata[, "age"]

pvaVn <- apply(dataMatrix, 2,
               function(feaVn) cor.test(ageVn, feaVn)[["p.value"]])

vipVn <- getVipVn(opls(dataMatrix, ageVn,
                       predI = 1, orthoI = NA,
                       fig.pdfC = "none"))
## OPLS
## 183 samples x 109 variables and 1 response
## standard scaling of predictors and response(s)
##       R2X(cum) R2Y(cum) Q2(cum) RMSEE pre ort pR2Y  pQ2
## Total    0.212    0.476    0.31  7.53   1   1 0.05 0.05
quantVn <- qnorm(1 - pvaVn / 2)
rmsQuantN <- sqrt(mean(quantVn^2))

opar <- par(font = 2, font.axis = 2, font.lab = 2,
            las = 1,
            mar = c(5.1, 4.6, 4.1, 2.1),
            lwd = 2, pch = 16)

plot(pvaVn, vipVn,
     col = "red",
     pch = 16,
     xlab = "p-value", ylab = "VIP", xaxs = "i", yaxs = "i")

box(lwd = 2)

curve(qnorm(1 - x / 2) / rmsQuantN, 0, 1, add = TRUE, col = "red", lwd = 3)

abline(h = 1, col = "blue")
abline(v = 0.05, col = "blue")

par(opar)

Figure 6: Relationship between VIP from one-predictive PLS or OPLS models with standardized variables, and p-values from Pearson correlation test. The \((p_j, VIP_j)\) pairs corresponding respectively to the VIP values from OPLS modelling of the age response with the sacurine dataset, and the p-values from the Pearson correlation test are shown as red dots. The \(y = \Phi^{-1}(1 - x/2) / z_{rms}\) curve is shown in red (where \(\Phi^{-1}\) is the inverse of the probability density function of the standard normal distribution, and \(z_{rms}\) is the quadratic mean of the \(z_j\) quantiles from the standard normal distribution; \(z_{rms} = 2.6\) for the sacurine dataset and the age response). The vertical (resp. horizontal) blue line corresponds to univariate (resp. multivariate) thresholds of \(p=0.05\) and \(VIP=1\), respectively (Thevenot et al. 2015).

The VIP properties above result from:

  1. OPLS models of a single response have a single predictive component,

  2. in the case of one-predictive component (O)PLS models, the general formula for VIPs can be simplified to \(VIP_j = \sqrt{m} \times |w_j|\) for each feature \(j\), were \(m\) is the total number of features and w is the vector of loading weights,

  3. in OPLS, w remains identical whatever the number of extracted orthogonal components,

  4. for a single-response model, w is proportional to X’y (where denotes the matrix transposition),

  5. if X and y are standardized, X’y is the vector of the correlations between the features and the response.

Galindo-Prieto, Eriksson, and Trygg (2014) have recently suggested new VIP metrics for OPLS, VIP_pred and VIP_ortho, to separately measure the influence of the features in the modeling of the dispersion correlated to, and orthogonal to the response, respectively (Galindo-Prieto, Eriksson, and Trygg 2014).

For OPLS(-DA) models, you can therefore get from the model generated with opls:

  1. the predictive VIP vector (which corresponds to the \(VIP_{4,pred}\) metric measuring the variable importance in prediction) with getVipVn(model),

  2. the orthogonal VIP vector which is the \(VIP_{4,ortho}\) metric measuring the variable importance in orthogonal modeling with getVipVn(model, orthoL = TRUE). As for the classical VIP, we still have the mean of \(VIP_{pred}^2\) (and of \(VIP_{ortho}^2\)) which, each, equals 1.

4.5.3 (Orthogonal) Partial Least Squares Discriminant Analysis: (O)PLS-DA

4.5.3.1 Two classes

When the y response is a factor of 2 levels (character vectors are also allowed), it is internally transformed into a vector of values \(\in \{0,1\}\) encoding the classes. The vector is centered and unit-variance scaled, and the (O)PLS analysis is performed.

Brereton and Lloyd (2014) have demonstrated that when the sizes of the 2 classes are unbalanced, a bias is introduced in the computation of the decision rule, which penalizes the class with the highest size (Brereton and Lloyd 2014). In this case, an external procedure using resampling (to balance the classes) and taking into account the class sizes should be used for optimal results.

4.5.3.2 Multiclass

In the case of more than 2 levels, the y response is internally transformed into a matrix (each class is encoded by one column of values \(\in \{0,1\}\)). The matrix is centered and unit-variance scaled, and the PLS analysis is performed.

In this so-called PLS2 implementation, the proportions of 0 and 1 in the columns is usually unbalanced (even in the case of balanced size of the classes) and the bias described previously occurs (Brereton and Lloyd 2014). The multiclass PLS-DA results from ropls are therefore indicative only, and we recommend to set an external procedure where each column of the matrix is modeled separately (as described above) and the resulting probabilities are aggregated (see for instance Bylesjo et al. (2006)).

