Abstract
The response rate of anti-PD1 therapy is limited, and the influence of anti-PD1 therapy on cancer patients is unclear. To address these challenges, we conducted a longitudinal analysis of plasma proteomic changes with anti-PD1 therapy in non-small cell lung cancer (NSCLC), alveolar soft part sarcoma (ASPS), and lymphoma patients. We included 339 plasma samples before and after anti-PD1 therapy from 193 patients with NSCLC, ASPS, or lymphoma. The plasma proteins were detected using data-independent acquisition-mass spectrometry and customable antibody microarrays. Differential proteomic characteristics in responders (R) and non-responders (NR) before and after anti-PD1 therapy were elucidated. A total of 1019 proteins were detected using our in-depth proteomics platform and distributed across 10–12 orders of abundance. By comparing the differential plasma proteome expression between R and NR groups, 50, 206, and 268 proteins were identified in NSCLC, ASPS, and lymphoma patients, respectively. Th17, IL-17, and JAK-STAT signal pathways were identified upregulated in NR group, while cellular senescence and transcriptional misregulation pathways were activated in R group. Longitudinal proteomics analysis revealed the IL-17 signaling pathway was downregulated after treatment. Consistently, many proteins were identified as potential combinatorial therapeutic targets (e.g., IL-17A and CD22). Five noninvasive biomarkers (FLT4, SFTPB, GNPTG, F5, and IL-17A) were further validated in an independent lymphoma cohort (n = 39), and another three noninvasive biomarkers (KIT, CCL3, and TNFSF1) were validated in NSCLC cohort (n = 76). Our results provide molecular insights into the anti-PD1 therapy in cancer patients and identify new therapeutic strategies for anti-PD1-resistant patients.
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Introduction
Immune checkpoint inhibitors (ICIs) targeting programmed death 1 (PD1) or programmed death-ligand 1 (PD-L1) have revolutionized the pattern of anti-tumor treatment with improved survival in multiple cancer types [1, 2]. However, a large portion of cancer patients cannot benefit from anti-PD1 therapy [3]. Previous genomic and transcriptomic studies have identified biomarkers for the efficacy prediction of anti-PD1 therapy. To date, only three markers were approved by the United States Food and Drug Administration (FDA) [4], including microsatellite instability (MSI)/mismatch-repair deficiency (dMMR) [5], tumor mutation burden (TMB) [6] in pancancer, and PD-L1 expression in non-small cell lung cancer (NSCLC) [7]. Moreover, the clinical predictive value of these biomarkers remains within the range of 20%–80% and is largely influenced by the assay used and cancer type [8,9,10,11,12]. Therefore, it is imperative to identify new biomarkers for anti-PD1 immunotherapy [13].
Proteomics technologies that can measure all proteins in clinical samples offer an alternative approach in elucidating the heterogeneous responses of cancer patients and discovering biomarkers for anti-PD1 therapy [14]. Compared to tissues, the detection of protein biomarkers is simple, noninvasive, and can be easily adapted in the clinic [15, 16]. In our previous study, we identified five autoantibody biomarkers for anti-PD1 therapy using high-throughput protein arrays [17]. In addition to autoantibodies, there are numerous plasma proteins that can be used as biomarkers in clinical diagnostics and prognosis prediction [18]. However, the detection of low-abundance proteins is particularly challenging for mass spectrometry (MS). To address this need, we developed an in-depth serum proteomic platform using DIA-MS and customizable antibody microarrays that can detect serum proteins covering 10–12 orders of abundance magnetite [19]. Using a similar strategy, Babačić et al. investigated serial plasma samples from 24 patients with metastatic melanoma and observed an increase in circulating PD1 during anti-PD1 therapy, as well as diverse immune plasma proteomic signatures in anti-PD1 responders [20]. However, the number of patients analyzed in that study is limited and thus requires validation using a larger cohort. Moreover, only one cancer type was investigated in the study, and the influence of PD1 therapy on different cancers is unclear.
In this study, we systematically analyzed the expression of the plasma proteome (n = 339) in a cohort of 193 NSCLC, alveolar soft part sarcoma (ASPS), and lymphoma patients longitudinally using our in-depth proteomic platform by integrating DIA-MS and antibody microarrays. The differentially expressed proteins between responders (R) and non-responders (NR) were identified by statistical analysis. Bioinformatics analysis further illustrated common and specific biological processes and signaling pathways that were altered in NSCLC, ASPS, and lymphoma cancer patients. In addition, biomarkers and combinational protein targets that could be potentially used to maximize therapeutic benefits for cancer patients were identified and validated in independent clinical cohorts.
