Published online Nov 15, 2020. doi: 10.4251/wjgo.v12.i11.1216
Peer-review started: August 9, 2020
First decision: August 22, 2020
Revised: September 6, 2020
Accepted: September 18, 2020
Article in press: September 18, 2020
Published online: November 15, 2020
Processing time: 94 Days and 12 Hours
Programmed death ligand 1 (PD-L1) immunotherapy remains poorly efficacious in colorectal cancer (CRC). The recepteur d’origine nantais (RON) receptor tyrosine kinase plays an important role in regulating tumor immunity.
To identify the patterns of RON and PD-L1 expression and explore their clinical significance in CRC.
Gene expression data from the Gene Expression Omnibus database (GEO; n = 290) and patients at the First Affiliated Hospital, Zhejiang University School of Medicine (FAHZUSM; n = 381) were analyzed to determine the prognostic value of RON and PD-L1 expression within the tumor microenvironment of CRC. HT29 cell line was treated with BMS-777607 to explore the relationship between RON activity and PD-L1 expression. Signaling pathways and protein expression perturbed by RON inhibition were evaluated by cellular immunofluorescence and Western blot.
In the GEO patient cohort, cut-off values for RON and PD-L1 expression were determined to be 7.70 and 4.3, respectively. Stratification of patients based on these cutoffs demonstrated that high expression of RON and PD-L1 was associated with a poor prognosis. In the FAHZUSM cohort, rates of high expression of RON in tumor cells, high PD-L1 expression in tumor cells and tumor infiltrating monocytes, and both high RON and high PD-L1 expression in the tumor microenvironment were 121 (32%), 43 (11%), 91 (24%), and 51 (13.4%), respectively. High expression of RON was significantly correlated with high expression of PD-L1 in the tumor cell compartment (P < 0.001). High expression of RON and that of PD-L1 were independent prognostic factors for poorer overall survival. Concurrent high expression of both RON and PD-L1 in the tumor microenvironment was significantly associated with a poor prognosis. In vitro, BMS-777607 inhibited the phosphorylation of RON, inhibited PD-L1 expression, and attenuated activation of the ERK1/2 and AKT signaling pathways in CRC cells.
RON, PD-L1, and their crosstalk are significant in predicting the prognostic value of CRC. Moreover, phosphorylation of RON upregulates PD-L1 expression, which provides a novel approach to immunotherapy in CRC.
Core Tip: Recepteur d’origine nantais (RON) expression plays an important role in regulating tumor immunity, and the efficacy of programmed death ligand 1 (PD-L1) immunotherapy in colorectal cancer (CRC) is still not satisfactory. This inspired us to study the clinical significance and correlation of RON and PD-L1 in CRC. The major discoveries and findings in this study are: (1) The abnormal expression of RON and PD-L1 was not only correlated, but was also significant biomarkers for poor prognosis of CRC. This finding was identified in 389 primary CRC clinical samples via multiplex immunofluorescence staining and immunohistochemistry staining; and (2) In in vitro experiments, activation of RON phosphorylation up-regulated the expression of PD-L1 in CRC cells.
- Citation: Liu YZ, Han DT, Shi DR, Hong B, Qian Y, Wu ZG, Yao SH, Tang TM, Wang MH, Xu XM, Yao HP. Pathological significance of abnormal recepteur d’origine nantais and programmed death ligand 1 expression in colorectal cancer. World J Gastrointest Oncol 2020; 12(11): 1216-1236
- URL: https://www.wjgnet.com/1948-5204/full/v12/i11/1216.htm
- DOI: https://dx.doi.org/10.4251/wjgo.v12.i11.1216
Colorectal cancer (CRC) is the fourth most common malignancy worldwide in 2018[1]. Despite advances in CRC treatment methods, it still has a poor prognosis, and many patients will have local recurrence and/or distant metastasis within 5 years after treatment[2].
Immunotherapy has become a promising strategy for treating a wide variety of malignancies[3]. Therapeutic antibodies that block the activity of programmed death ligand 1 (PD-L1, also known as CD274) protein are effective against many cancer types[4]. PD-L1 is a transmembrane immune checkpoint protein that can be expressed on both immune cells and cancer cells, including CRC cells[5-7]. When expressed on immune cells, PD-L1 can be regulated by a variety of inflammatory mediators and cytokines. When expressed on the surface of tumor cells (TCs), PD-L1 enables TCs to evade the immune system[8,9]. Cancer cells can induce the expression of PD-L1 through activation of oncogenic pathways, such as the RAS-ERK or PI3K-AKT pathways, to facilitate immune escape[10-12].
However, the efficacy of PD-L1 immunosuppressive agents in CRC is poor[13,14]. The overall poor response of CRC to PD-L1 blockade may be due to the activity of multiple oncogenes[15,16]. For example, KRAS mutations can up-regulate the expression of PD-L1 in CRC cells, thereby reducing the efficacy of PD-L1 immunosuppressive agents[17]. RON (macrophage-stimulating 1 receptor, MST1R), a member of the MET proto-oncogene family and a receptor for MSP, is an effector of KRAS signaling, and exhibits “KRAS addiction”, a phenomenon that plays an important role in the initiation and development of tumors[18-20]. RON is overexpressed pathologically in various types of cancer, including CRC, and many small-molecule inhibitors are being developed to target RON and its associated compounds[20-22]. BMS-777607 is a highly selective small molecule inhibitor of RON (IC50 1.8nM for RON)[23]. Activation of RON leads to RON phosphorylation, which then activates different signaling pathways in cancer cells, including the RAS-ERK and PI3K-AKT pathways[24-26]. Interactions between RON and other membrane receptors further promote pathway activation, enhancing the migration and invasion of CRC cells[20,22]. In addition, overexpression of RON can damage immune cells and inhibit anti-tumor immunity[27,28]. Thus, abnormal expression of RON may affect the efficacy of PD-L1 immunotherapy in CRC.
In this study, we investigated the clinical significance of expression patterns of RON and PD-L1 in primary CRC samples, and evaluated the potential for RON and PD-L1 as prognostic biomarkers in CRC. We treated CRC cells with BMS777607 in vitro to explore if RON inhibition affects the expression of PD-L1 and results in changes in related signaling pathways in CRC cells. Our data suggested that RON inhibition may be a novel approach to augment immunotherapy in CRC.