4.6 Working on SummarizedExperiment objects

The SummarizedExperiment class from the SummarizedExperiment bioconductor package has been developed to conveniently handle preprocessed omics objects, including the variable x sample matrix of intensities, and two DataFrames containing the sample and variable metadata, which can be accessed by the assay, colData and rowData methods respectively (remember that the data matrix is stored with samples in columns).

The opls method can be applied to a SummarizedExperiment object, by using the object as the x argument, and, for (O)PLS(-DA), by indicating as the y argument the name of the sample metadata to be used as the response (i.e. the name of the column in the colData). It returns the updated SummarizedExperiment object with the loading, score, VIP, etc. data as new columns in the colData and rowData, and with the PCA/(O)PLS(-DA) models in the metadata slot.

Getting the sacurine dataset as a SummarizedExperiment (see the Appendix to see how such an SummarizedExperiment was built):

data(sacurine)
sac.se <- sacurine[["se"]]

We then build the PLS-DA model of the gender response

sac.se <- opls(sac.se, "gender")

Note that the opls method returns an updated SummarizedExperiment with the metadata about scores, loadings, VIPs, etc. stored in the colData and rowData DataFrames:

library(SummarizedExperiment)
SummarizedExperiment::colData(sac.se)
## DataFrame with 183 rows and 6 columns
##              age       bmi   gender gender_PLSDA_xscor-p1 gender_PLSDA_xscor-p2
##        <numeric> <numeric> <factor>             <numeric>             <numeric>
## HU_011        29     19.75        M              -2.69395              3.396080
## HU_014        59     22.64        F               0.75108              2.186106
## HU_015        42     22.72        M              -4.39096              0.854612
## HU_017        41     23.03        M              -3.19297             -0.898535
## HU_018        34     20.96        M              -2.39676             -1.725307
## ...          ...       ...      ...                   ...                   ...
## HU_205      33.0     28.37        M             -3.630871             -1.950319
## HU_206      45.0     22.15        F             -0.195070             -1.137140
## HU_207      33.0     19.47        F              6.295316              0.449583
## HU_208      27.0     18.61        F              3.880127             -3.448405
## HU_209      17.5     21.48        F              0.348284             -2.028042
##        gender_PLSDA_fitted
##                <character>
## HU_011                   M
## HU_014                   F
## HU_015                   M
## HU_017                   M
## HU_018                   M
## ...                    ...
## HU_205                   M
## HU_206                   M
## HU_207                   F
## HU_208                   F
## HU_209                   F
SummarizedExperiment::rowData(sac.se)
## DataFrame with 109 rows and 7 columns
##                                         msiLevel        hmdb chemicalClass
##                                        <integer> <character>   <character>
## (2-methoxyethoxy)propanoic acid isomer         2                    Organi
## (gamma)Glu-Leu/Ile                             2                    AA-pep
## 1-Methyluric acid                              1   HMDB03099 AroHeP:Xenobi
## 1-Methylxanthine                               1   HMDB10738        AroHeP
## 1,3-Dimethyluric acid                          1   HMDB01857        AroHeP
## ...                                          ...         ...           ...
## Threonic acid/Erythronic acid                  2                    Carboh
## Tryptophan                                     1   HMDB00929        AA-pep
## Valerylglycine isomer 1                        2             AA-pep:AcyGly
## Valerylglycine isomer 2                        2             AA-pep:AcyGly
## Xanthosine                                     1   HMDB00299        Nucleo
##                                        gender_PLSDA_xload-p1
##                                                    <numeric>
## (2-methoxyethoxy)propanoic acid isomer             0.0398502
## (gamma)Glu-Leu/Ile                                -0.0455062
## 1-Methyluric acid                                  0.0892685
## 1-Methylxanthine                                   0.0925960
## 1,3-Dimethyluric acid                              0.0533869
## ...                                                      ...
## Threonic acid/Erythronic acid                      0.2027800
## Tryptophan                                         0.0310755
## Valerylglycine isomer 1                            0.1292152
## Valerylglycine isomer 2                            0.1988077
## Xanthosine                                        -0.0163006
##                                        gender_PLSDA_xload-p2 gender_PLSDA_VIP
##                                                    <numeric>        <numeric>
## (2-methoxyethoxy)propanoic acid isomer             0.0118907         0.413403
## (gamma)Glu-Leu/Ile                                -0.1898538         1.486543
## 1-Methyluric acid                                 -0.2004731         0.994359
## 1-Methylxanthine                                  -0.1662373         0.909199
## 1,3-Dimethyluric acid                             -0.1667939         0.703483
## ...                                                      ...              ...
## Threonic acid/Erythronic acid                     -0.1230309         1.271197
## Tryptophan                                        -0.0745869         0.685333
## Valerylglycine isomer 1                           -0.0585523         0.874374
## Valerylglycine isomer 2                           -0.0968777         1.282966
## Xanthosine                                        -0.1810501         1.033331
##                                        gender_PLSDA_coef
##                                                <numeric>
## (2-methoxyethoxy)propanoic acid isomer         0.0213141
## (gamma)Glu-Leu/Ile                            -0.0844622
## 1-Methyluric acid                             -0.0446014
## 1-Methylxanthine                              -0.0407458
## 1,3-Dimethyluric acid                         -0.0261733
## ...                                                  ...
## Threonic acid/Erythronic acid                -0.00295612
## Tryptophan                                   -0.04277201
## Valerylglycine isomer 1                       0.02554144
## Valerylglycine isomer 2                       0.02567323
## Xanthosine                                   -0.05027981