Materials and methods
Plasma sample collection
We longitudinally collected serial plasma samples before and after treatment, including the 1st, 2nd, 3rd, or more than 3rd assessment time points. A total of 339 plasma samples were collected from August 2016 to March 2022 from 93 NSCLC patients (92 patients have pre-treatment samples), 12 ASPS patients, and 88 lymphoma patients (Table S1). Among NSCLC patients, six patients were EGFR mutation positive, none had ALK rearrangements, in 29 NSCLC patients with PD-L1 expression level available, and PD-L1 scores of TPS ≥ 50%, TPS 1 to 49%, and TPS < 1% were observed in 10, 11, and 8 patients, respectively. All blood samples were collected in EDTA tubes. After centrifugation at 16,000g at 4 °C for 10 min, the plasma was collected in a new tube and stored at − 80 °C until use.
Patient baseline characteristics including age at treatment start, gender, ECOG performance, and tumor stage are shown in Table S2. Three approved anti-PD1 antibodies including Sintilimab, Toripalimab, and Nivolumab were used. Treatment efficacy was evaluated by oncologists and radiologists according to clinical and radiological examination results. The clinical response was defined as complete response (CR), partial response (PR), stable disease (SD), or progressive disease (PD) based on Response Evaluation Criteria in Solid Tumours (RECIST) version 1.1 for ASPS, NSCLC, and International Working Group 2007 Criteria for lymphoma [21, 22]. Responder (R) patients were defined as patients with CR/PR or SD lasting ≥ 6 months. The non-responder (NR) group included patients who had PD on/before 6 months [23,24,25].
All experiments were conducted with the approval of the Research Ethics Committee and according to the Declaration of Helsinki.
Screening of serum proteome using antibody microarrays
The preparation of antibody microarray and serum screening were performed as previously described [19]. Briefly, 10 μL of serum samples were diluted to 100 μL with phosphate-buffered saline (PBS pH 7.4) and then labeled by NHS-PEG4-Biotin (Thermo Fisher Scientific, MA, USA) at room temperature for 1 h. Excess biotin molecules were removed, and the biotinylated serum samples were diluted with 400 μL of PBS containing 5% milk (w/v). In parallel to biotin labeling, antibody microarrays were blocked with 500 μL of PBS with 5% milk (w/v) for 1 h at room temperature. After removing the milk, the microarrays were incubated with biotinylated serum for 2 h at room temperature, followed by washing with PBS containing 0.05% (w/v) Tween-20 (PBST). To detect bound proteins, the arrays were incubated with 2 µg/mL streptavidin–phycoerythrin (PE) (Jackson Immunoresearch, USA) for 1 h at room temperature in the dark and then washed with PBST. After centrifuging for 2 min at 1000g, the slides were scanned using a GenePix 4300A microarray scanner at a wavelength of 532 nm. BSA was used as negative control for protein detection by microarray.
Measurement of serum proteome using DIA-MS
Peptide sample preparation and data-independent acquisition analysis were performed as previously described [26]. Briefly, 2 µL serum sample was diluted with lysis buffer containing 6 M urea (Sigma, USA). Next, the serum was reduced with 10 mM dithiothreitol (DTT) at 37 °C for 60 min and then alkylated with 500 mM iodoacetamide (IAA) at room temperature for 45 min in the dark. Proteins were sequentially digested with trypsin for 16 h at 37 °C. The tryptic peptides were acidified with 1% trifluoroacetic acid and desalted with a C18 desalination column according to the manufacturer’s protocol. The desalted peptide was dried under vacuum and dissolved in 20 μL of buffer containing 0.1% formic acid and 2% acetonitrile. Peptide concentrations were measured by Nanoscan (Analytik Jena AG, Jena, Germany). Approximately 1.5 µg of peptides were separated on a 30-min LC gradient using an analytical column (150 µm × 250 mm, 2 µm 200 Å C18 particles) and injected into a QE-HF mass spectrometer (Q Exactive HF Hybrid Quadrupole Orbitrap™, Thermo Fisher). The DIA acquisition scheme consisted of 45 fixed windows ranging from 350 to 1500 m/z. The windows were set for DIA acquisition as follows: 348–400, 400–424, 424–449, 449–465, 465–478, 478–489, 489–500, 500–514, 514–527, 527–540, 540–550, 550–559, 559–568, 568–579, 579–588, 588–599, 599–609, 609–621, 621–631, 631–641, 641–651, 651–663, 663–674, 674–686, 686–696, 696–708, 708–720, 720–733, 733–746, 746–760, 760–774, 774–788, 788–804, 804–820, 820–837, 837–856, 856–876, 876–898, 898–922, 922–949, 949–979, 979–1017, 1017–1064, 1064–1138, and 1138–1400 m/z. The resolution distribution of MS1 and MS2 was 60,000 and 30,000, respectively. A Spectronaut Pulsar X 12.0 (Biognosys, Schlieren, Switzerland) was used for identification and quantification. Finally, peptides FDR and proteins FDR were all set at 1% (FDR).
