Abstract
Background
Chemotherapy-induced peripheral neuropathy (CIPN) is a serious therapy-limiting side effect of commonly used anticancer drugs. Previous studies suggest that lipids may play a role in CIPN. Therefore, the present study aimed to identify the particular types of lipids that are regulated as a consequence of paclitaxel administration and may be associated with the occurrence of post-therapeutic neuropathy.
Methods
High resolution mass spectrometry lipidomics was applied to quantify d = 255 different lipid mediators in the blood of n = 31 patients drawn before and after paclitaxel therapy for breast cancer treatment. A variety of supervised statistical and machine-learning methods was applied to identify lipids that were regulated during paclitaxel therapy or differed among patients with and without post-therapeutic neuropathy.
Results
Twenty-seven lipids were identified that carried relevant information to train machine learning algorithms to identify, in new cases, whether a blood sample was drawn before or after paclitaxel therapy with a median balanced accuracy of up to 90%. One of the top hits, sphinganine-1-phosphate (SA1P), was found to induce calcium transients in sensory neurons via the transient receptor potential vanilloid 1 (TRPV1) channel and sphingosine-1-phosphate receptors.SA1P also showed different blood concentrations between patients with and without neuropathy.
Conclusions
Present findings suggest an important role for sphinganine-1-phosphate in paclitaxel-induced biological changes associated with neuropathic side effects. The identified SA1P, through its receptors, provides a potential drug target for co-therapy with paclitaxel to reduce one of its major and therapy-limiting side effects.
Introduction
Paclitaxel is a standard adjuvant treatment for breast cancer and several other cancers. Originally isolated from the yew tree Taxus brevifolia, it inhibits mitosis by stabilizing microtubules and preventing tubulin depolymerization (5–7). A serious dose- and therapy-limiting side effect, which it shares with other commonly used cytostatic drugs, is the chemotherapy-induced peripheral neuropathy and neuropathic pain (CIPN), which affects up to 80% of treated patients (1, 2). Currently, there are no pharmacologic treatments for CIPN expert for duloxetine (1, 3, 4). Therefore, research on the mechanism of paclitaxel indued CIPN with possible identification of novel treatments is an active research topic.
Several genes and neurofilament proteins have been implicated in paclitaxel-induced neuropathy . More recently, lipid mediators have been shown to be produced at high levels in sensory neurons, neuronal tissue and immune cells after chemotherapy due to oxidative stress and have been shown to contribute to chemotherapy-induced neuropathy and neuropathic pain by modulating neuronal ion channels (11–14). Therefore, they are of particular interest as signaling molecules and potential markers for chemotherapy-induced neuropathy in patients. In fact, lipids are already considered markers for other neurological diseases such as Alzheimer’s disease and amyotrophic lateral sclerosis (ALS) (15–17). However, a systematic approach to investigate lipids in patients with paclitaxel-induced neuropathy has not been performed.
In this prospective clinical cohort study, plasma concentrations of 255 different lipid mediators were evaluated for changes in their concentrations associated with paclitaxel treatment. A comprehensive LC-MS/MS-based targeted and LC-QTOFMS-based untargeted lipidomics screening was performed on plasma samples from paclitaxel-treated patients. Lipid groups measured included eicosanoids, endocannabinoids, oxidized linoleic acid metabolites, sphingolipids, lysophospholipids and free fatty acids, many of which have been previously associated with persistent pain states (18–20). A data-driven approach was used to identify lipid mediators whose concentrations could be used to train machine learning algorithms to identify, in new cases, whether a plasma sample was collected before or after therapy, or from a patient with or without post-therapy neuropathy. The biological relevance of the findings was then validated in vitro by applying SA1P to primary sensory neurons using calcium imaging.
Materials and Methods
Patients and study design
This was a prospective single-arm study enrolling patients with breast cancer. The study was conducted in accordance with the Declaration of Helsinki on Biomedical Research Involving Human Subjects and was approved by the Ethics Committee of the Medical Faculty of the Goethe-University, Frankfurt am Main, Germany. Informed written consent was obtained from each of the participants.