The opls model(s) are stored in the metadata of the sac.se SummarizedExperiment object, and can be accessed with the getOpls method:

sac_opls.ls <- getOpls(sac.se)
names(sac_opls.ls)
## [1] "gender_PLSDA"
plot(sac_opls.ls[["gender_PLSDA"]], typeVc = "x-score")

4.6.1 ExpressionSet format

The ExpressionSet format is currently supported as a legacy representation from the previous versions of the ropls package (< 1.28.0) but will now be supplanted by SummarizedExperiment in future versions. Note that the as(x, "SummarizedExperiment") method from the SummarizedExperiment package enables to convert an ExpressionSet into the SummarizedExperiment format.

exprs, pData, and fData for ExpressionSet are similar to assay, colData and rowData for SummarizedExperiment except that assay is a list which can potentially include several matrices, and that colData and rowData are of the DataFrame format. SummarizedExperiment format further enables to store additional metadata (such as models or ggplots) in a dedicated metadata slot.

In the example below, we will first build a minimal ExpressionSet object from the sacurine data set and view the data, and we subsequently perform an OPLS-DA.

Getting the sacurine dataset as an ExpressionSet (see the Appendix to see how such an ExpressionSet was built)

data("sacurine")
sac.set <- sacurine[["eset"]]
# viewing the ExpressionSet
# ropls::view(sac.set)

We then build the PLS-DA model of the gender response

# performing the PLS-DA
sac.plsda <- opls(sac.set, "gender")

Note that this time opls returns the model as an object of the opls class. The updated ExpressionSet object can be accessed with the getEset method:

sac.set <- getEset(sac.plsda)
library(Biobase)
head(Biobase::pData(sac.set))
##        age   bmi gender gender_PLSDA_xscor-p1 gender_PLSDA_xscor-p2
## HU_011  29 19.75      M            -2.6939546             3.3960801
## HU_014  59 22.64      F             0.7510799             2.1861065
## HU_015  42 22.72      M            -4.3909624             0.8546116
## HU_017  41 23.03      M            -3.1929659            -0.8985349
## HU_018  34 20.96      M            -2.3967633            -1.7253069
## HU_019  35 23.41      M            -1.5622495            -1.5750081
##        gender_PLSDA_fitted
## HU_011                   M
## HU_014                   F
## HU_015                   M
## HU_017                   M
## HU_018                   M
## HU_019                   M

4.7 Working on MultiAssayExperiment objects

The MultiAssayExperiment format is useful to handle multi-omics datasets (Ramos et al. 2017). (O)PLS(-DA) models can be built in parallel for each dataset by applying opls to such formats. We provide an example based on the NCI60_4arrays cancer dataset from the omicade4 package (which has been made available in this ropls package in the MultiAssayExperiment format).

Getting the NCI60 dataset as a MultiAssayExperiment (see the Appendix to see how such a MultiAssayExperiment can be built):

data("NCI60")
nci.mae <- NCI60[["mae"]]

Building the PLS-DA model of the cancer response for each dataset:

nci.mae <- opls(nci.mae, "cancer",
                predI = 2, fig.pdfC = "none")
## 
## 
## Building the model for the 'agilent' dataset:
## PLS-DA
## 60 samples x 300 variables and 1 response
## standard scaling of predictors and response(s)
##       R2X(cum) R2Y(cum) Q2(cum) RMSEE pre ort pR2Y  pQ2
## Total    0.262    0.231   0.182 0.275   2   0 0.05 0.05
## 
## 
## Building the model for the 'hgu133' dataset:
## PLS-DA
## 60 samples x 298 variables and 1 response
## standard scaling of predictors and response(s)
##       R2X(cum) R2Y(cum) Q2(cum) RMSEE pre ort pR2Y  pQ2
## Total    0.318    0.234   0.218 0.273   2   0 0.05 0.05
## 
## 
## Building the model for the 'hgu133p2' dataset:
## PLS-DA
## 60 samples x 268 variables and 1 response
## standard scaling of predictors and response(s)
##       R2X(cum) R2Y(cum) Q2(cum) RMSEE pre ort pR2Y  pQ2
## Total    0.312    0.234   0.214 0.273   2   0 0.05 0.05
## 
## 
## Building the model for the 'hgu95' dataset:
## PLS-DA
## 60 samples x 288 variables and 1 response
## standard scaling of predictors and response(s)
##       R2X(cum) R2Y(cum) Q2(cum) RMSEE pre ort pR2Y  pQ2
## Total    0.329    0.232   0.214 0.273   2   0 0.05 0.05