This study involved a GEO (Gene Expression Omnibus) cohort and a FAHZUSM (The First Affiliated Hospital, Zhejiang University School of Medicine) cohort. In the GEO cohort, the median age of all 287 CRC patients was 70 years (range: 24-97 years). There were 158 (55.1%) male patients and 129 (44.9%) female patients. The median survival time was 58 months, and 94 patients died during follow-up. In the FAHZUSM cohort, the median age of the CRC patients undergoing tumor resection was 61 years (range: 29-94 years). In this cohort, 215 (56.4%) patients were male and 166 (43.6%) were female. The median survival time was 100 months, and 91 patients died during follow-up. The primary site of a tumor, pathological grade, TNM stage, disease stage, histological type, and treatment status of CRC patients are shown in Table 1.
FAHZUSM cohort (n = 381) | GEO cohort (n = 287) | ||||||||||||||||
Characteristic | Cases | RON expression | PD-L1 expression | Cases No (%) | RON expression | PD-L1 expression | |||||||||||
Low | High | 1P value | Low | High (TIMC) | 2P value | Low | High (TC) | 3P value | Low | High | 1P value | Low | High (TC) | 3P value | |||
No. of cases number | 381 | 260 | 121 | 247 | 91 | 247 | 43 | 287 | 193 | 94 | 48 | 239 | |||||
Age (mean ± SD) | 61.16 ± 12.419 | 60.40 ± 12.560 | 62.81 ± 11.997 | 0.859 | 60.94 ± 12.37 | 62.04 ± 13.080 | 0.771 | 60.94 ± 12.37 | 61.16 ± 12.419 | 0.938 | 68.44 ± 14.00 | 66.87 ± 13.18 | 71.65 ± 15.12 | 0.006 | 66.94 ± 14.33 | 68.74 ± 13.95 | 0.417 |
Sex | |||||||||||||||||
Man | 215 (56.4) | 157 (60.4) | 58 (47.9) | 0.023 | 143 (57.9) | 54 (59.3) | 0.811 | 143 (57.9) | 18 (41.9) | 0.051 | 158 (55.1) | 111 (57.5) | 47 (50) | 0.230 | 30 (62.5) | 128 (53.6) | 0.256 |
Women | 166 (43.6) | 103 (39.6) | 63 (52.1) | 104 (42.1) | 37 (40.7) | 104 (42.1) | 25 (58.1) | 129 (44.9) | 82 (42.5) | 47 (50) | 18 (37.5) | 111 (46.4) | |||||
Principal diagnosis | |||||||||||||||||
Rectum | 229 (60.1) | 158 (61.1) | 71 (58.7) | 0.698 | 153 (61.9) | 47 (51.6) | 0.088 | 153 (61.9) | 29 (67.4) | 0.491 | 165 (57.5) | 111 (57.5) | 54 (57.4) | 0.920 | 34 (70.8) | 131 (54.8) | 0.040 |
Colon | 152 (39.9) | 102 (38.9) | 50 (41.3) | 94 (38.1) | 44 (48.4) | 94 (38.1) | 14 (32.6) | 122 (42.5) | 82 (42.5) | 40 (42.6) | 14 (29.2) | 108 (45.2) | |||||
Pathological grade | |||||||||||||||||
Well/moderate | 9 (2.4) | 6 (2.3) | 3 (2.5) | 0.177 | 5 (2) | 3 (3.3) | 0.778 | 5 (2) | 1 (2.3) | 0.898 | NA | ||||||
Poor | 346 (90.8) | 232 (89.2) | 114 (94.2) | 224 (90.7) | 82 (90.1) | 224 (90.7) | 40 (93) | ||||||||||
Unknown | 26 (6.8) | 22 (8.5) | 4 (3.3) | 18 (7.1) | 6 (6.3) | 18 (7.3) | 2 (4.7) | ||||||||||
T stage | |||||||||||||||||
Tis-T2 | 107 (28.1) | 85 (32.7) | 22 (18.2) | 0.001 | 73 (29.6) | 23 (25.3) | 0.105 | 73 (29.6) | 11 (25.6) | 0.864 | 28 (9.7) | 18 (9.3) | 10 (10.6) | 0.459 | 3 (6.3) | 25 (10.5) | 0.437 |
T3 | 177 (46.5) | 121 (46.5) | 56 (46.3) | 118 (47.8) (46.8%) | 37 (40.7) | 118 (47.8) | 22 (51.2) | 208 (72.5) | 144 (74.6) | 64 (68.1)20 | 39 (81.3) | 169 (70.7) | |||||
T4 | 97 (25.5) | 54 (20.8) | 43 (35.5) | 56 (22.7) | 31 (34.1) | 56 (22.7) | 10 (23.3) | 51 (17.8) | 31 (16.1) | 20 (21.3) | 6 (12.5) | 45 (18.8) | |||||
N stage | |||||||||||||||||
N0 | 251 (65.9) | 184 (70.8) | 67 (55.4) | 0.003 | 164 (66.4) | 62 (68.1) | 0.764 | 164 (66.4) | 25 (58.1) | 0.294 | 141 (49.1) | 97 (50.3) | 44 (46.8) | 0.583 | 27 (56.3) | 114 (44.7) | 0.279 |
N (1-2) | 91 (23.9) | 76 (29.2) | 54 (44.6) | 83 (33.6) | 29 (31.9) | 83 (33.6) | 12 (27.9) | 146 (50.9) | 96 (49.7) | 50 (53.2) | 21 (43.7) | 125 (52.3) | |||||
M stage | |||||||||||||||||
M0 | 368 (96.6) | 252 (96.9) | 116 (95.9) (96.3%) | 0.822 | 241 (97.6) | 85 (93.4) | 0.133 | 241 (97.6) | 42 (97.7) | 1.000 | 268 (93.4) | 183 (94.8) | 85 (90.4) | 0.160 | 47 (97.9) | 221 (92.5) | 0.216 |
M1 | 13 (3.4) | 8 (3.1) | 5 (4.1) | 6 (2.4) | 6 (6.6) | 6 (2.4) | 1 (2.3) | 19 (6.6) | 10 (5.2) | 9 (9.6) | 1 (2.1) | 18 (7.5) | |||||
Disease stage | |||||||||||||||||
0-II | 246 (64.6) | 180 (69.2) | 66 (54.5) | 0.016 | 162 (65.6) | 59 (64.8) | 0.897 | 162 (65.6) | 25 (58.1) | 0.346 | 139 (48.4) | 95 (49.2) | 44 (46.8) | 0.701 | 27 (56.3) | 112 (46.9) | 0.235 |
III-IV | 135 (35.4) | 80 (30.8) | 55 (45.5) | 85 (34.4) | 32 (35.2) | 85 (34.4) | 18 (41.9) | 148 (51.6) | 98 (50.8) | 50 (53.2) | 21 (43.8) | 127 (53.1) | |||||
Histological type | |||||||||||||||||