Sixty patients (one male, 59 female with breast cancer and undergoing paclitaxel treatment were recruited from the Tumor Center of the University Hospital Frankfurt, Germany (UCT). Most patients (n = 47) received the “paclitaxel-weekly” schedule, consisting of 12 cycles of paclitaxel treatment (80 mg/m², each week); a few patients (n = 13) received mixed carboplatin/paclitaxel treatment (Table S1). A blood sample was collected from each patient before and after chemotherapy, and the degree of neuropathy after chemotherapy was assessed as described below. Plasma was isolated from the blood samples immediately after blood collection to ensure lipid stability. Plasma was stored at −80°C until analysis.
All patients provided a blood sample before chemotherapy; however, only 36 patients of the patients provided a second blood sample after chemotherapy. For our analysis, we focused on patients that had two blood samples. Therefore, 72 samples from 36 patients (before and after chemotherapy) were analyzed using both LC-MS/MS-based targeted and LC-QTOFMS-based untargeted lipidomics. A total of 255 individual lipids were detected in each sample. From the resulting data, five patients had to be excluded due to incomplete lipidomics data (more than 20% of the analytes could not be detected). The remaining 62 samples from 31 patients were used for the machine learning analysis (Figure 1).
Assessment of neuropathy
The occurrence and severity of peripheral neuropathy was assessed according to the guidelines of the NCI Common Terminology Criteria for Adverse Events (CTCAE) v5.0, Published: November 27, 2017, by the U.S. Department of Health and Human Services (https://ctep.cancer.gov/protocoldevelopment/electronic_applications/docs/ctcae_v5_quick_reference_5×7.pdf). Neuropathy assessment was performed prospectively, i.e., before the first paclitaxel treatment and again after the 12th treatment cycle. Neuropathy was assessed regularly upon visit of the patient. The last assessment was performed 4.5 years after initial chemotherapy (Table S1).
The severity of neuropathy was graded into five grades: Grade 1 Mild; asymptomatic or mild symptoms; clinical or diagnostic observations only; intervention not indicated. Grade 2 Moderate; minimal, local or noninvasive intervention indicated; limiting age-appropriate instrumental ADL (activities of daily living). Grade 3 Severe or medically significant but not immediately life-threatening hospitalization or prolongation of hospitalization indicated; disabling; limiting self-care ADL. Grade 4 Life-threatening consequences; urgent intervention indicated. Grade 5 Death related to AE. In the present cohort, grades 1-3 were detected following paclitaxel chemotherapy (Table S1). Of the 31 patients with a full set of samples, 17 had neuropathy after chemotherapy (54.9%), 12 had grade 1, 3 had grade 2 and two patients with grade 3 (Table S1).
Lipidomics analysis using LC-MS/MS and LC-QTOFMS
Blood was collected from patients in EDTA tubes and immediately centrifuged at 2000 xg for 10 minutes at 4°C.The supernatant was immediately frozen at −80°C until further processing. Approximately 2-3 ml of plasma was considered sufficient for each patient. Liquid chromatography-tandem mass spectrometry (LC-MS/MS) analysis of eicosanoids, oxidized linoleic acid metabolites (O(x)LAMs), prostanoids, endocannabinoids, LPAs, pterins, sphingolipids and ceramides, and lipidomics screening were performed as described previously (13, 19, 21). A total of 255 lipids were quantified in each plasma sample. These lipids belong to the groups of eicosanoids, oxidized linoleic acid metabolites, endocannabinoids, lysophosphatidic acids, pterins, sphingolipids, ceramides, cholesterols, cholesterol esters, diacylglycerols, triacylglycerols, phospholipids, lysophospholipids, and free fatty acids. Full details of the lipids detected are given in Table S2. Full details of the LC-MS methods used can be found in the Supporting Information Methods section (Tables 1-10).
Data analysis
The data analysis combined statistical and machine learning methods (“mixture of experts” approach) shown to be superior to relying on a single method (23)(24), such as regression analysis alone (22). The data analysis included unsupervised and supervised methods (Figure 1). Unsupervised methods were used to establish whether the lipidomics data contained structures that supported prior classification into (i) baseline and post-treatment samples, or (ii) subjects with or without neuropathy in the post-treatment samples. Supervised methods were then used to identify lipid mediators that carried information relevant to the class structure of the data set. Programming was performed in R language (25) using the R software package (26), version 4.1.2, for Linux, available free of charge from the Comprehensive R Archive Network (CRAN) at https://CRAN.R-project.org/, and in Python language (27) using Python version 3.8.12, available free of charge at https://www.python.org (accessed March 1, 2022). The data analysis is summarized in Figure 1 and described in detail in the supporting information.