The opls method returns an updated MultiAssayExperiment with the metadata about scores, loadings, VIPs, etc. stored in the colData and rowData of the individual SummarizedExperiment:

SummarizedExperiment::colData(nci.mae[["agilent"]])
## DataFrame with 60 rows and 4 columns
##                         .id cancer_PLSDA_xscor-p1 cancer_PLSDA_xscor-p2
##                 <character>             <numeric>             <numeric>
## BR.MCF7             BR.MCF7              -4.05869               3.60974
## BR.MDA_MB_231 BR.MDA_MB_231               2.85600               3.25368
## BR.HS578T         BR.HS578T               7.16701               1.23469
## BR.BT_549         BR.BT_549               5.27739               3.56892
## BR.T47D             BR.T47D               1.21882               3.88150
## ...                     ...                   ...                   ...
## RE.CAKI_1         RE.CAKI_1               4.01588               5.10785
## RE.RXF_393       RE.RXF_393               7.30202               5.28137
## RE.SN12C           RE.SN12C               3.43798               4.65690
## RE.TK_10           RE.TK_10               1.65842               5.41697
## RE.UO_31           RE.UO_31               5.65133               4.90524
##               cancer_PLSDA_fitted
##                       <character>
## BR.MCF7                        CO
## BR.MDA_MB_231                  RE
## BR.HS578T                      RE
## BR.BT_549                      RE
## BR.T47D                        RE
## ...                           ...
## RE.CAKI_1                      RE
## RE.RXF_393                     RE
## RE.SN12C                       RE
## RE.TK_10                       RE
## RE.UO_31                       RE

The opls model(s) are stored in the metadata of the individual SummarizedExperiment objects included in the MultiAssayExperiment, and can be accessed with the getOpls method:

mae_opls.ls <- getOpls(nci.mae)
names(mae_opls.ls)
## [1] "agilent"  "hgu133"   "hgu133p2" "hgu95"
plot(mae_opls.ls[["agilent"]][["cancer_PLSDA"]], typeVc = "x-score")

4.7.1 MultiDataSet objects

The MultiDataSet format (Ramos et al. 2017) is currently supported as a legacy representation from the previous versions of the ropls package (<1.28.0) but will now be supplanted by MultiAssayExperiment in future versions. Note that the mds2mae method from the MultiDataSet package enables to convert a MultiDataSet into the MultiAssayExperiment format.

Getting the NCI60 dataset as a MultiDataSet (see the Appendix to see how such a MultiDataSet can be built):

data("NCI60")
nci.mds <- NCI60[["mds"]]

Building PLS-DA models for the cancer type:

# Restricting to the "agilent" and "hgu95" datasets
nci.mds <- nci.mds[, c("agilent", "hgu95")]
# Restricting to the 'ME' and 'LE' cancer types
library(Biobase)
sample_names.vc <- Biobase::sampleNames(nci.mds[["agilent"]])
cancer_type.vc <- Biobase::pData(nci.mds[["agilent"]])[, "cancer"]
nci.mds <- nci.mds[sample_names.vc[cancer_type.vc %in% c("ME", "LE")], ]
# Building PLS-DA models for the cancer type
nci.plsda <- ropls::opls(nci.mds, "cancer", predI = 2)

Getting back the updated MultiDataSet:

nci.mds <- ropls::getMset(nci.plsda)

4.8 Importing/exporting data

The datasets from the SummarizedExperiment and MultiAssayExperiment (as well as ExpressionSet and MultiDataSet) can be imported/exported to text files with the reading and writing functions from the phenomis package. The phenomis package is currently available on github and should be soon available on Bioconductor.

Each dataset is imported/exported to 3 text files (tsv tabular format):

  • dataMatrix.tsv: data matrix with features as rows and samples as columns

  • sampleMetadata.tsv: sample metadata

  • variableMetadata.tsv: feature metadata

install.packages("devtools")
devtools::install_github("https://github.com/odisce/phenomis")
data(sacurine)
sacurine.se <- sacurine[["se"]]
library(phenomis)
phenomis::writing(sacurine.se, dir.c = getwd())
detach(sacurine)

4.9 Graphical User Interface

The features from the ropls package can also be accessed via a graphical user interface in the Multivariate module from the Workflow4Metabolomics.org online resource for computational metabolomics, based on the Galaxy environment.