Adenocarcinoma | 335 (87.9) | 227 (87.3) | 108 (89.3) | 0.706 | 214 (86.6) | 84 (92.3) | 0.130 | 214 (86.6) | 37 (86) | 0.488 | 287 (100) | 193 (100) | 94 (100) | 48 (100) | 239 (100) | ||
Mucinous/SRCC | 36 (9.4) | 25 (9.6) | 11 (9.1) | 28 (11.3) | 4 (4.4) | 28 (11.3) | 4 (9.3) | 0 (0) | 0 (0) | 0 (0) | 0 (0) | 0 (0) | |||||
Other | 10 (2.6) | 8 (3.1) | 2 (1.7) | 5 (2.0) | 3 (3.3) | 5 (2.0) | 2 (4.7) | 0 (0) | 0 (0) | 0 (0) | 0 (0) | 0 (0) | |||||
Treatment | |||||||||||||||||
Yes | 173 (45.4) | 110 (42.3) | 63 (52.1) | 0.043 | 112 (45.3) | 38 (41.8) | 0.694 | 112 (45.3) | 23 (32.6) | 0.472 | 115 (40.1) | 89 (46.1) | 26 (27.7) | 0.003 | 22 (45.8) | 93 (38.9) | 0.372 |
No | 158 (41.5) | 119 (45.8) | 39 (32.2) | 105 (42.5) | 39 (42.9) | 105 (42.5) | 14 (53.5) | 172 (59.9) | 104 (53.9) | 68 (72.3) | 26 (54.2) | 146 (61.1) | |||||
Unknown | 50 (13.1) | 31 (11.9) | 19 (15.7) | 30 (12.1) | 14 (15.4) | 30 (12.1) | 6 (14) | 0 (0) | 0 (0) | ||||||||
PD-L1 (protein) | |||||||||||||||||
Low | 247 (64.8) | 177 (73.1) | 70 (26.9) | 0.9764 | NA | ||||||||||||
High (TIMCs) | 91 (23.9) | 65 (26.9) | 26 (27.1) | ||||||||||||||
High (TCs) | 43 (11.3) | 18 (9.2) | 25 (26.3) | < 0.0015 | |||||||||||||
PD-L1 (mRNA) | |||||||||||||||||
Low | NA | 48 (16.7) | 31 (16.1) | 17 (18.1) | 0.666 | ||||||||||||
High | 239 (83.3) | 162 (83.9) | 77 (81.9) |
The CRC cell line HT29 was obtained from the American Type Cell Culture (ATCC, Manassas, VA, United States). Flow cytometric analysis revealed that RON and PD-L1 were strongly expressed in HT29 cells (Supplementary Figure 1). Cells were cultured in growth medium supplemented with 10% fetal bovine serum and incubated under standard cell culture conditions at 37 °C and 5% CO2. Rabbit anti-RON antibody (5029) and mouse anti-RON monoclonal antibodies (Zt/f2 and Zt/g4) were used as previously described[28]. Macrophage-stimulating protein (MSP) is an activation factor for RON receptor tyrosine kinase phosphorylation and catalytic activity of a number of signal transduction proteins[29]. Human mature MSP was obtained from R&D Systems (Minneapolis, MN, United States). Antibodies against phospho-tyrosine (P-Tyr-100, Cat # 9411), AKT (Cat # 4685), phospho-AKT (Cat # 4060), extracellular signaling regulated kinase (ERK) 1/2 (Cat # 4695), and phospho-ERK1/2 (p44/42) (Cat # 4376) were obtained from Cell Signaling Technology (Beverly, MA, United States). CK antibody was from ZSGB-BIO (Cat # ZM-0069, Beijing, China). The BMS-777607 RON inhibitor was from Medchem Express (Monmouth Junction, NJ, United States). BMS-777607 was dissolved in dimethyl sulfoxide (DMSO) to a final concentration of 10 mmol/L and stored at -20 °C. The PD-L1 antibody (Cat # 13864) for immunohistochemistry and multiplex immunofluorescence was obtained from Cell Signaling Technology (Beverly, MA, United States). The PD-L1 antibody (Cat # 205921) used for cell experiments was from Abcam (Burlingame, CA, United States). Opal tyramine signal amplification (TSA) staining kit was from PerkinElmer (Hopkinton, MA, United States).
Gene expression data for RON and PD-L1 and clinical data for CRC patients are available from the GEO database and accessed through the browser web site (https://geonames.org/)[30]. A total of 290 primary CRC tumors from patients with detailed RON and PD-L1 expression data were selected from the GEO database, based on the completeness of patient clinical data. Only patients with complete tumor characteristics, overall survival (OS), and RNA-seq information, and patients whose tumor samples were obtained prior to treatment were included. The clinicopathologic features of the patients included age, sex, tumor location, histological type, tumor-lymph node-metastasis (TNM) stage, treatment regimen, and OS.
The CRC specimens used for this study were obtained from 381 CRC patients who were pathologically diagnosed and treated between January 2006 and November 2009 at the FAHZUSM. Clinical data for patients included age, sex, tumor location, histological type, TNM stage, tumor differentiation, treatment pattern, and OS rate (Table 1). CRC tissues were fixed in 10% buffered formalin, embedded in paraffin, and were available for immunohistochemical (IHC) evaluation. Detailed demographic data and clinical features of the FAHZUSM cohort are provided in Table 1. This study was approved by the Ethics Committee of the First Affiliated Hospital, Zhejiang University School of Medicine (reference number: 2017427-1).