Following log-transformation and missing-value imputation, the lipid marker concentrations were analyzed using unsupervised methods to assess whether they contained structures that were consistent with the prior class structure. Z-standardized data were projected from the high-dimensional space onto lower dimensional planes by means of principal component analysis (PCA) (28, 29) as one of the classical methods established. As an alternative approach, unsupervised machine learning was implemented as self-organizing maps (SOM) of artificial neurons (30). In their special form of emergent SOM (ESOM (31)), the present map consisted of 4,000 neurons arranged on a two-dimensional toroidal grid with 50 rows and 80 columns (32, 33).
Supervised methods included binary logistic regression (36) and, since a mixture of experts was preferred (22–24), additional machine-learning algorithms of different types known to work well for tabular numerical data were applied. These included random forests (37, 38) as a robust tree-based bagging classifier, support vector machines (SVM) (39) as a hyperplane separation-based method. Classifier tuning is described in the supporting information. The analyses were performed using cross-validation and training, testing, and validation splits of the dataset as a machine learning standard. That is, a class-proportional random sample of 20% of the dataset was set aside before the analyses started and served as a validation sample that was not touched during algorithm training and feature selection. In the remaining 80% of the dataset, feature selection was performed using supervised analyses in 100-fold nested cross-validation scenarios. Feature selection, i.e., identification of the individual lipid mediators that contained relevant information to assign a sample to either the pre- or post-therapy day or to a patient with or without neuropathy, was identified by majority vote among 17 different feature selection methods, including univariate and multivariate types listed in the supporting information. After quantifying the importance of each feature, the most relevant subset of lipid mediators was identified by subjecting the importance measures to computed ABC analysis (cABC analysis) (40), an item categorization technique adopted from economics that aims to divide a set of positive numerical data into three disjoint subsets labeled “A,” “B,” and “C”. The set “A” should contain the “few important” elements (41), which was retained. The resulting final sets of lipid mediators were then used to train the algorithms to perform the task of assigning a sample to either the pre- or post-therapy day or to a patient with or without neuropathy in the hold-out 20% validation sample mentioned above.
Calcium Imaging with primary sensory neurons
Primary sensory neurons were cultured as described previously (42). For calcium imaging experiments, neurons were stained with Fura-2-AM (Thermo Fisher) for at least 60 min at 37°C and washed afterwards twice with Ringeŕs solution consisting of 145 mM NaCl, 1.25 mM CaCl2 × 2H2O, 1 mM MgCl2 x 6 H2O, 5 mM KCl, 10 mM D-glucose, and 10 mM HEPES adjusted to a pH of 7.3. To investigate the effect of SA1P or LPC 24:0 on different TRP channels, sensory neurons were incubated with the lipids for 1 min at a concentration of 1 or 10 µM, respectively. The gold standard agonists for TRPV1 and TRPA1 were capsaicin (200 nM, 20s) and AITC (allyl isothiocyanate, 75 µM, 30s). Fingolimod was used at a concentration of 1 µM and pre-incubated for 1 h prior to measurement. As a positive control, final stimulation with KCl (50 mM, 1 min) was used to depolarize all neurons. All stimulating compounds were dissolved in Ringer’s solution to their final concentrations.
The calcium imaging data were analyzed using descriptive statistics. All calcium imaging data are presented as the mean ± SEM. Normal distribution was confirmed using the Shapiro-Wilk test. For experiments comparing only two groups, unpaired and heteroscedastic Student’s t-tests were conducted following Welch’s correction. When comparing more than two groups, one-way analysis of variance (ANOVA) was used, and for the comparison of more than three groups, two-way ANOVA was conducted. For all statistical analyses of the calcium imaging data, the software GraphPad Prism 9.5 was used. Statistical significance was set at p value < 0.05.