5 Appendix

5.1 Additional datasets

In addition to the sacurine dataset presented above, the package contains the following datasets to illustrate the functionalities of PCA, PLS and OPLS (see the examples in the documentation of the opls function):

  • aminoacids Amino-Acids Dataset. Quantitative structure property relationship (QSPR) (Wold, Sjostrom, and Eriksson 2001).

  • cellulose NIR-Viscosity example data set to illustrate multivariate calibration using PLS, spectral filtering and OPLS (Multivariate calibration using spectral data. Simca tutorial. Umetrics, Sweden).

  • cornell Octane of various blends of gasoline: Twelve mixture component proportions of the blend are analysed (Tenenhaus 1998).

  • foods Food consumption patterns accross European countries (FOODS). The relative consumption of 20 food items was compiled for 16 countries. The values range between 0 and 100 percent and a high value corresponds to a high consumption. The dataset contains 3 missing data (Eriksson et al. 2001).

  • linnerud Three physiological and three exercise variables are measured on twenty middle-aged men in a fitness club (Tenenhaus 1998).

  • lowarp A multi response optimization data set (LOWARP) (Eriksson et al. 2001).

  • mark Marks obtained by french students in mathematics, physics, french and english. Toy example to illustrate the potentialities of PCA (Baccini 2010).

5.2 Cheat sheets for Bioconductor (multi)omics containers

5.2.1 SummarizedExperiment

The SummarizedExperiment format has been designed by the Bioconductor team to handle (single) omics datasets (Morgan et al. 2022).

An example of SummarizedExperiment creation and a summary of useful methods are provided below.

Please refer to package vignettes for a full description of SummarizedExperiment objects .

# Preparing the data (matrix) and sample and variable metadata (data frames):
data(sacurine, package = "ropls")
data.mn <- sacurine[["dataMatrix"]] # matrix: samples x variables
samp.df <- sacurine[["sampleMetadata"]] # data frame: samples x sample metadata
feat.df <- sacurine[["variableMetadata"]] # data frame: features x feature metadata

# Creating the SummarizedExperiment (package SummarizedExperiment)
library(SummarizedExperiment)
sac.se <- SummarizedExperiment(assays = list(sacurine = t(data.mn)),
                               colData = samp.df,
                               rowData = feat.df)
# note that colData and rowData main format is DataFrame, but data frames are accepted when building the object
stopifnot(validObject(sac.se))

# Viewing the SummarizedExperiment
# ropls::view(sac.se)
Methods Description Returned class
Constructors
SummarizedExperiment Create a SummarizedExperiment object SummarizedExperiment
makeSummarizedExperimentFromExpressionSet SummarizedExperiment
Accessors
assayNames Get or set the names of assay() elements character
assay Get or set the ith (default first) assay element matrix
assays Get the list of experimental data numeric matrices SimpleList
rowData Get or set the row data (features) DataFrame
colData Get or set the column data (samples) DataFrame
metadata Get or set the experiment data list
dim Get the dimensions (features of interest x samples) integer
dimnames Get or set the dimension names list of length 2 character/NULL
rownames Get the feature names character
colnames Get the sample names character
Conversion
as(, "SummarizedExperiment") Convert an ExpressionSet to a SummarizedExperiment SummarizedExperiment

5.2.2 MultiAssayExperiment

The MultiAssayExperiment format has been designed by the Bioconductor team to handle multiomics datasets (Ramos et al. 2017).

An example of MultiAssayExperiment creation and a summary of useful methods are provided below. Please refer to package vignettes or to the original publication for a full description of MultiAssayExperiment objects (Ramos et al. 2017).

Loading the NCI60_4arrays from the omicade4 package:

data("NCI60_4arrays", package = "omicade4")

Creating the MultiAssayExperiment:

library(MultiAssayExperiment)
# Building the individual SummarizedExperiment instances
experiment.ls <- list()
sampleMap.ls <- list()
for (set.c in names(NCI60_4arrays)) {
  # Getting the data and metadata
  assay.mn <- as.matrix(NCI60_4arrays[[set.c]])
  coldata.df <- data.frame(row.names = colnames(assay.mn),
                           .id = colnames(assay.mn),
                           stringsAsFactors = FALSE) # the 'cancer' information will be stored in the main colData of the mae, not the individual SummarizedExperiments
  rowdata.df <- data.frame(row.names = rownames(assay.mn),
                           name = rownames(assay.mn),
                           stringsAsFactors = FALSE)
  # Building the SummarizedExperiment
  assay.ls <- list(se = assay.mn)
  names(assay.ls) <- set.c
  se <- SummarizedExperiment(assays = assay.ls,
                             colData = coldata.df,
                             rowData = rowdata.df)
  experiment.ls[[set.c]] <- se
  sampleMap.ls[[set.c]] <- data.frame(primary = colnames(se),
                                      colname = colnames(se)) # both datasets use identical sample names
}
sampleMap <- listToMap(sampleMap.ls)

