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Expression of CD40 is a positive prognostic factor of diffuse large B-cell lymphoma treated with R-CHOP (rituximab, cyclophosphamide, doxorubicin, vincristine, and prednisone)

Authors Song G, Ni H, Zou L, Wang S, Tian F, Liu H, Cho W 

Received 23 September 2015

Accepted for publication 5 February 2016

Published 23 June 2016 Volume 2016:9 Pages 3799—3805

DOI https://doi.org/10.2147/OTT.S96992

Checked for plagiarism Yes

Review by Single anonymous peer review

Peer reviewer comments 2

Editor who approved publication: Professor Min Li



Guoqi Song,1 Huiyun Ni,1 Linqing Zou,2 Shukui Wang,3 Fuliang Tian,4 Hong Liu,1 William C Cho5

1Department of Hematology, Affiliated Hospital of Nantong University, Nantong, 2Department of Human Anatomy, Nantong University, Nantong, 3Central Laboratory of Nanjing First Hospital, Nanjing Medical University, Nanjing, 4Maternal and Child Health Hospital of Lianyungang, Lianyungang, Jiangsu, People’s Republic of China; 5Department of Clinical Oncology, Queen Elizabeth Hospital, Kowloon, Hong Kong

Objectives: The objective of this study was to investigate the expression level of CD40 and its role in the prognosis of patients with diffuse large B-cell lymphoma (DLBCL) who were treated with rituximab-CHOP (rituximab, cyclophosphamide, doxorubicin, vincristine, and prednisone).
Design and methods: The immunohistochemical expressions of CD40 in 186 well-characterized DLBCL patients were evaluated by tissue microarrays, thereby revealing the relationship of the molecule CD40 with known tumor, patient-related variables, and survival rates.
Results: The results showed that CD40 expressions were not statistically different between the germinal center B-cell-like (GCB) type and the non-GCB type. We also analyzed the relationships of CD40 expression with overall survival (OS) and progression-free survival (PFS) in DLBCL patients who were uniformly treated with R-CHOP. A low expression of CD40 compared to high expression is related to poor OS and PFS.
Conclusion: Our findings indicate that the CD40 level at onset acts as an independent prognostic predictor of DLBCL patients treated with R-CHOP.

Keywords: CD40, diffuse large B-cell lymphoma, R-CHOP, prognostic factor

Introduction

Diffuse large B-cell lymphoma (DLBCL) is one of the most common histological subtypes of non-Hodgkin’s lymphoma, characterized by heterogeneity in its clinical, immunophenotypic, and genetic features.1 The discovery of rituximab and its correct application in combination with cyclophosphamide, doxorubicin, vincristine, and prednisone (CHOP) (standard first-line treatment) have significantly improved clinical outcome in DLBCL patients and have made the disease a curable malignant tumor. However, still a number of patients with DLBCL undergo relapse or show no response to the standard first-line therapy.2,3 Prediction of outcome is important to avoid overtreatment and also to identify others who might benefit from intensive therapy. As the most important prognostic factor for survival – International Prognostic Index (IPI) – has gained wide acceptance, it is considered to be the strongest indicator to identify high-risk patients and also as a guidance for individual treatment.4

The IPI, based on clinical features (eg, age, stage, and level of lactate dehydrogenase), neither reflects the molecular heterogeneity of DLBCL nor predicts responsiveness to therapy. The IPI score is no longer considered to be the strongest prognostic indicator in rituximab (R)-CHOP-treated patients, and a recent analysis revealed that it failed to recognize a subgroup with long-term survival rate of less than 50%.5,6 Biomarkers seem to contribute to perfect risk-stratification in DLBCL and to identify high-risk subgroups benefiting from intensified or novel therapies.7,8 Therefore, there arises an urgent need for biomarkers as new standard prognostic indicators not only for patients with DLBCL but also for patients with other tumors.

Several biological markers have been studied in order to recognize high-risk patients, who show an early relapse or poor response to standard treatment, but none has been proved to be completely effective, and more independent factors have still to be identified and confirmed. Proposed scoring systems are too sophisticated for daily use or their predictive value is inferior to IPI. CD40 is a 43kD membrane glycoprotein and a member of the tumor necrosis factor (TNF) receptor family, and it is expressed in certain cells, including B lymphocytes and antigen-presenting cells such as dendritic cells and monocytes. As we all know, CD40 is a growth signal receptor for B lymphocytes.9 Recent studies have shown that CD40 is expressed in DLBCL, and the higher its expression level, the better the prognosis of patients.1012

In the present study, we used immunohistochemistry (IHC) to examine 186 paraffin-embedded tumor tissues from patients with DLBCLs treated with R-CHOP and correlated CD40 expression with patients’ clinicopathological features and clinical outcomes.