Validation of biomarkers via enzyme-linked immunosorbent assay (ELISA)
To verify the prognostic value of biomarkers on the efficacy of NSCLC patients using immunotherapy, we collected plasma samples of an external cohort of 76 NSCLC patients. The ELISA kit we used was assessed from Novus, Proteintech, and Sino Biological. The detailed steps were strictly followed by the manufacturer’s instruction.
Data analysis
We included 615 positive array-detected proteins and 509 MS proteins in the analyses, and all proteins were named by gene names. The testing data were normalized using the quantile method and log2 transformed. To investigate differentially expressed plasma proteins (DEPs) in pre-treatment samples between the R and NR groups and during treatment among the ASPS, NSCLC, and lymphoma patients, the Mann–Whitney U test was used, and differences with p < 0.05 were defined as statistically significant. The DEPs were clustered by the Hiplot platform (https://hiplot.com.cn).
Pathway and Gene Ontology (GO) enrichment analyses were performed by ClueGo in Cytoscape (version3.8.0) or omicsbean (http://www.omicsbean.cn/login/?next=/dashboard/). Protein drug targets were obtained from the Human Protein Atlas (HPA), comprehensive information was collected from the HPA and the Therapeutic Target Database (TTD) [27], and information on clinical trials was obtained from the clinical trial database (https:// clinicaltrials.gov/). Hierarchical clustering and principle component analysis (PCA) were implemented and plotted using the statistical language R (version 4.2.3). A Venn diagram was constructed using an online platform (http://bioinformatics.psb.ugent.be/webtools/Venn/). We used TIMER2.0 for analysis of immune infiltrates [28]. Survival curves were constructed using Kaplan–Meier analyses. Multivariate Cox regression analyses were applied to further identify the prognostic effect of the biomarkers. In group comparisons of categorical variables, chi-square test was used. The analyses were carried out via GraphPad Prism (version 8.0) and R (version 4.2.3).
Results
In-depth profiling of the plasma proteome in cancer patients receiving anti-PD1 therapy
The plasma samples from NSCLC, ASPS, and lymphoma patients were collected before and at various time points after treatment (Fig. 1A). The plasma proteome was detected by DIA-MS and antibody microarray as previously described [19] (Fig. 1B). The detection correlation coefficients of plasma proteins within and among different experiments using antibody microarray were 0.976 and 0.913, respectively (Figure S1). To assess the reproducibility of DIA-MS, we employed H293 cell lysates as a control, which was tested in 45 consecutive time points throughout the plasma screen. The average Pearson correlation coefficient of 45 QC tests was 0.94 (Figure S2). These results suggest that our in-depth proteomic platform in plasma proteome screening is reproducible.
Using our platform, 96.5% (615/637, Figure S3) of the proteins were detected by microarray. We identified 1018, 1019, and 1012 proteins in NSCLC, ASPS, and lymphoma patients, respectively. Notably, there were no marked differences between the number of proteins identified in the R and NR patient groups in the three cancers (Fig. 1C, D). The concentration of these proteins was distributed across 12 orders of magnitude in plasma (Fig. 1E). Bioinformatics analysis showed that the proteins detected by antibody microarrays enriched B cell and T cell activation; CCKR, P53, PI3K, interleukin, PDGF, TGF-β, and VEGF pathways; and the proteins detected by DIA-MS enriched the cadherin, cytoskeletal regulation, proline biosynthesis, nicotinic acetylcholine, fructose galactose metabolism, and pentose phosphate pathways (Fig. 1F). These results demonstrate the advantages of our platform in acquiring the expression information of plasma proteins according to breadth (> 1000 proteins) and depth (12 orders of magnitude).
Proteomic landscape mapping of the dysregulated pathways in anti-PD1-resistant cancer patients
Using the Mann–Whitney U test, 50 (NR 32 vs. R 18), 206 (NR 172 vs. R 34), and 268 (NR 179 vs. R 89) differentially expressed proteins were identified in NSCLC, ASPS, and lymphoma patients, respectively (Fig. 2A–C). Principle component analysis (PCA) revealed that the plasma profile in R group was distinct to that in NR patients (Figure S4). GO terms of these DEPs were enriched in processes of cytokine secretion and angiogenesis regulation in NSCLC, cell-substrate adhesion and metabolism in ASPS, and protein activation and humoral immune response in lymphoma. Moreover, some common processes were shared in NR patients of the three cancers, such as platelet degranulation (Figure S5). KEGG pathway analysis revealed that proteins upregulated in NR patients were enriched in cytokine-cytokine receptor interactions and TNF signal pathways in NSCLC (Fig. 2D), adherent junction and apoptosis in ASPS (Fig. 2E), and EGFR TKI resistance and complement coagulation cascades in lymphoma patients (Fig. 2F). Some common pathways were shared in NR patients compared to R patients across three cancer types, including immune-related pathways such as Th17 cell differentiation, the IL-17 signal pathway, and the HIF-1 signal pathway, as well as tumor, infection, autoimmune disease-related pathways such as the JAK-STAT signal pathway and cell adhesion pathways (Fig. 2D–F). For R patients, proteins altered might be involved in cellular senescence and transcriptional misregulation pathways (Fig. 2D–F). The activated pathway details are shown in Figure S6. Some differentially expressed proteins in cell adhesion (CADM1 in NSCLC, TUBA1B and ITGA5 in ASPS, and CDH5 and ICAM3 in lymphoma) and immune modulation (CCR3 and CD27 in NSCLC, FOS and MMP2 in ASPS, and CXCL13 and CCL26 in lymphoma) are shown in Figure S7.