Multiplex immunofluorescence staining of paraffin-embedded sections was performed using Zt/f2 (5 μg/mL) as the primary antibody for RON, rabbit anti-PD-L1 antibody (1:150, 13864, CST) for PD-L1, and mouse anti-CK mAb (1:200, ZM-0069, ZSGB-BIO) for CK, and visualized using the Opal tyramine signal amplification (TSA) staining kit. First, the concentration and sequence of the RON, PD-L1, and CK antibodies were optimized. The primary antibodies/fluorescent dyes for PD-L1/Opal 530, RON/Opal 690, and CK /Opal 520 were applied to the CRC tissues in sequence. Finally, sections were stained with DAPI and mounted with an anti-fading mounting agent. PerkinElmer software version 2.1 was used to analyze multispectral images.
IHC staining was performed according to standard protocols. Primary antibodies were incubated overnight using a dilution of 1:150 for PD-L1 (13684, CST, United States) and 1:800 for RON. Mouse anti-RON mAb (Zt/f2) was used as previously described[31]. The primary antibody was visualized with diaminobenzidine until a brown precipitate appeared at the antigenic site using EnVision + System-HRP (Dako, Carpentaria, CA, United States). Then, sections were counterstained with hematoxylin.
The IHC-stained sections were independently scored by two pathologists who were blinded to the clinicopathological data. RON expression was determined using a semi-quantitative system. According to the percentage of positive staining area in the whole cancer area, the scoring was as follows: 0 (< 5%), 1 (5%-25%), 2 (26%-50%), 3 (51%-75%), and 4 (> 75%). The staining intensity was scored as 0 (negative), 1 (weak), 2 (medium), or 3 (strong). The total score was obtained by adding the positive proportion score and the staining level score. Samples were categorized as follows: Samples with a final staining score ≤ 4 were considered to be low and those with a score of > 4 were considered to be high for RON expression.
PD-L1 expression was evaluated using an anti-PD-L1 rabbit antibody (13684, CST, United States). A cutoff of 5% for the total proportion of cells that were positive for PD-L1 was used, such that samples with < 5% PD-L1 positive cells were considered to be low and samples with ≥ 5% PD-L1 positive cells were considered to be high for PD-L1 expression. This standard has been established in various types of cancer[32-34].
The result of Cell Counting Kit 8 illustrated that the half-maximal inhibitory concentration (IC50) of BMS-777607 in HT29 cells at 72 h was 2 μmol/L (Supplementary Figure 2). HT29 cells were treated with 2 nmol/L MSP, 2 μmol/L BMS-777607, or 2 nmol/L MSP + 2 μmol/L BMS-777607 for 24 h. The culture medium was removed and the cells were washed with ice-cold phosphate buffered saline (PBS). Cells were digested with trypsin, collected, and washed with PBS to remove residual trypsin. Cells were lysed in radioimmunoprecipitation (RIPA) buffer, and 25 μg of total protein per sample was separated by 8% SDS-PAGE. Western blot was performed using antibodies against RON, phospho-RON, PD-L1, ERK1/2, phospho-ERK1/2, AKT, and phospho-AKT; GAPDH protein was evaluated as an internal control to ensure equal sample loading. Immunoreactive protein bands were visually detected using enhanced chemiluminescence reagents.
HT29 cells were cultured overnight in a 6-well plate on a cover slide. After treatment with 2 nmol/L MSP, 2 μmol/L BMS-777607, or 2 nmol/L MSP + 2 μmol/L BMS-777607 for 24 h, cells were fixed with 4% paraformaldehyde at 37 °C for 20 min, then washed with PBS five times for 3 min. Cover slides were then blocked with 5% BSA in PBS at room temperature for 30 min. After that, the cells were incubated with primary antibody against PD-L1 (205921, Abcam, United States) and mouse anti-RON mAb (Zt/f2) overnight at 4 °C. Primary antibodies were then removed by washing with PBS five times for 3 min. The cells were then incubated with a fluorescently labeled secondary antibody in the dark at room temperature for 1 h. Excess secondary antibody was removed and the cells were counterstained with DAPI. Slides were mounted with an anti-quenching agent and sealed. The fluorescently labeled cells were observed using a LEICA DMi8 microscope (Leica). Representative images were selected and photographed.
Clinical quantitative data are expressed as the mean ± standard deviation (SD) and count data are expressed as constituent ratio (%) or ratio (%). Statistical evaluation was conducted with SPSS 25.0 (IBM Corp., Armonk, NY, United States) and GraphPad Prism v.8 (La Jolla, CA, United States). X-tile 3.6.1 software (Yale University, New Haven, CT, United States) was used to determine the optimal cut-off values for RON and PD-L1 expression in the GEO cohort[35]. χ2 tests were used to analyze relationships between clinicopathological parameters and RON and PD-L1 expression. Differences between quantitative data with a normal distribution were compared using two independent samples t-tests between two groups and one-way analysis of variance among three groups and SNK-q test between groups. Kaplan-Meier method and log-rank test were used for OS analysis. Univariate and multivariate Cox regression analyses were used for identifying the risk factors for OS. A P value < 0.05 was considered statistically significant. All confidence intervals (CIs) are stated at the 95% confidence level.
In the GEO cohort, X-tile was used to find the optimal cutoff values to divide the data of RON (the upper panel) and PD-L1 (the lower panel) mRNA expression into either low or high expression by selecting the highest χ2 value and the smallest P value of a standard log-rank test. The cut-off values for RON and PD-L1 mRNA in TCs were determined as 7.70 and 4.30, respectively (Figure 1A and B), and the log-rank χ2 values for RON and PD-L1 were 4.544 and 4.078, respectively. Patients in the GEO cohort were stratified according to RON and PD-L1 status: RON ≤ 7.70 and RON > 7.70, and PD-L1 ≤ 4.30 and PD-L1 > 4.30 (Figure 1A and B). We found that the high expression of RON and PD-L1 was associated with a poor prognosis.
In CRC tissue samples, multiple immunofluorescence staining was used to show the expression patterns of RON in TCs and PD-L1 in the tumor microenvironment. We found that both RON and PD-L1 exhibited membrane-enhanced expression in TCs (Figure 2A); elevated RON expression on the tumor cell membrane was accompanied by enhanced PD-L1 expression in tumor-infiltrating mononuclear cells (TIMCs) (Figure 2B). We also observed cases where PD-L1 expression was enhanced on the tumor cell membrane (Figure 2C) or in TIMCs (Figure 2D), but RON expression was low. Additionally, there were cases where RON expression was enhanced on the TC membrane, but PD-L1 was not expressed in the tumor microenvironment (Figure 2E). In addition, RON and PD-L1 were often accompanied by a cytoplasmic expression of cancer cells. In general, when RON and PD-L1 were enhanced in the tumor cell membrane and cytoplasm, PD-L1 was also expressed in TIMCs. The results of multiplex immunofluorescence are consistent with the evaluation of RON and PD-L1 by immunohistochemical staining (Figure 3A-C).