Results
All patients received paclitaxel as adjuvant or neoadjuvant therapy, without any other potentially neurotoxic substances. Of the 60 patients from our analysis cohort, two were excluded due to rescheduling of paclitaxel therapy. Blood samples were obtained from 31 patients before and after chemotherapy. Twenty lipid marker variables had > 20% missing values. Following exclusion of these patients and variables and imputation, a data matrix for further analyses was obtained, sized 79 × 255 (79 data set instances, samples, and 255 different lipid mediators Figure 1). An overview of the distribution of the lipid marker data is shown in Figure S1. These included 48 samples drawn on day 1 before therapy and 31 samples drawn on day 2 after 12 cycles of paclitaxel therapy. On day 2, n = 17 of the 31 patients had symptoms of neuropathy (54.9%), which is in line with previous clinical reports on occurrence and severity of paclitaxel-induced neuropathy (43, 44). Most patients reported grade 1 neuropathy, although two patients experienced grade 3 neuropathy. Occurrence and degree of neuropathy were monitored 4.5 years after finishing chemotherapy. The neuropathy lasted for several months or, in many cases, still persisted for 4.5 years after chemotherapy at the last examination (Table S1).
Results of unsupervised analysis of structure in the lipidomics data supporting prior knowledge
An overview of the distribution of the lipid marker data is shown in Figure S1. PCA yielded d = 28 components with eigenvalues > 1, which together explained 93.93% of the total variance in the lipid mediators (Figure 2). The d = 86 lipid mediators that contributed most to the relevant PCs were identified based on the membership to category “A” in the cABC analysis of the weighted variable contributions to each PC (Figure S2). This was carried over as one of the several feature importance measures to the supervised analyses reported in the next chapter. On the emergent self-organizing map (ESOM, Figure 2a), a clear separation of two clusters was observed, which provided support that the lipid mediators contained a data structure contingent with the prior classification into pre- and posttherapy samples (Fisher’s exact test: p = 0.01054, odds ratio: 3.572973 with 95% confidence interval 1.28 - 10.52; Figure 2b). The separation of samples on the ESOM also corresponded, but to a lesser extent, with the occurrence of neuropathy observed at the time of the 2nd blood sample (p = 0.03279, odds ratio 0.16, 95% confidence interval 0.0137 - 1.022).
The results of the unsupervised analysis thus supported that the lipidomics data contained a structure contingent on a known prior classification. This supported the continuation of data analysis with supervised methods to determine which of the lipids carried relevant information to assign a probe to a particular prior class.
Results of supervised analyses identifying lipid mediators relevant to the class structure
Lipid mediators informative for assigning samples to before or after paclitaxel therapy
Based on the majority vote of the different approaches to feature selection including PCA importance and further univariate and multivariate feature selection methods specified in the supplementary information, d = 77 lipid mediators were found to provide relevant information on whether a sample was collected before or after paclitaxel therapy (Figure S3). When statistical (logistic regression) and machine learning (random forests, support vector machines - SVM) algorithms were trained with this set of lipid mediators, the assignment of a sample to day 1 or 2 was well above the guessing level (Table 2). By contrast, when the training data were randomly permuted, the performance fell to a balanced accuracy of 0.5, i.e., guessing level, which established that the obtained class assignment in the non-permuted scenario had not been due to overfitting. In addition, by rerunning the cABC analysis on the mediators assigned to subset “A” in the first run (“recursive” cABC analysis (45)), the informative set of lipid mediators could be further reduced to d = 27 (Table 1). With these mediators, SVM and random forest were still able to detect whether an instance of a lipidomics dataset was from before or after paclitaxel treatment at a balanced accuracy better than expected from guessing.
Lipid mediators informative for assigning post-paclitaxel therapy samples to neuropathy
The n = 31 samples from day 2 were probably too small to detect whether a sample was from a patient with neuropathy. Although the median balanced accuracies for the three algorithms to detect neuropathy in new cases unseen during training were up to 0.75, while only the guess level of 0.5 was achieved when using permuted data for training, the 95% CI of the performance measures was not separated from guess level. Therefore, features were selected using univariate methods (Cohen’s d, FPR, FWE). The small set of lipid mediators emerging from all three methods as informative for neuropathy again included SA1P (see above), and in addition sphingomyelin 33:1, and sphingomyelin 43:1. The three mediators differed significantly between samples from neuropathy-positive and neuropathy-negative patients (Figure 3).