Longitudinal changes of the plasma proteome of cancer patients after therapy
We performed longitudinal analyses of proteomic changes before and after anti-PD1 therapy, wherein we identified 339, 462, and 800 overexpressed proteins in the R group and 354, 201, and 258 overexpressed proteins in the NR group of NSCLC, ASPS, and lymphoma patients, respectively (p < 0.05). The DEPs were classified into six patterns by the Hiplot platform, and the pathways of each cluster were annotated by ClueGo in Cytoscape. The corresponding pathways for every cluster in the R and NR groups of NSCLC, ASPS, and lymphoma patients are shown in Figures S8–S10, respectively. Downregulated proteins after treatment in R were significantly enriched in the IL-17 signal pathway, whereas upregulated proteins were enriched in the vitamin digestion and absorption pathway (Fig. 3A–C and S11). For NR patients, proteins involved in the complement and coagulation cascades pathway were upregulated after treatment (Fig. 3D–F). These findings imply that the dysfunction of IL-17 signal modulation and coagulation function probably related to the benefit of anti-PD1 therapy.
Notably, we identified 15 noninvasive monitoring biomarkers whose expression is well correlated with changes in tumor size in the three cancers (R > 0.8, p < 0.05) (Fig. 3G). GO enrichment analysis further identified six proteins (CD19, CFI, IGHV3OR15-7, IGHV4-39, LTA, MBL2) related to adaptive immune response (p < 0.05). Longitudinal analysis showed that the expression of IGHV4-39 possessed a similar trend, while MBL2 and LTA showed an opposite trend to tumor size, which may have the potential to predict cancer recurrence after therapy (Fig. 3H, I).
Identification of combinatorial targets in cancer patients who did not benefit from anti-PD1 therapy
To identify protein targets for cancer patients treated with anti-PD1 antibodies, we performed Venn diagram analysis of 1019 proteins that were detected using our in-depth plasma proteomics platform and 2080 protein targets from the HPA database (https://www.proteinatlas.org/). 214 proteins including 128 approved and 86 potential targets were identified (Fig. 4A). We further selected 40 potential targets whose expressions were upregulated in NR patients or downregulated in R patients among the list of all DEPs (Fig. 4B). Protein class analysis indicated these proteins belonged to signal receptor, enzyme, activity modulator, cytokine, and other classes (Fig. 4C). KEGG pathway analysis showed that these 40 proteins significantly enriched in cancer signaling pathways, including the HIF-1, JAK-STAT, cytokine–cytokine receptor interaction, and p53 signal pathways (Fig. 4D).
Detailed information on these targets, including full name, bioclass, drug information, and indications, is shown in Table S3. Among these protein targets, 70% (28/40) of the targets were approved or in clinical trials, and 66% (8/12) of these were administered in combination in clinical trials and have entered phases II and III. The approved indications focused on tumor/leukemia, autoimmune disease, or infectious disease (Fig. 4E). Notably, four clinical trials on myeloma, diffuse large B cell lymphoma (DLBCL), melanoma, and NSCLC are ongoing which combine anti-PD1 antibody and IL-17A (NCT03111992), CD22 (NCT03287817), KIT (NCT04493203), or AXL (NCT04681131), respectively (Fig. 4F).
To explore potential combination therapy mechanisms of anti-IL-17A and immunotherapy, analysis of the IL-17 signal relevant data showed high expression of multiple molecules on the pathway including MAPKs, IL6, CXCL8, MMP9, etc. The immune infiltration showed IL-17A was positive correlated with expression microphage M2, PD-L1, T cell regulatory (Tregs), negatively correlated with macrophage M1, in general, creating an immunosuppressive microenvironment (Figure S12). The therapeutic benefits of these combinatorial therapies to cancer patients have yet to be identified.
Validation of predictive biomarkers in the independent lymphoma cohort and external NSCLC cohort
To validate our findings, we collected pre-treatment samples from a validation cohort of 39 lymphoma patients, including 20 R and 19 NR patients. The results showed that 110 of 268 differentially expressed proteins in the lymphoma discovery cohort were successfully validated (p < 0.05). PCA analysis using the discovery and validation cohorts showed that patients with different responses were distributed in two separate areas (Fig. 5A, B). Pathway analysis showed that the validated proteins significantly enriched immune-related pathways, including the Th17 cell differentiation, IL-17 signal pathway, and estrogen signal pathways (Figure S13).