In the FAHZUSM cohort, CRC patients were divided into two groups based on high or low expression of RON and PD-L1 detected by IHC staining. In 381 CRC patients, high and low RON expression in TCs was observed in 121 (31.8%) and 260 (68.2%), respectively. High and low expression of PD-L1 in TCs and TIMCs was noted in 43 (11.3%) and 91 (23.9%) patients, respectively, and PD-L1 was lowly expressed in TIMCs in 247 (64.8%) cases. None of the patients had high PD-L1 expression in both TCs and TIMCs. Among all samples expressing RON and PD-L1 in TCs, the proportion with both high RON and high PD-L1 expression was 8.6% (25/290), while the proportion of samples expressing high PD-L1 in TIMCs and high RON in TCs was 7.7% (26/338). Chi-square tests were used to determine the correlation between the expression of RON and PD-L1 in tumor tissues. Compared to samples with low expression of RON, samples with high RON expression levels were more likely to have high levels of PD-L1 in TCs, demonstrating a significant correlation between high RON expression and high PD-L1 expression in TCs (P < 0.001, Table 1). The expression of PD-L1 in TIMCs was not significantly correlated with RON expression in TCs (Table 1).
We compared the clinical characteristics of patient groups categorized based on the expression of RON and PD-L1. High expression of RON was associated with gender, T stage, N stage, disease stage, and treatment. High RON and high PD-L1 expression in TCs was related to T stage (Table 2). High expression of RON and PD-L1 (TIMCs) was associated with T stage, principal diagnosis, histological type, and treatment (P < 0.05; Table 3).
Characteristic | Cases | RON and PD-L1 (TCs) expression in the tumor microenvironment | ||||
RON low/PD-L1 low | RON high/PD-L1 low | RON low/PD-L1 high | RON high/PD-L1 high | P value | ||
Number of cases | 290 | 177 | 70 | 18 | 25 | |
Age (mean ± SD) | 60.89 ± 12.215 | 60.37 ± 12.299 | 62.40 ± 12.518 | 58.39 ± 12.930 | 62.12 ± 10.179 | 0.495 |
Sex | ||||||
Man | 161 (55.5) | 108 (61) | 35 (50.0) | 9 (50.0) | 9 (36.0) | 0.061 |
Women | 129 (44.5) | 68 (39) | 35 (50.0) | 9 (50.0) | 16 (64.0) | |
Principal diagnosis | s | |||||
Rectum | 182 (62.8) | 116 (65.5) | 37 (52.9) | 14 (77.8) | 15 (60.0) | 0.149 |
Colon | 108 (37.2) | 61 (34.5) | 33 (47.1) | 4 (22.2) | 10 (40.0) | |
Pathological grade | ||||||
Well/moderate | 6 (2.1) | 3 (1.7) | 2 (2.9) | 0 (0.0) | 1 (4.0) | 0.264 |
Poor | 264 (9.1) | 158 (89.3) | 66 (94.3) | 16 (88.9) | 24 (96.0) | |
Unknown | 20 (6.9) | 16 (9.0) | 2 (2.9) | 2 (11.1) | 0 (0.0) | |
T stage | ||||||
Tis-T2 | 84 (29) | 64 (36.2) | 9 (12.9) | 5 (27.8) | 6 (24.0) | 0.003 |
T3 | 140 (48.3) | 82 (46.3) | 36 (51.4) | 11 (61.1) | 11 (44.0) | |
T4 | 66 (22.8) | 31 (17.5) | 25 (35.7) | 2 (11.1) | 8 (32.0) | |
N stage | ||||||
N0 | 238 (66.9) | 125 (70.6) | 39 (55.7) | 12 (66.7) | 13 (66.4) | 0.072 |
N (1-2) | 118 (33.1) | 52 (29.4) | 31 (44.3) | 6 (33.3) | 12 (33.6) | |
M stage | ||||||
M0 | 283 (97.6) | 173 (97.7) | 68 (97.1) | 18 (100) | 24 (96.0) | 0.735 |
M1 | 7 (2.4) | 4 (2.3) | 2 (2.9) | 0 (0.0) | 1 (4.0) | |
Stage | ||||||
0-II | 187 (64.5) | 123 (69.5) | 39 (55.7) | 12 (66.7) | 13 (52.0) | 0.110 |
III-IV | 103 (35.5) | 54 (30.5) | 31 (33.3) | 6 (33.3) | 12 (48.0) | |
Histological type | ||||||
Adenocarcinoma | 251 (86.6) | 152 (85.9) | 62 (88.6) | 15 (83.3) | 22 (88.0) | 0.493 |
Mucinous/SRCC | 32 (11) | 21 (11.9) | 7 (10.0) | 1 (5.6) | 3 (12.0) | |
Other | 7 (2.4) | 4 (2.3) | 1 (1.4) | 2 (11.1) | 0 (0.0) | |
Treatment | ||||||
Yes | 135 (46.6) | 83 (46.9) | 22 (31.4) | 6 (33.3) | 12 (48.0) | 0.158 |
No | 119 (41.0) | 74 (41.8) | 38 (54.3) | 11 (61.1) | 8 (32.0) | |
Unknown | 36 (12.4) | 20 (11.3) | 10 (14.3) | 1 (5.6) | 5 (20.0) |
Characteristic | Cases | RON and PD-L1 (TIMCs) expression in the tumor microenvironment | ||||
RON low/PD-L1 low | RON high/PD-L1 low | RON low/PD-L1 high | RON high/PD-L1 high | P value | ||
Number of cases | 338 | 177 | 70 | 65 | 26 | |
Age (mean ± SD) | 61.24 ± 12.555 | 60.37 ± 12.299 | 62.40 ± 12.518 | 61.03 ± 13.286 | 64.58 ± 12.436 | 0.348 |
Sex | ||||||
Man | 197 (58.3) | 108 (61) | 35 (50.0) | 40 (61.5) | 14 (52.8) | 0.368 |
Women | 141 (41.7) | 68 (39) | 35 (50.0) | 25 (38.5) | 12 (46.2) | |
Principal diagnosis | ||||||
Rectum | 200 (59.2) | 116 (65.5) | 37 (52.9) | 28 (43.1) | 19 (73.1) | 0.004 |
Colon | 138 (40.8) | 61 (34.5) | 33 (47.1) | 37 (56.9) | 7 (26.9) | |
Pathological grade | ||||||
Well/moderate | 8 (2.4) | 3 (1.7) | 2 (2.9) | 3 (4.6) | 0 (0) | 0.492 |
Poor | 306 (90.5) | 158 (89.3) | 66 (94.3) | 58 (89.2) | 24 (92.3) | |
Unknown | 24 (7.1) | 16 (9.0) | 2 (2.9) | 4 (6.2) | 2 (7.7) | |
T stage | ||||||
Tis-T2 | 96 (28.4) | 64 (36.2) | 9 (12.9) | 16 (2.6) | 7 (26.9) | 0.002 |