Materials and methods

Patients

Pretreatment biopsies of 186 consented patients with DLBCL admitted to the Nanjing First Hospital and Affiliated Hospital of Nantong University from 2005 to 2010 were studied, the patients met the following criteria: 1) confirmed diagnosis of DLBCL (diagnosis of de novo DLBCL in human immunodeficiency virus (HIV)-negative patients; primary mediastinal B-cell lymphoma, cutaneous LBCL, intravascular LBCL, and involvement of central nervous system at the time of diagnosis were excluded) following a pathologic review; 2) treatment with R-CHOP (rituximab, cyclophosphamide, adriamycin, vincristine, and prednisone); 3) diagnostic paraffin material detected by tissue microarray (TMA); and 4) tested negative for HIV l. All the cases were histologically reviewed by two senior pathologists according to the World Health Organization classification of tumors of hematopoietic and lymphoid tissues to confirm the diagnosis. For germinal center B-cell-like (GCB) type, CD10+, BCL-2-, centerine+, and MUM1 are immunologically stained. For non-GCB type, CD10-, BCL-2+, centerine-, and MUM1+ are immunologically stained. Complete response (CR), partial response (PR), stable disease, and progressive disease were defined according to International Working Group recommendations.13 Clinical follow-up data were obtained from the patients’ medical records. The study was approved by the Institutional Review Boards of Nantong University (People’s Republic of China) and Nanjing Medical University (People’s Republic of China). The study was conducted in accordance with the Declaration of Helsinki. Written informed consent was obtained from each participant or from the patient representatives.

Tissue microarray

Tumor samples were arrayed as described previously.14,15 Slides of 5 μm tissue sections were stained with hematoxylin–eosin stain and used to identify and mark out a representative viable tumor tissue. Using a 0.6 mm needle, core biopsies from the areas of corresponding paraffin-embedded blocks were placed at defined coordinates in the recipient paraffin array blocks using a manual arrayer (Beecher Instruments, Sun Prairie, WI, USA). The array blocks were constructed at a density of 80–150 cores per array. A single core was evaluated from each case. The analysis of single TMA core typically shows more than 90% concordance with the conventional whole section analysis of tumor markers and it has been validated previously.16

Immunohistochemistry

Consecutive tissue sections (4 μm thickness) from the TMAs were cut into adhesive-coated slides and deparaffinized with serial xylene, ethanol gradient, and distilled water. Heat-induced antigen retrieval was performed in a pressure cooker containing 1 mM ethylene diamine tetraacetic acid (pH 8.0) or 10 mM citrate (pH 6.0) at 120°C for 3 minutes. Endogenous peroxidase was blocked using 10% hydrogen peroxide solution at room temperature for 5 minutes. The sections were then rinsed in phosphate buffered saline (PBS) for 5 minutes and incubated at 4°C overnight with monoclonal antibodies against CD40 (Santa Cruz Biotechnology, Inc., Dallas, TX, USA). After washing with PBS, two to three drops of secondary antibody were added, and the sections were incubated at room temperature for 30 minutes. Finally, the sections were counterstained with Mayer’s hematoxylin and then mounted. Additional sections, running in parallel but without addition of the primary antibody in the first incubation, served as negative controls.

IHC staining was evaluated independently by two experienced pathologists, who were blinded to the clinical data. One hundred cells were evaluated in each tumor core, and the percentage of positive cells was calculated. The scores of the three tumor cores were finally averaged for each patient. A case was considered positive if 10% or more of the cells were stained with an antibody. Digital microscopy images were captured using an Olympus BX51 microscope (Olympus, Tokyo, Japan), imported into Image Pro Plus Version 4.5 (Media Cybernetics Inc., Bethesda, MD, USA), and processed digitally for adjustments of contrast, brightness, and color balance. The integrated optical density (IOD) of all the positive staining in each field and area of interest (AOI) were measured. The IOD was used to evaluate the area and intensity of the positive staining. The mean density (IOD/AOI) represented the concentration of specific protein per unit area. Using the median staining mean density of CD40 by IHC as the staining threshold, we separated patients into low-expression group with values <89.27 and high-expression group with values ≥89.27.