To identify specific predictive biomarkers, we selected five biomarkers (F5, FLT4, GNPTG, IL-17A, and SFTPB) that were differentially expressed between the R and NR patient groups in both lymphoma cohorts from the top 20% of significantly differentially expressed proteins (p < 0.05). The AUCs of these five biomarkers (F5, FLT4, GNPTG, IL-17A, and SFTPB) were 0.72, 0.69, 0.72, 0.72, and 0.74 in the discovery cohort and 0.75, 0.74, 0.69, 0.69, and 0.76 in the validation cohort, respectively (Fig. 5C, D). The results indicate that these biomarkers may potentially be utilized in predicting anti-PD1 therapy outcomes, though they still require validation in a large independent cohort.
To further validate the predictive capability of the biomarkers in NSCLC patients, we collected an external validation cohort of 76 pre-treatment NSCLC patients, including 33 R and 43 NR. Three (TNFSF12, CCL3, and KIT) biomarkers were observed to be effective in clinical validation. In KIT and TNFSF12 high expression group, significantly prolonged PFS (KIT: p = 0.012; TNFSF12: p = 0.030) and higher ratio of responder patients toward anti-PD1 therapy (KIT: 57% vs. 30%, p = 0.012; TNFSF12: 67% vs. 41%, p = 0.037) were observed. In CCL3 high expression group, patients presented a worse PFS (p = 0.030) and the proportion of non-responder patients was higher (60% vs. 37%, p = 0.024) compared to CCL3 low expression group (Fig. 5E, F). PD-L1 expression is a known predictive biomarker for anti-PD1 therapy in NSCLC; however, it is limited by the availability of biopsy tissue. In patients with PD-L1 expression available, the PD-L1 expression did not appear as a significant predictor of PFS and OS outcome in our cohort, and no association was observed between PD-L1 expression and three (TNFSF12, CCL3, and KIT) biomarkers (Figure S14). To avoid potential confounding factors, we did multivariate Cox regression analyses of the clinical characteristics including PD-L1 expression and the three plasma biomarkers. Multivariate Cox regression analyses confirmed that TNFSF12, CCL3, and KIT were independent risk factors (Figure S15).
Discussion
Although extensive studies have been conducted in the field of immunotherapy, understanding of the molecular mechanism of anti-PD1 treatment of cancer remains unclear, and the availability of biomarkers for predicting responses remains limited. We conducted the largest, to our knowledge, dynamic proteomic study of 193 ASPS, NSCLC, and lymphoma patients who received anti-PD1 therapy using an in-depth plasma proteomic platform. And we validated the prognostic biomarkers in lymphoma (n = 39) and NSCLC cohort (n = 76).
The results identified a total of 534 DEPs, which involved in Th17 cell differentiation, IL-17 signaling pathway, JAK-STAT signaling pathway, and cell adhesion molecular pathways. Helper T cells 17 (Th17) are a subpopulation of T cells that are capable of secreting IL-17, IL-21, and IL-22, which mainly play important roles in autoimmunity and defense response against extracellular bacteria or fungi [29]. Th17 cell differentiation is induced by IL-23, STAT3, and retinoid acid-related-orphan nuclear receptorγt (RORγt). The activation of RORγt initiates the differentiation cascade of Th17 cells; following activation, RORγt promotes the expression of the IL-17 and IL-23 receptors (IL-23R) [30]. The JAK-STAT signaling pathway is necessary for immune modulation of host immune responses or immune interactions with non-immune factors [31, 32]. Besides Th17 cells, IL-17A can be secreted by natural killer T cells (NKT) and lymphoid tissue-inducing cells. IL-17 plays a role in promoting tumor development by facilitating angiogenesis and tumor cell proliferation and inhibiting apoptosis to promote tumor growth [33,34,35]. IL-23R can recruit Jak2, the JAK-STAT signaling system induced by IL-23 regulates Th17 cells, and drugs that inhibit the JAK-STAT signal pathway can target Th17 cells [36]. JAK-STAT signaling components are polarized in epithelial cells, and the JAK-STAT pathway also targets many genes controlling cell polarity and adhesion. Thus, activation of the JAK-STAT pathway is associated with cell adhesion [37]. The activation of JAK-STAT signaling is associated with upregulated PD-L1 expression in tumor cells, which promotes immune cell exhaustion and therapy resistance [38]. Consistent with the training cohort, we confirmed the Th17 and IL-17 signaling pathways in the validation cohort. We hypothesize that the immunosuppressive microenvironment induced by the JAK-STAT, Th17, and IL-17 axis correlates with efficacy of anti-PD1 therapy, although the detailed mechanism has yet to be elucidated.