T3 | 155 (45.9) | 82 (46.3) | 36 (51.4) | 28 (43.1) | 9 (34.6) | |
T4 | 87 (25.7) | 31 (17.5) | 25 (35.7) | 21 (32.3) | 10 (38.5) | |
N stage | ||||||
N0 | 226 (66.9) | 125 (70.6) | 39 (55.7) | 47 (72.3) | 15 (57.7) | 0.075 |
N (1-2) | 112 (33.1) | 52 (29.4) | 31 (44.3) | 18 (27.7) | 11 (42.3) | |
M stage | ||||||
M0 | 326 (96.4) | 173 (97.7) | 68 (97.1) | 61 (93.8) | 24 (92.3) | 0.235 |
M1 | 12 (3.6) | 4 (2.3) | 2 (2.9) | 4 (2.3) | 2 (7.7) | |
Stage | ||||||
0-II | 221 (65.4) | 123 (69.5) | 39 (55.7) | 45 (69.2) | 14 (53.8) | 0.104 |
III-IV | 117 (34.6) | 54 (30.5) | 31 (33.3) | 20 (30.8) | 12 (46.2) | |
Histological type | ||||||
Adenocarcinoma | 287 (84.9) | 152 (85.9) | 62 (88.6) | 60 (92.3) | 13 (50) | < 0.001 |
Mucinous/SRCC | 40 (11.8) | 21 (11.9) | 7 (10.0) | 3 (4.6) | 9 (34.6) | |
Other | 11 (3.3) | 4 (2.3) | 1 (1.4) | 2 (3.1) | 4 (15.4) | |
Treatment | ||||||
Yes | 298 (88.2) | 83 (46.9) | 22 (31.4) | 30 (46.2) | 24 (92.3) | < 0.001 |
No | 32 (9.5) | 74 (41.8) | 38 (54.3) | 25 (38.5) | 1 (3.8) | |
Unknown | 8 (2.4) | 20 (11.3) | 10 (14.3) | 10 (15.4) | 1 (3.8) |
In the GEO cohort, univariate Cox regression analysis showed that age, T stage, M stage, disease stage, RON, and PD-L1 (TCs) expression were significantly correlated with a poor prognosis in CRC patients (P < 0.05). Multivariate analysis after adjustment showed that only age, T stage, and M stage were independent prognostic factors for OS in CRC patients (P < 0.05); disease stage, RON expression, and PD-L1 expression were not significant factors in the multivariate analysis (P > 0.05; Table 4). Kaplan-Meier analysis showed that high expression of RON or PD-L1 (TCs), and both high RON and PD-L1 expression were all associated with a poor OS (P < 0.05; Figure 1A-C). High expression of RON was associated with patient age and treatment type, and high expression of PD-L1 (TCs) was associated with the primary site of the tumor (P < 0.05; Table 1).
Variable | FAHZUSM cohort | GEO cohort | ||||||
Univariate analysis, HR (95%CI) | P value | Multivariate analysis, HR (95%CI) | P value | Univariate analysis, HR (95%CI) | P value | Multivariate analysis, HR (95%CI) | P value | |
Age (mean ± SD) | 1.029 (1.011-1.048) | 0.002 | 1.031 (1.011-1.050) | 0.002 | 1.025 (1.009-1.041) | 0.002 | 1.028 (1.012-1.045) | 0.001 |
Gender | ||||||||
Male | 1.000 | 0.011 | 1.000 | 0.008 | 1.000 | 0.293 | 1.000 | 0.076 |
Female | 0.562 (0.362-0.874) | 0.527 (0.328-0.847) | 0.814 (0.555-1.194) | 0.698 (0.469-1.039) | ||||
Principal diagnosis | ||||||||
Rectum | 1.000 | 0.298 | 1.000 | 0.318 | 1.000 | 0.688 | 1.000 | 0.544 |
Colon | 0.796 (0.518-1.224) | 0.790 (0.497-1.255) | 1.081 (0.738-1.585) | 0.882 (0.589-1.322) | ||||
Histological type | ||||||||
Adenocarcinoma | 1.000 | 0.408 | 1.000 | 0.387 | NA | |||
Mucinous/SRCC | 2.464 (0.343-17.710) | 2.720 (0.263-28.122) | ||||||
Unknown | 3.355 (0.433-25.986) | 1.232 (0.129-11.795) | ||||||
T stage | ||||||||
Tis-T2 | 1.000 | < 0.001 | 1.000 | 0.003 | 1.000 | 0.001 | 1.000 | 0.007 |
T3 | 0.211 (0.108-0.413) | 0.298 (0.141-0.632) | 0.333 (0.145-0.766) | 0.381 (0.159-0.914) | ||||
T4 | 0.503 (0.325-0.781) | 0.596 (0.361-0.897) | 0.455 (0.292-0.709) | 0.476 (0.295-0.769) | ||||
N stage | ||||||||
N0 | 1.000 | < 0.001 | 1.000 | 0.111 | 1.000 | 0.062 | 1.000 | 0.141 |
N (1-2) | 3.156 (2.083-4.783) | 5.376 (0.678-42.660) | 1.435 (0.982-2.097) | 0.306 (0.063-1.479) | ||||
M stage | ||||||||
M0 | 1.000 | < 0.001 | 1.000 | 0.039 | 1.000 | < 0.001 | 1.000 | 0.008 |
M1 | 4.338 (2.094-8.985) | 2.445 (1.048-5.701) | 3.546 (2.013-6.247) | 2.481 (1.269-4.852) | ||||
Stage | ||||||||
0-II | 1.000 | < 0.001 | 1.000 | 0.406 | 1.000 | 0.029 | 1.000 | 0.099 |
III-IV | 3.102 (2.044-4.708) | 0.409 (0.050-3.366) | 1.530 (1.045-2.242) | 3.924 (0.774-19.888) | ||||
Pathological grade | ||||||||
Well/moderate | 1.000 | < 0.001 | 1.000 | 0.003 | NA | |||
Poor | 7.689 (2.434-24.290) | 4.044 (1.103-14.830) | ||||||
Unknown | 1.266 (0.513-3.126) | 0.375 (0.104-1.357) | ||||||
RON (protein) | ||||||||
Low | 1.000 | 0.001 | 1.000 | 0.012 | 1.000 | 0.035 | 1.000 | 0.466 |
High | 2.060 (1.364-3.112) | 1.788 (1.138-2.808) | 1.515 (1.030-2.228) | 1.170 (0.767-1.785) | ||||
RON (mRNA) | ||||||||
Low | NA | 1.000 | 0.035 | 1.000 | 0.466 | |||
High | 1.515 (1.030-2.228) | 1.170 (0.767-1.785) | ||||||
PD-L1 (protein) | ||||||||
Low | 1.000 | < 0.001 | 1.000 | 0.001 | NA | |||
High (TIMCs) | 0.544 (0.293-1.011) | 0.676 (0.350-1.304) | ||||||
High (TCs) | 1.325 (0.669-2.511) | 1.654 (0.819-3.338) | ||||||
PD-L1 (mRNA) | ||||||||
Low | NA | 1.000 | 0.047 | 1.000 | 0.083 | |||
High | 1.835 (1.007-3.345) | 1.719 (0.931-3.173) |