Biological in-vitro validation of the machine learning based results
The results of the supervised analysis thus established a limited set of lipid mediators to be regulated in association with paclitaxel therapy or with its side effect of inducing neuropathy. The top hit was sphinganine-1-phosphate (SA1P), also known as dihydrosphingosine-1-phosphate (DH-S1P), providing a basis for in vitro validation of its biological effects in the present context of neuropathy.
Calcium imaging measurements were performed on primary sensory neurons obtained from the murine dorsal root ganglia. We stimulated the neurons with 1 and 10 µM SA1P (ranked as the primary hit) or LPC 24:0 (ranked as one of the least relevant lipids by machine learning analysis). We observed that SA1P caused a direct calcium transient in approximately 11.7% of KCl-responsive sensory neurons (Figure 4a, b). However, LPC 24:0 did not induce any notable activation of sensory neurons at concentration of 1 and 10 µM (Figure S4a-c). To further characterize the SA1P-responding neurons, we investigated their responsiveness to agonists of the TRP channels TRPV1 (capsaicin) and TRPA1 (AITC, allyl isothiocyanate), both of which are hallmarks of subpopulations of primary sensory neurons (46). Stimulating SA1P-responsive neurons with capsaicin and AITC revealed that 73% of these neurons also responded to capsaicin and 25% of them responded to AITC, whereas only 9.6% responded to both stimuli. Neurons were identified as responders to KCl (50 mM, 1 min; Figure 4c, d).
To identify the receptors or channels responsible for SA1P-mediated calcium transients in sensory neurons, the selective TRPV1 antagonist AMG9810 was used. Neurons were stimulated twice with SA1P (1 µM, 1 min) and AMG9810 (1 µM or vehicle) was added two minutes prior to the second SA1P stimulus. The second SA1P response was entirely abolished when the neurons were treated with AMG9810, but not with the vehicle (Figure 5a-c). The potency of AMG9810 was validated using the same measurement protocol as before but with capsaicin (200 nM, 20s) instead of SA1P, which is the gold standard agonist of TRPV1. AMG9810 completely blocked the second capsaicin response (Figure 5d). The involvement of S1P-receptors previously suggested to be the receptors for SA1P (47), was evident by studying S1PR1 and S1PR3 as the most highly expressed S1P receptors in sensory neurons (48), which are also targets of the approved drug fingolimod. Sensory neurons were incubated with fingolimod or vehicle for one hour and stimulated the neurons with SA1P (Fig. 5e, f). Comparing fingolimod- and vehicle-treated neurons, we observed that the response intensity to SA1P was similar (Figure 5g), while the number of neurons responding to SA1P was significantly decreased after fingolimod treatment (Figure 5h).
Discussion
SA1P induced a direct calcium transient in sensory neurons dependent on sphingosine 1-phosphate receptors (S1PR) and the transient receptor potential vanilloid 1 (TRPV1) channel. The results suggest that lipids are altered during paclitaxel treatment and that alterations in sphingolipid metabolism may be critical for the development of paclitaxel-induced peripheral neuropathy in patients. The final (“sparse”) set of lipids regulated between sampling days (before and after paclitaxel treatment) was enriched for sphingolipids. Specifically, sphingolipids were significantly overrepresented among the top hits of lipids regulated between sampling days (Fisher’s exact test: p = 0.01), i.e., while 46 of the original 255 lipid mediators were sphingolipids (18%) (Table S2), 11 of the 27 members of the final sparse marker set (40.7%) belonged to the group of sphingolipids. The main pathway in which the top hits are involved is shown in Figure 6. With the top hits (“sparse” feature set), three different algorithms (logistic regression, random forests, support vector machines) could be trained to identify, in new cases, whether a blood sample was drawn before or after paclitaxel therapy with a median balanced accuracy of up to 90%. Furthermore, the classification of patients with regard to neuropathy after paclitaxel treatment was reflected in lipidomics in another sphingolipid, i.e., dihydrosphingosine sphinganine-1-phosphate (SA1P), which was elevated in patients with neuropathy.