# The sample metadata are stored in the colData data frame (both datasets have the same samples)
stopifnot(identical(colnames(NCI60_4arrays[[1]]),
                    colnames(NCI60_4arrays[[2]])))
sample_names.vc <- colnames(NCI60_4arrays[[1]])
colData.df <- data.frame(row.names = sample_names.vc,
                         cancer = substr(sample_names.vc, 1, 2))

nci.mae <- MultiAssayExperiment(experiments = experiment.ls,
                                colData = colData.df,
                                sampleMap = sampleMap)

stopifnot(validObject(nci.mae))
Methods Description Returned class
Constructors
MultiAssayExperiment Create a MultiAssayExperiment object MultiAssayExperiment
ExperimentList Create an ExperimentList from a List or list ExperimentList
Accessors
colData Get or set data that describe the patients/biological units DataFrame
experiments Get or set the list of experimental data objects as original classes experimentList
assays Get the list of experimental data numeric matrices SimpleList
assay Get the first experimental data numeric matrix matrix, matrix-like
sampleMap Get or set the map relating observations to subjects DataFrame
metadata Get or set additional data descriptions list
rownames Get row names for all experiments CharacterList
colnames Get column names for all experiments CharacterList
Subsetting
mae[i, j, k] Get rows, columns, and/or experiments MultiAssayExperiment
mae[i, ,] i: GRanges, character, integer, logical, List, list MultiAssayExperiment
mae[,j,] j: character, integer, logical, List, list MultiAssayExperiment
mae[,,k] k: character, integer, logical MultiAssayExperiment
mae[[i]] Get or set object of arbitrary class from experiments (Varies)
mae[[i]] Character, integer, logical
mae$column Get or set colData column vector (varies)
Management
complete.cases Identify subjects with complete data in all experiments vector (logical)
duplicated Identify subjects with replicate observations per experiment list of LogicalLists
mergeReplicates Merge replicate observations within each experiment MultiAssayExperiment
intersectRows Return features that are present for all experiments MultiAssayExperiment
intersectColumns Return subjects with data available for all experiments MultiAssayExperiment
prepMultiAssay Troubleshoot common problems when constructing main class list
Reshaping
longFormat Return a long and tidy DataFrame with optional colData columns DataFrame
wideFormat Create a wide DataFrame, one row per subject DataFrame
Combining
c Concatenate an experiment MultiAssayExperiment
Viewing
upsetSamples Generalized Venn Diagram analog for sample membership upset
Exporting
exportClass Exporting to flat files csv or tsv files

5.2.3 ExpressionSet

The ExpressionSet format (Biobase package) was designed by the Bioconductor team as the first format to handle (single) omics data. It has now been supplanted by the SummarizedExperiment format.

An example of ExpressionSet creation and a summary of useful methods are provided below. Please refer to ‘An introduction to Biobase and ExpressionSets’ from the documentation from the Biobase package for a full description of ExpressionSet objects.

# Preparing the data (matrix) and sample and variable metadata (data frames):
data(sacurine)
data.mn <- sacurine[["dataMatrix"]] # matrix: samples x variables
samp.df <- sacurine[["sampleMetadata"]] # data frame: samples x sample metadata
feat.df <- sacurine[["variableMetadata"]] # data frame: features x feature metadata
# Creating the ExpressionSet (package Biobase)
sac.set <- Biobase::ExpressionSet(assayData = t(data.mn))
Biobase::pData(sac.set) <- samp.df
Biobase::fData(sac.set) <- feat.df
stopifnot(validObject(sac.set))
# Viewing the ExpressionSet
# ropls::view(sac.set)
Methods Description Returned class
exprs ‘variable times samples’ numeric matrix matrix
pData sample metadata data.frame
fData variable metadata data.frame
sampleNames sample names character
featureNames variable names character
dims 2x1 matrix of ‘Features’ and ‘Samples’ dimensions matrix
varLabels Column names of the sample metadata data frame character
fvarLabels Column names of the variable metadata data frame character

5.2.4 MultiDataSet

Loading the NCI60_4arrays from the omicade4 package:

data("NCI60_4arrays", package = "omicade4")