The low efficiency of anti-PD1 therapy is currently an impeding problem that needs to be solved, and thus, screening for effective markers to predict and identify responder populations and to monitor cancer relapse is essential to improve the success of immunotherapy. To address this question, we validated eight plasma proteins (IL-17A, F5, FLT4, SFTPB, and GNPTG in lymphoma, TNFSF12, CCL3, and KIT in NSCLC) for response prediction and three plasma proteins (IL36G, SERPINC1, and LTA) for relapse monitoring. We found that the upregulated expression of IL-17A is associated with the poor prognosis of anti-PD1 therapy. In line with this finding, one study has reported that an increase in IL-17A can promote lung cancer growth by promoting inflammation, which results in resistance to anti-PD1 therapy and sensitizes tumors to cytokine and neutrophil depletion [39]. We also found that proteins to the IL-17 signal pathway were downregulated following treatment, which could lead to an anti-tumor microenvironment. Studies have shown that IL-17 reduces the presence of CD4 + and CD8 + lymphocytes in the tumor microenvironment, increases infiltrative Tregs, and further promotes angiogenesis, invasion, and metastasis [40]. In addition, coagulation factor V (F5) is the central regulator of hemostasis and results in the activation of prothrombin to thrombin. A study has reported the association between disorders of the coagulation–fibrinolysis system and immune activation by ICIs in cancer patients [41]. Fms-related tyrosine kinase 4 (FLT4) encodes vascular endothelial growth factor receptors (VEGFR3). This protein plays an important role in lymphangiogenesis and tumor metastasis. Studies also reveal that the VEGFR3 signal axis can influence tumor-associated microphages to inhibit anti-tumor immunity and promote tumor growth, and that it is correlated with patient survival [42, 43]. Besides efficacy, the association of blood proteins and toxicity of anti-PD1 therapy or use of corticosteroids is worthy of exploration.
Anti-PD1-resistant cancers require effective therapies, and the discovery of new drug targets or combinational drug targets to reverse anti-PD1 resistance has become a critical issue in the field of immunotherapy. To address this concern, we explored protein targets for combination therapy with anti-PD1 antibodies, which identified 40 potential drug targets that enriched cancer-related pathways. Among the 40 targets identified by longitudinal analysis, at least four clinical trials are ongoing, which is suggestive of its potential use. The IL-17 signaling axis plays an important role in the pathogenesis of rheumatoid arthritis, multiple sclerosis, and systemic lupus erythematosus. Antibodies targeting IL-17A have been approved for the treatment of plaque psoriasis; the observation in our cohort supports the rationale for combining anti-PD1 antibodies with IL-17A-targeted therapy in multiple cancer patients for overcoming immune suppression [44, 45]. A clinical trial utilizing the anti-IL-17A antibody alone or with the anti-PD1 antibody in multiple myeloma patients is ongoing [46]. In addition, the SERPINC1 gene encodes the antithrombin III protein, which was identified in our cohort to be correlated with tumor size and can serve as a monitoring biomarker; medicines targeting SERPINC1 have been approved for venous thrombosis and coagulation defect treatment, although the combinatorial effect of SERPINC1-targeted therapy with anti-PD1 antibodies has yet to be explored.
This study has several limitations. The number of ASPS samples employed in this study is limited, it would be ideal to involve more clinical samples and validate in a large and different cohort. In addition, the detailed roles of the biomarker proteins or function of combinatorial targets with anti-PD1 antibodies require further investigation, such as IL-17A, should be further elucidated or in vitro and in vivo experimentally validated. At last, PD-L1 expression did not appear as a significant predictor of outcome in multivariate analysis in our cohort, which may be due to the small subset of patients with available measured PD-L1 expression (n = 29), and the predictive performance of the proteins in combination with other known biomarkers (e.g., TMB, MSI/dMMR) can also be explored.
In conclusion, our study provides fundamental insights into the molecular changes in different cancer patients before and after anti-PD1 therapy and has identified biomarkers as well as combinatorial targets for patients who are resistant to treatment. These results are valuable for understanding the mechanism of anti-PD1 treatment and for developing new therapeutic strategies.
Data and materials availability
All data associated with this study are available in the main text or supplementary materials.
References
Fritz JM, Lenardo MJ (2019) Development of immune checkpoint therapy for cancer. J Exp Med 216:1244–1254
Homet Moreno B, Ribas A (2015) Anti-programmed cell death protein-1/ligand-1 therapy in different cancers. Br J Cancer 112:1421–1427
Kalbasi A, Ribas A (2020) Tumour-intrinsic resistance to immune checkpoint blockade. Nat Rev Immunol 20:25–39
Administration FaD (2023) https://www.fda.gov/medical-devices/in-vitro-diagnostics/list-cleared-or-approved-companion-diagnostic-devices-in-vitro-and-imaging-tools.