The results from an unbiased machine-learning-based analysis are in line with those of previous reports that had used classical statistics mainly. For example, S1P was elevated in the spinal cord of mice after bortezomib treatment and during bortezomib-induced neuropathic pain. Blocking S1P1 receptor S1P1R with fingolimod effectively reduced bortezomib-induced mechanical hypersensitivity in vivo (14). Interestingly, targeting the S1P-S1P1R-axis was also found to reduce paclitaxel-induced neuropathic pain in vivo in a preclinical study (49). Further agreements of the present results relate to previous preclinical reports highlighting the significance of the sphingolipid pathway in persistent and neuropathic pain states (14, 50, 51). In addition, the S1P signaling axis was observed to be relevant in neuropathy and chemotherapy-induced neuropathic pain, which led to the suggestion of targeting S1P receptors as a novel approach to ameliorate chemotherapy-induced neuropathy and neuropathic pain (49, 52-55). Taken together, present results from lipid screening and unbiased machine-learning approach point towards a significant contribution of sphingolipid signaling in paclitaxel-induced neuropathy in patients, mainly via sphinganine-1-pshophate and sphingomyelins 33:1 and 43:1.
Sphinganine is a key branching point in the sphingolipid pathway, where it can either be acylated to form dihydroceramides or phosphorylated to SA1P by sphingosine kinases (56). Accumulation of sphinganine has been previously associated with reduced activity of ceramide synthase CerS2 (57). Interestingly, low CerS2 expression is a hallmark of various tumors (58). It is conceivable that a subgroup of the patient cohort still exhibits low CerS2 expression after paclitaxel treatment, which is associated with higher SA1P levels and a higher occurrence of neuropathy. We also identified SA1P as a potential proalgesic lipid mediator, as it causes direct calcium transients in approximately 10% of sensory neurons. This effect is mediated, at least in part, by S1P receptors S1P1 and S1P3 and the TRPV1 channel. The TRPV1 channel has previously been identified as an important mediator of neuropathic pain and is associated with exacerbated activity of sensory neurons during paclitaxel-induced neuropathic pain (59–61). Our data suggest that an S1P receptor modulator, such as fingolimod may be a potential treatment strategy for reducing the proalgesic effect of SA1P and possibly for reducing paclitaxel-induced neuropathy in patients.
Several other lipids were found in the extended list of hits previously associated with chemotherapy-induced neuropathy or acute pain in preclinical studies, such as LPC 18:1, sphingosin-1-phosphate (S1P), and 9,10-EpOME. LPC 18:1 has previously been identified as an endogenous activator of TRPV1 and TRM8 and was found at elevated levels in murine DRGs 24 h after oxaliplatin treatment. This may contribute to oxaliplatin-induced acute pain (62). Similarly, 9,10-EpOME was elevated in the DRGs of paclitaxel-treated mice. locking its synthesis with the CYP2J2-inhibitor and the approved drug telmisartan was shown to reduce acute paclitaxel-induced mechanical hypersensitivity in vivo and prevent paclitaxel-induced mechanical allodynia by pretreatment (13). In addition, the direct TRPV1 agonist LPA 18:1 was found in the extended list of hits. Lipid was shown to bind to the C-terminal binding site of TRPV1 to increase the opening probability of the channel (63). Other signaling lipids with potential proalgesic effects and potential TRP channel activators that have been described previously have also been identified as crucial for group separation by our unbiased machine-learning approach, which strengthens the presumption that the identified lipids may indeed be connected with paclitaxel neurotoxicity and paclitaxel-induced neuropathy in patients. Additionally, we found several precursor fatty acids in the extended list of hits, including arachidonic acid, linoleic acid, and palmitic acid. These results imply a major dysregulation of lipids after paclitaxel treatment, leading to enhanced plasma levels of precursors for eicosanoids and oxidized linoleic acid metabolites, which may explain the observed enhanced concentrations of the eicosanoids of 5-HETE, 5,6-DHET, and the oxidized linoleic acid metabolites 9,10-EpOME, 9- and 13-HODE.