In the FAHZUSM cohort, Kaplan-Meier analysis showed that high expression of RON in TCs, high PD-L1 expression in TCs, or high PD-L1 expression in TIMCs in CRC tissue samples was correlated with a lower OS (P < 0.05) (Figure 4A-C). Univariate Cox regression analysis showed that age, gender, TNM stage, disease stage, pathological grade, RON expression, and PD-L1 expression were associated with a poor OS in patients with CRC (P < 0.05). Multivariate analysis after adjustment showed that age, gender, T stage, M stage, pathological grade, RON expression, and PD-L1 expression remained independent prognostic factors for OS in CRC patients (P < 0.05), while N and disease stage were not significant (P > 0.05; Table 4). We further analyzed the relationship between OS and RON and PD-L1 expression in the tumor microenvironment. High expression of both RON and PD-L1 in TCs predicted a significantly worse OS, and high RON expression in TCs and high PD-L1 expression in TIMCs were associated with a significantly worse prognosis (P < 0.001; Figure 4D and E).
In order to study the relationship between RON and PD-L1 in CRC cells, HT29 cells (following serum starvation) were treated with MSP, BMS-777607, or MSP + BMS-777607 for 24 h. The effects of treatment on RON and PD-L1 expression were analyzed by cellular immunofluorescence. Activating RON phosphorylation promoted PD-L1 expression, while inhibiting RON phosphorylation down-regulated PD-L1 expression (Figure 5A). This result was confirmed by analysis of protein expression by Western blot (P < 0.05; Figure 5B and C). In addition, we found that RON inhibition significantly reduced the phosphorylation of AKT and ERK1/2, which signal downstream of RON (Figure 6A-D).
The application of PD-L1 immunotherapy in cancer treatment is becoming more and more important, but its therapeutic effect has been limited in CRC. This may be due in part to the prevalence of the mismatch repair (MMR) proficient or microsatellite stabilization (MSS) subtypes of CRC[36]. In addition, c-MET plays an important role in regulating PD-L1 expression[37,38]. Therefore, RON may promote the expression of PD-L1 in tumor tissue to affect the efficacy of PD-L1 immunosuppressants.
RON and PD-L1 play important roles in cancer initiation and development and are important targets for tumor therapy. However, few studies have explored the relationship between RON and PD-L1 expression in CRC and the impact that RON and PD-L1 expression patterns may have on pathological characteristics and disease outcomes. It was our hypothesis that activation of the RON receptor tyrosine kinase may promote the expression of PD-L1 in CRC tissue and impair the efficacy of PD-L1 immunotherapy. The purpose of our study was to analyze the expression and clinical significance of RON and PD-L1 in the tumor microenvironment in CRC samples, and to determine whether RON can regulate the expression of PD-L1 in CRC. We discovered that high expression of both RON and PD-L1 in the tumor microenvironment was associated with the poorest OS rate compared to CRC tumors with other RON and PD-L1 expression states. RON and PD-L1 were independent prognostic factors for OS in CRC patients. In addition, we showed that RON phosphorylation led to increased expression of PD-L1 in CRC cells, and that inhibiting RON phosphorylation can reduce PD-L1 expression.
We used publicly available data from the GEO database to investigate the relationship between RON and PD-L1 expression and clinical outcomes in CRC. We used X-tile to determine the optimal cut-off values for RON and PD-L1 levels in the GEO cohort. Kaplan-Meier survival analysis revealed a positive correlation of high RON or PD-L1 expression with worse OS, and high expression of RON and PD-L1 together was associated with the worst OS for CRC patients. However, RON and PD-L1 levels in the GEO dataset were determined by RNA sequencing using RNA extracted from tumor tissue to quantify the expression level in TCs, and it is difficult to determine the interactions between RON and PD-L1 that may arise within the tumor microenvironment from the GEO dataset. Therefore, we used the FAHZUSM cohort, a larger patient cohort with pathological tumor samples, to further study the expression of RON and PD-L1 in CRC tissues and to determine the pathological significance of elevated RON and PD-L1 expression in the tumor microenvironment.
Dysregulation of RON and PD-L1 signal transduction is a key feature of many tumors. Our results and previous studies demonstrated that high expression of RON or PD-L1 in CRC tumor tissues correlated with the extent of primary tumor, lymph node metastasis, and distant metastasis[39,40]. Furthermore, high expression of RON or PD-L1 in the tumor microenvironment was associated with a poor survival in CRC patients[22,39-42].