Marcus L, Lemery SJ, Keegan P et al (2019) FDA approval summary: pembrolizumab for the treatment of microsatellite instability-high solid tumors. Clin Cancer Res 25:3753–3758
Marcus L, Fashoyin-Aje LA, Donoghue M et al (2021) FDA approval summary: pembrolizumab for the treatment of tumor mutational burden-high solid tumors. Clin Cancer Res 27:4685–4689
Bai R, Lv Z, Xu D et al (2020) Predictive biomarkers for cancer immunotherapy with immune checkpoint inhibitors. Biomark Res 8:34
Prasad V, Addeo A (2020) The FDA approval of pembrolizumab for patients with TMB >10 mut/Mb: was it a wise decision? No. Ann Oncol 31:1112–1114
Grigg C, Rizvi NA (2016) PD-L1 biomarker testing for non-small cell lung cancer: truth or fiction? J Immunother Cancer 4:48
Cui L, Zhang F (2021) Inappropriate use of the same cutoff by different sequencing panels for tumor mutation burden as immunotherapy biomarker. JAMA Oncol 7:1244–1245
Bonneville R, Krook MA, Kautto EA et al (2017) Landscape of microsatellite instability across 39 cancer types. JCO Precis Oncol 2017:1–15
Jardim DL, Goodman A, de Melo GD et al (2021) The challenges of tumor mutational burden as an immunotherapy biomarker. Cancer Cell 39:154–173
Pilard C, Ancion M, Delvenne P et al (2021) Cancer immunotherapy: it’s time to better predict patients’ response. Br J Cancer 125:927–938
Harel M, Ortenberg R, Varanasi SK et al (2019) Proteomics of melanoma response to immunotherapy reveals mitochondrial dependence. Cell 179:236–250 e218
Siravegna G, Mussolin B, Venesio T et al (2019) How liquid biopsies can change clinical practice in oncology. Ann Oncol 30:1580–1590
Lennon AM, Buchanan AH, Kinde I et al (2020) Feasibility of blood testing combined with PET-CT to screen for cancer and guide intervention. Science 369:eabb9601
Tan Q, Wang D, Yang J et al (2020) Autoantibody profiling identifies predictive biomarkers of response to anti-PD1 therapy in cancer patients. Theranostics 10:6399–6410
Harel M, Oren-Giladi P, Kaidar-Person O et al (2015) Proteomics of microparticles with SILAC Quantification (PROMIS-Quan): a novel proteomic method for plasma biomarker quantification. Mol Cell Proteomics 14:1127–1136
Xu M, Deng J, Xu K et al (2019) In-depth serum proteomics reveals biomarkers of psoriasis severity and response to traditional Chinese medicine. Theranostics 9:2475–2488
Babacic H, Lehtio J, Pico de Coana Y et al (2020) In-depth plasma proteomics reveals increase in circulating PD-1 during anti-PD-1 immunotherapy in patients with metastatic cutaneous melanoma. J Immunother Cancer 8:e000204
Schwartz LH, Litiere S, de Vries E et al (2016) RECIST 1.1-Update and clarification: from the RECIST committee. Eur J Cancer 62:132–137
Shi Y, Su H, Song Y et al (2019) Safety and activity of sintilimab in patients with relapsed or refractory classical Hodgkin lymphoma (ORIENT-1): a multicentre, single-arm, phase 2 trial. Lancet Haematol 6:e12–e19
Rizvi NA, Hellmann MD, Snyder A et al (2015) Cancer immunology. Mutational landscape determines sensitivity to PD-1 blockade in non-small cell lung cancer. Science 348:124–128
Samstein RM, Lee CH, Shoushtari AN et al (2019) Tumor mutational load predicts survival after immunotherapy across multiple cancer types. Nat Genet 51:202–206
Snyder A, Makarov V, Merghoub T et al (2014) Genetic basis for clinical response to CTLA-4 blockade in melanoma. N Engl J Med 371:2189–2199
Wang G, Wang Y, Zhang L et al (2020) Proteomics analysis reveals the effect of Aeromonas hydrophila sirtuin CobB on biological functions. J Proteomics 225:103848
Wang Y, Zhang S, Li F et al (2020) Therapeutic target database 2020: enriched resource for facilitating research and early development of targeted therapeutics. Nucleic Acids Res 48:D1031–D1041
Li T, Fu J, Zeng Z et al (2020) TIMER2.0 for analysis of tumor-infiltrating immune cells. Nucleic Acids Res 48:W509–W514
Chong WP, Mattapallil MJ, Raychaudhuri K et al (2020) The cytokine IL-17A limits Th17 pathogenicity via a negative feedback loop driven by autocrine induction of IL-24. Immunity 53:384–397 e385
Bunte K, Beikler T (2019) Th17 cells and the IL-23/IL-17 axis in the pathogenesis of periodontitis and immune-mediated inflammatory diseases. Int J Mol Sci 20:3394
Villarino AV, Kanno Y, Ferdinand JR et al (2015) Mechanisms of Jak/STAT signaling in immunity and disease. J Immunol 194:21–27