Creating the MultiDataSet:

library(MultiDataSet)
# Creating the MultiDataSet instance
nci.mds <- MultiDataSet::createMultiDataSet()
# Adding the two datasets as ExpressionSet instances
for (set.c in names(NCI60_4arrays)) {
  # Getting the data
  expr.mn <- as.matrix(NCI60_4arrays[[set.c]])
  pdata.df <- data.frame(row.names = colnames(expr.mn),
                        cancer = substr(colnames(expr.mn), 1, 2),
                        stringsAsFactors = FALSE)
  fdata.df <- data.frame(row.names = rownames(expr.mn),
                        name = rownames(expr.mn),
                        stringsAsFactors = FALSE)
  # Building the ExpressionSet
  eset <- Biobase::ExpressionSet(assayData = expr.mn,
                                 phenoData = new("AnnotatedDataFrame",
                                                 data = pdata.df),
                                 featureData = new("AnnotatedDataFrame",
                                                   data = fdata.df),
                                 experimentData = new("MIAME",
                                                      title = set.c))
  # Adding to the MultiDataSet
  nci.mds <- MultiDataSet::add_eset(nci.mds, eset, dataset.type = set.c,
                                     GRanges = NA, warnings = FALSE)
}
stopifnot(validObject(nci.mds))
Methods Description Returned class
Constructors
createMultiDataSet Create a MultiDataSet object MultiDataSet
add_eset Create a MultiAssayExperiment object MultiDataSet
Subsetting
mset[i, ] i: character,logical (samples to select) MultiDataSet
mset[, k] k: character (names of datasets to select) MultiDataSet
mset[[k]] k: character (name of the datast to select) ExpressionSet
Accessors
as.list Get the list of data matrices list
pData Get the list of sample metadata list
fData Get the list of variable metadata list
sampleNames Get the list of sample names list
Management
commonSamples Select samples that are present in all datasets MultiDataSet
Conversion
mds2mae Convert a MultiDataSet to a MultiAssayExperiment MultiAssayExperiment

6 Session info

Here is the output of sessionInfo() on the system on which this document was compiled:

## R version 4.4.0 beta (2024-04-15 r86425)
## Platform: x86_64-pc-linux-gnu
## Running under: Ubuntu 22.04.4 LTS
## 
## Matrix products: default
## BLAS:   /home/biocbuild/bbs-3.19-bioc/R/lib/libRblas.so 
## LAPACK: /usr/lib/x86_64-linux-gnu/lapack/liblapack.so.3.10.0
## 
## locale:
##  [1] LC_CTYPE=en_US.UTF-8       LC_NUMERIC=C              
##  [3] LC_TIME=en_US.UTF-8        LC_COLLATE=en_US.UTF-8    
##  [5] LC_MONETARY=en_US.UTF-8    LC_MESSAGES=en_US.UTF-8   
##  [7] LC_PAPER=en_US.UTF-8       LC_NAME=C                 
##  [9] LC_ADDRESS=C               LC_TELEPHONE=C            
## [11] LC_MEASUREMENT=en_US.UTF-8 LC_IDENTIFICATION=C       
## 
## time zone: America/New_York
## tzcode source: system (glibc)
## 
## attached base packages:
## [1] stats4    stats     graphics  grDevices utils     datasets  methods  
## [8] base     
## 
## other attached packages:
##  [1] MultiDataSet_1.32.0         MultiAssayExperiment_1.30.0
##  [3] SummarizedExperiment_1.34.0 Biobase_2.64.0             
##  [5] GenomicRanges_1.56.0        GenomeInfoDb_1.40.0        
##  [7] IRanges_2.38.0              S4Vectors_0.42.0           
##  [9] BiocGenerics_0.50.0         MatrixGenerics_1.16.0      
## [11] matrixStats_1.3.0           ropls_1.36.0               
## [13] BiocStyle_2.32.0           
## 
## loaded via a namespace (and not attached):
##  [1] sass_0.4.9              SparseArray_1.4.0       lattice_0.22-6         
##  [4] magrittr_2.0.3          digest_0.6.35           evaluate_0.23          
##  [7] grid_4.4.0              calibrate_1.7.7         bookdown_0.39          
## [10] fastmap_1.1.1           jsonlite_1.8.8          Matrix_1.7-0           
## [13] limma_3.60.0            tinytex_0.50            BiocManager_1.30.22    
## [16] httr_1.4.7              UCSC.utils_1.0.0        jquerylib_0.1.4        
## [19] abind_1.4-5             cli_3.6.2               rlang_1.1.3            
## [22] crayon_1.5.2            XVector_0.44.0          cachem_1.0.8           
## [25] DelayedArray_0.30.0     yaml_2.3.8              BiocBaseUtils_1.6.0    
## [28] S4Arrays_1.4.0          tools_4.4.0             GenomeInfoDbData_1.2.12
## [31] R6_2.5.1                lifecycle_1.0.4         magick_2.8.3           
## [34] zlibbioc_1.50.0         MASS_7.3-60.2           bslib_0.7.0            
## [37] qqman_0.1.9             Rcpp_1.0.12             statmod_1.5.0          
## [40] xfun_0.43               highr_0.10              knitr_1.46             
## [43] htmltools_0.5.8.1       rmarkdown_2.26          compiler_4.4.0

References

Baccini, A. 2010. “Statistique Descriptive Multidimensionnelle (Pour Les Nuls).”