We demonstrated that high expression of both RON and PD-L1 in TCs was associated with a poor OS in CRC patients. Interestingly, the expression levels of RON were positively correlated with those of PD-L1 in TCs, which has not been previously reported. This may be related to the fact that RON can regulate both the production of and response to IFN-γ[43]. In TCs, long-term continuous activation of IFN-γ can mediate adaptive resistance to PD-L1 tumor immunosuppression; high expression of RON may attenuate resistance, restore the efficacy of PD-L1 targeted therapy, and may even have a promoting effect on the expression of PD-L1 by inhibiting the production of IFN-γ[10,43-45].
MEK/ERK and PI3K/AKT signaling pathways play a central role towards understanding the mechanisms underlying tumorigenesis and tumor development, prevention, and treatment. For example, autophagy caused by the activation of PI3K/AKT pathway plays a significant role in tumors[46,47]. In our study, we demonstrated that RON phosphorylation increased the expression of PD-L1 in CRC cells, proving that RON activation promotes the expression of PD-L1, likely acting through the downstream AKT and ERK1/2 signaling pathways. Previous studies have shown that there is crosstalk between RON phosphorylation and other receptors, which can affect the surface expression of other receptors[22]. Phosphorylation of RON activates downstream oncogenic signaling pathways, such as the RAS-ERK and PI3K-AKT pathways, thereby promoting tumor initiation, growth, invasion, and metastasis[20]. Treatment with BRAF inhibitors or MEK inhibitors, or down-regulation of ERK1/2 can lead to down-regulation of PD-L1 expression in TCs[48]. Thus, RON phosphorylation may promote the expression of PD-L1 in TCs through the RAS-ERK signaling pathway. In addition, PTEN interacts with RTK-dependent signals at multiple levels[48], and has an antagonistic effect on PI3K, which plays an important role in mediating RTK-dependent cell signaling and tumor immune escape[10,48,49]. Therefore, RON phosphorylation may interact with PTEN to activate the PI3K-AKT signaling pathway, thereby promoting PD-L1 expression in TCs.
TIMCs are regarded as an indicator of host immune response to a tumor, and have long been considered an unfavorable prognostic marker in CRC[41,42]. Moreover, RON expression plays an important role in anti-tumor immune responses[27,50]. Previous studies also have shown that RON activation reduced the polarization of inflammatory M1 macrophages and induced the differentiation of immunosuppressive M2 macrophages. M2 macrophages promote PD-L1 expression through autocrine VEGF signaling[51]. In our study, we demonstrated that high expression of both RON and PD-L1 (TIMCs) was associated with a poor OS in patients with CRC. Thus, high expression of RON may impair the anti-tumor immune response by promoting the expression of PD-L1 in TIMCs, leading to tumor growth, invasion, and metastasis.
There were some limitations in this study. First, although we have analyzed a large patient cohort, this was a retrospective analysis and there is the potential for selection bias. Second, we did not evaluate which specific immune cell components in TIMCs expressed PD-L1. Third, although we have preliminarily studied that RON phosphorylation promotes the expression of PD-L1 in CRC cells, the mechanism by which RON promotes PD-L1 expression still needs to be further studied.
In summary, high expression of RON and/or PD-L1 in CRC samples is associated with a poor prognosis in CRC patients. The expression status of RON and PD-L1 may be helpful as biomarkers to evaluate the prognosis of patients with CRC. In addition, RON phosphorylation can promote the expression of PD-L1 in CRC cells, possibly through activation of the AKT and ERK1/2 signaling pathways, which provides a new idea for the immunotherapy of CRC.
Programmed death ligand 1 (PD-L1) protein expression on immune cells enables tumor cells to evade the immune system in a wide variety of malignancies. However, the efficacy of PD-L1 immunosuppressive agents in colorectal cancer (CRC) is poor. The recepteur d’origine nantais (RON) receptor tyrosine kinase plays an important role in regulating tumor immunity.
The poor anti-tumor effect of PD-1 inhibitors in CRC promoted the research on the mechanism of PD-1 expression, so as to improve the therapeutic effect of PD-1 inhibitors on CRC.
The present study aimed to identify patterns of RON and PD-L1 expression and explore the clinical significance of these patterns in CRC.
The gene expression data from the Gene Expression Omnibus database (GEO; n = 290) and patients at the First Affiliated Hospital, Zhejiang University School of Medicine (FAHZUSM; n = 381) were analyzed to determine the prognostic value of RON and PD-L1 expression in the tumor microenvironment of CRC. HT29 cells were treated with BMS-777607 to explore the relationship between RON activity and PD-L1 expression. Signaling pathways and protein expression perturbed by RON inhibition were evaluated by cellular immunofluorescence and Western blot.
In the GEO patient cohort, the cut-off values for RON and PD-L1 expression were determined to be 7.70 and 4.30, respectively. Stratification of patients based on these cutoffs demonstrated that high expression of RON and PD-L1 was associated with a poor prognosis. In the FAHZUSM cohort, rates of high expression of RON in tumor cells, high PD-L1 expression in tumor cells and tumor infiltrating monocytes, and both high RON and high PD-L1 expression in the tumor microenvironment were 121 (32%), 43 (11%), 91 (24%), and 51 (13.4%), respectively. High expression of RON was significantly correlated with high expression of PD-L1 in the tumor cell compartment (P < 0.001). High expression of RON and PD-L1 were independent prognostic factors for poorer overall survival. Concurrent high expression of both RON and PD-L1 in the tumor microenvironment was significantly associated with a poor prognosis. In vitro, BMS-777607 inhibited the phosphorylation of RON and PD-L1 expression, and attenuated the activation of the ERK1/2 and AKT signaling pathways in CRC cells.
RON, PD-L1, and their crosstalk are significant in predicting the prognostic value of CRC. Moreover, phosphorylation of RON upregulates PD-L1 expression, which provides a novel approach to immunotherapy in CRC.
The study of RON and PD-L1 expression will help improve the efficacy of PD-L1 immunosuppressive agents for CRC.
Manuscript source: Invited manuscript
Specialty type: Pathology
Country/Territory of origin: China
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P-Reviewer: Koustas E, Zhu Y S-Editor: Gong ZM L-Editor: Wang TQ P-Editor: Li JH
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