Schwartz DM, Bonelli M, Gadina M et al (2016) Type I/II cytokines, JAKs, and new strategies for treating autoimmune diseases. Nat Rev Rheumatol 12:25–36
Razi S, Baradaran Noveiry B, Keshavarz-Fathi M et al (2019) IL-17 and colorectal cancer: from carcinogenesis to treatment. Cytokine 116:7–12
Zhang Q, Liu S, Zhang Q et al (2014) Interleukin-17 promotes development of castration-resistant prostate cancer potentially through creating an immunotolerant and pro-angiogenic tumor microenvironment. Prostate 74:869–879
Benevides L, da Fonseca DM, Donate PB et al (2015) IL17 Promotes mammary tumor progression by changing the behavior of tumor cells and eliciting tumorigenic neutrophils recruitment. Cancer Res 75:3788–3799
Raychaudhuri SK, Abria C, Raychaudhuri SP (2017) Regulatory role of the JAK STAT kinase signalling system on the IL-23/IL-17 cytokine axis in psoriatic arthritis. Ann Rheum Dis 76:e36
Chen SL, Cai GX, Ding HG et al (2020) JAK/STAT signaling pathway-mediated microRNA-181b promoted blood-brain barrier impairment by targeting sphingosine-1-phosphate receptor 1 in septic rats. Ann Transl Med 8:1458
Lu C, Talukder A, Savage NM et al (2017) JAK-STAT-mediated chronic inflammation impairs cytotoxic T lymphocyte activation to decrease anti-PD-1 immunotherapy efficacy in pancreatic cancer. Oncoimmunology 6:e1291106
Akbay EA, Koyama S, Liu Y et al (2017) Interleukin-17A promotes lung tumor progression through neutrophil attraction to tumor sites and mediating resistance to PD-1 blockade. J Thorac Oncol 12:1268–1279
Li J, Lau GK, Chen L et al (2011) Interleukin 17A promotes hepatocellular carcinoma metastasis via NF-kB induced matrix metalloproteinases 2 and 9 expression. PLoS ONE 6:e21816
Sato R, Imamura K, Sakata S et al (2019) Disorder of coagulation-fibrinolysis system: an emerging toxicity of Anti-PD-1/PD-L1 monoclonal antibodies. J Clin Med 8:762
Crona DJ, Skol AD, Leppanen VM et al (2019) Genetic variants of VEGFA and FLT4 are determinants of survival in renal cell carcinoma patients treated with sorafenib. Cancer Res 79:231–241
Tacconi C, Ungaro F, Correale C et al (2019) Activation of the VEGFC/VEGFR3 pathway induces tumor immune escape in colorectal cancer. Cancer Res 79:4196–4210
Li S, Na R, Li X et al (2022) Targeting interleukin-17 enhances tumor response to immune checkpoint inhibitors in colorectal cancer. Biochim Biophys Acta Rev Cancer 1877:188758
Liu C, Liu R, Wang B et al (2021) Blocking IL-17A enhances tumor response to anti-PD-1 immunotherapy in microsatellite stable colorectal cancer. J Immunother Cancer 9:e001895
Ruiz de Morales JMG, Puig L, Dauden E et al (2020) Critical role of interleukin (IL)-17 in inflammatory and immune disorders: an updated review of the evidence focusing in controversies. Autoimmun Rev 19:102429
Acknowledgements
We thank LetPub (www.letpub.com) for its language editing service during the preparation of this manuscript.
Funding
This work was supported by the National Key Research and Development Program of China (2022YFC2703100), New National Natural Science Foundation of China (82200212), State Key Laboratory of Proteomics (SKLP-O202205), and Beijing Municipal Natural Science Foundation (L234034).
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YKS and XHH designed and supervised the study. YKS, XHH, QYT, JLY, PYX, SY, SSW, JRY, ZSZ, LT, and RYG collected the patient plasma samples and clinical data. QYT, XMZ, GBW, and RYG collected the experimental data. XHH, YKS, XBY, QYT, XMZ, and RYG analyzed the data and did the statistical analysis. QYT, XMZ, and RYG wrote the manuscript, and YKS, XHH, and XBY revised the manuscript. All authors reviewed the manuscript and approved the final version.
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This study was approved by the Ethics Committee of the National Cancer Center/National Clinical Research Center for Cancer/Cancer Hospital, Chinese Academy of Medical Sciences & Peking Union Medical College (Permission No.19–019/1804). Written informed consent was obtained from individual or guardian participants.
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Tan, Q., Gao, R., Zhang, X. et al. Longitudinal plasma proteomic analysis identifies biomarkers and combinational targets for anti-PD1-resistant cancer patients. Cancer Immunol Immunother 73, 47 (2024). https://doi.org/10.1007/s00262-024-03631-7
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DOI: https://doi.org/10.1007/s00262-024-03631-7