Brereton, Richard G., and Gavin R. Lloyd. 2014. “Partial Least Squares Discriminant Analysis: Taking the Magic Away.” Journal of Chemometrics 28 (4): 213–25. http://dx.doi.org/10.1002/cem.2609.

Bylesjo, M, M Rantalainen, O Cloarec, J Nicholson, E Holmes, and J Trygg. 2006. “OPLS Discriminant Analysis: Combining the Strengths of PLS-DA and SIMCA Classification.” Journal of Chemometrics 20: 341–51. http://dx.doi.org/10.1002/cem.1006.

Bylesjo, M., M. Rantalainen, J. Nicholson, E. Holmes, and J. Trygg. 2008. “K-OPLS Package: Kernel-Based Orthogonal Projections to Latent Structures for Prediction and Interpretation in Feature Space.” BMC Bioinformatics 9 (1): 106. http://dx.doi.org/10.1186/1471-2105-9-106.

Eriksson, L., E. Johansson, N. Kettaneh-Wold, and S. Wold. 2001. Multi- and Megavariate Data Analysis. Principles and Applications. Umetrics Academy.

Galindo-Prieto, B., L. Eriksson, and J. Trygg. 2014. “Variable Influence on Projection (VIP) for Orthogonal Projections to Latent Structures (OPLS).” Journal of Chemometrics 28 (8): 623–32. http://dx.doi.org/10.1002/cem.2627.

Gaude, R., F. Chignola, D. Spiliotopoulos, A. Spitaleri, M. Ghitti, JM. Garcia-Manteiga, S. Mari, and G. Musco. 2013. “Muma, an R Package for Metabolomics Univariate and Multivariate Statistical Analysis.” Current Metabolomics 1: 180–89. http://dx.doi.org/10.2174/2213235X11301020005.

Hubert, M., PJ. Rousseeuw, and K. Vanden Branden. 2005. “ROBPCA: A New Approach to Robust Principal Component Analysis.” Technometrics 47: 64–79. http://dx.doi.org/10.1198/004017004000000563.

Mehmood, T., KH. Liland, L. Snipen, and S. Saebo. 2012. “A Review of Variable Selection Methods in Partial Least Squares Regression.” Chemometrics and Intelligent Laboratory Systems 118 (0): 62–69. http://dx.doi.org/10.1016/j.chemolab.2012.07.010.

Morgan, Martin, Valerie Obenchain, Jim Hester, and Hervé Pagès. 2022. SummarizedExperiment: SummarizedExperiment Container. https://bioconductor.org/packages/SummarizedExperiment.

Pinto, RC., J. Trygg, and J. Gottfries. 2012. “Advantages of Orthogonal Inspection in Chemometrics.” Journal of Chemometrics 26 (6): 231–35. http://dx.doi.org/10.1002/cem.2441.

Ramos, Marcel, Lucas Schiffer, Angela Re, Rimsha Azhar, Azfar Basunia, Carmen Rodriguez, Tiffany Chan, et al. 2017. “Software for the Integration of Multiomics Experiments in Bioconductor.” Cancer Research 77 (21): e39–e42. https://doi.org/10.1158/0008-5472.CAN-17-0344.

R Development Core Team. 2008. R: A Language and Environment for Statistical Computing. Vienna, Austria: R Foundation for Statistical Computing. http://www.R-project.org.

Szymanska, E., E. Saccenti, AK. Smilde, and JA. Westerhuis. 2012. “Double-Check: Validation of Diagnostic Statistics for PLS-DA Models in Metabolomics Studies.” Metabolomics 8 (1, 1): 3–16. http://dx.doi.org/10.1007/s11306-011-0330-3.

Tenenhaus, M. 1998. La Regression PLS : Theorie et Pratique. Editions Technip.

Thevenot, EA., A. Roux, X. Ying, E. Ezan, and C. Junot. 2015. “Analysis of the Human Adult Urinary Metabolome Variations with Age, Body Mass Index and Gender by Implementing a Comprehensive Workflow for Univariate and OPLS Statistical Analyses.” Journal of Proteome Research 14 (8): 3322–35. http://dx.doi.org/10.1021/acs.jproteome.5b00354.

Trygg, J., and S. Wold. 2002. “Orthogonal Projection to Latent Structures (O-PLS).” Journal of Chemometrics 16: 119–28. http://dx.doi.org/10.1002/cem.695.

Wehrens, R. 2011. Chemometrics with R: Multivariate Data Analysis in the Natural Sciences and Life Sciences. Springer.

Wold, S., M. Sjostrom, and L. Eriksson. 2001. “PLS-Regression: A Basic Tool of Chemometrics.” Chemometrics and Intelligent Laboratory Systems 58: 109–30. http://dx.doi.org/10.1016/S0169-7439(01)00155-1.