Several limitations need to be addressed. First, the cohort size (n=60 patients, n=31 patients who provided blood samples before and after paclitaxel chemotherapy our patient cohort allowed for errors due to interindividual differences. Second, the paclitaxel treatment regimen differed in some patients included in this study. While the majority of the patients received paclitaxel as “pacli weekly” regime consisting of a weekly dose of 80 mg/m² for 12 consecutive weeks in, some few patients received paclitaxel doses up to 220 mg/m² or a combination chemotherapy consisting of carboplatin/paclitaxel. These variabilities within the patient cohort hamper interindividual correlations between plasma lipid mediator concentrations and paclitaxel-induced neuropathy throughout the treatment course. Third, the assessment of peripheral neuropathy in patients was performed according to the guidelines of the NCI Common Terminology Criteria for Adverse Events (CTCAE) v5.0, which ranks the severity of neuropathy into five grades but is rather focused on general adverse events of chemotherapy rather than specifically assessing peripheral neuropathy in detail. We did not perform any neurological testing of sensory parameters, such as quantitative sensory testing (QST) (64), to determine the sensory status quo of the patients. The study lacked a separate validation cohort with similar data to the main cohort. However, an independent second cohort was available from another hospital (Oncological Center in Offenbach, Germany). This cohort consisted of 28 patients treated with the “paclitaxel weekly” regimen (paclitaxel 80 mg/m², once weekly) as adjuvant or neoadjuvant therapy for breast or ovarian cancer. All patients provided informed consent into study participation and publication of the results. Blood samples were available from routine collections and were analyzed by LC-MS/MS (Figure S5, Table S3). In contrast to the main cohort, plasma from patients in the second cohort was collected after 6 cycles of paclitaxel treatment due to local routines. Therefore, the second cohort cannot be considered a state-of-the-art validation cohort. In addition, only six patients in this cohort had neuropathy after chemotherapy (26.5%), all with grade 1 neuropathy (Table S4). Despite these limitations, algorithms trained with lipid information from cohort 1 were able to successfully identify whether a probe was taken before or after paclitaxel therapy in the second cohort at a better than guessing level. Furthermore, a trend towards different SA1P concentrations in the plasma of patients after paclitaxel treatment was observed (p = 0.086, Figure 7).
Conclusions
Here, we demonstrate that the combination of state-of-the-art lipidomics using LC-MS/MS, LC-QTOF-MS, and machine learning-based data analysis can robustly lead to the generation of testable hypotheses and the identification of biologically relevant signaling mediators of neuropathy in an unbiased manner. Lipidomic profiles were compared within the same patients, allowing analysis of individual paclitaxel-induced lipidome changes in the same patients. These analyses led to the identification of a lipid mediator that can directly activate calcium transients in sensory neurons, thereby modulating nociceptive processing and sensory neuron activity. The identified SA1P, through its receptors, provides a potential drug target for co-therapy with paclitaxel to reduce one of its major and therapy-limiting side effects.
Data availability
Data are available on request from the senior author. Relevant Python and R code is available at https://github.com/JornLotsch/PaclitaxelNeuropathyProject.
Author Contributions
MS and GG conceptualized and designed the experiments. JL and SM performed the machine learning analysis. LH, CA, YS, ST, DT, and NFB performed lipidomics measurements and analyzed the data. SW and MS performed calcium imaging experiments. KG, CB, and CS assembled the patient cohorts. JL, KG, SW and MS wrote the manuscript. All authors have reviewed and edited the manuscript.
Acknowledgements
MS was supported by the Deutsche Forschungsgemeinschaft (German Research Foundation, DFG, Grants SFB1039 A09 and Z01) and from the Fraunhofer Foundation Project: Neuropathic Pain as well as the Fraunhofer Cluster of Excellence for Immune-Mediated Diseases (CIMD). This work was also supported by the Leistungszentrum Innovative Therapeutics (TheraNova) funded by the Fraunhofer Society and the Hessian Ministry of Science and Arts. JL was supported by the Deutsche Forschungsgemeinschaft (DFG LO 612/16-1). These public funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript. We would also like to thank Drs Tabea Osthues, Béla Zimmer and Vittoria Rimola, as well as Mr. Maksim Sendetski for their help in patient sample processing.
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