Statistical analysis

Statistical analyses were performed with SPSS software version 11.0. Mann–Whitney U-test (two-tailed) was performed to compare two groups, and one-way analysis of variance (ANOVA) and Pearson correlation were performed to determine the significance of differences in multiple comparisons. Overall survival (OS) and progression-free survival (PFS) time distributions were calculated by the Kaplan–Meier method and analyzed by log-rank test. PFS was defined as the interval between the date of initial diagnosis and the date of disease progression or death from lymphoma or treatment toxicity. OS was calculated as the time from diagnosis to the date of death or last contact. Differences were considered statistically significant if P-values were less than 0.05.

Results

Clinical characteristics of the series

A summary of the clinical characteristics of the entire series of patients is given in Table 1. Complete clinical and histopathologic data were available for all 186 patients. All patients received six to eight (median 6.8) cycles of standard R-CHOP regimen. The overall response rate (CR+PR) was 86.7% (CR was 67.7%), while disease was stable in 7.9% and progressed in 5.4% patients. The median follow-up time for all patients was 50.4 months. The median follow-up time for patients alive at the follow-up was 46 (6–92) months. The estimated 3-year OS was 70.5% and the estimated PFS was 61.3%.

Table 1 Summary of clinical characteristics of 186 patients with diffuse large B-cell lymphoma

Correlation between CD40 expression and clinicopathological parameters

About 131 patients (70.4%) showed IHC-positive CD40. Based on Muris algorithm, 68 patients (36.5%) were classified as GCB subtype and 63 patients (33.9%) as non-GCB subtype. About 55 patients (29.6%) showed IHC-negative CD40. Twenty nine patients out of 55 (15.6%) were classified as GCB subtype and 26 patients (14%) as non-GCB subtype. There were no statistically significant differences in DLBCL subclassification between moderate positivity (Figure 1A) and high positivity groups (Figure 1B) (P>0.05). The CD40 expression was observed to correlate with age, sex, stage, lactate dehydrogenase level, and IPI score, but no statistical significances were obtained (Table 2) (P>0.05).

Figure 1 CD40 immunohistochemistry in tissues of DLBCL patients.
Notes: (A) Low and (B) high CD40 expression in a case of DLBCL ×200 magnification.
Abbreviation: DLBCL, diffuse large B-cell lymphoma.

Table 2 Association between CD40 expression (IOD/AOI) and different clinicopathological features of diffuse large B-cell lymphoma
Notes: Data are presented as Mean ± SD. Results are in response to a one way analysis of variance (ANOVA). P-values were considered significant at <0.05.
Abbreviations: IOD, integrated optical density; AOI, area of interest; SD, standard deviation, IPI, International Prognostic Index.

Effect of CD40 expression on therapeutic response

Given the expression level of CD40 has an important prediction value for therapeutic response (R-CHOP), we found among 186 documented cases, CD40 was expressed in high expression group in 85 complete remissions (67.5%) and in low expression group only in 41 cases (32.5%) (P<0.05). In patients with complete remission (n=126), CD40 was expressed in 49.4% of the tumor cells on average (95% confidence interval [CI], 35–89), whereas in patients without complete remission, CD40 was expressed in 18.7% of tumor cells (95% CI, 5–42; P<0.05). CD40 expression was the highest in patients with CR and higher in patients with PR compared to patients with no response (P<0.05) (Figure 2). All factors associated with failure to achieve complete remission in the univariate models were involved in multivariate analysis, which showed that CD40 expression in <35% of tumor cells (P=0.018), B symptoms (P=0.022), and high IPI (P=0.009) were the independent predictive factors for treatment resistance.

Figure 2 Mean expression of CD40 using immunohistochemistry in tumors CR, PR, NR, and control.
Notes: *P<0.05. The black lines connecting different bars represent the comparison made between the two. Comparisons were made between CR with PR and CR vs NR, PR vs NR. P-values were considered significant at <0.05.
Abbreviations: CR, complete response; PR, partial response; NR, no response; IOD, integrated optical density; AOI, area of interest.

Correlation of CD40 expression with PFS and OS

The relationships between the percentage of CD40 expression and survival rates for 186 DLBCL patients (an average of 4.1 years of follow-up) were also examined. Figure 3 shows the Kaplan–Meier survival curves of the patients grouped by the percentage of CD40-expressing cells in their tumors. The cumulative survival rate of the patients with high expression of CD40 was significantly higher compared with patients with low expression of CD40 (P<0.05). Patients with high expression of CD40 lived longer compared with patients with low expression of CD40.

Figure 3 Overall survival (A) and progression-free survival (B) curves of patients according to CD40 protein expression level.
Note: P<0.05.

Discussion

The chimeric monoclonal antibody – rituximab – chooses CD20 antigen as its target in B cells. Therefore, in the treatment of DLBCL, it is an extremely important drug. Young and elderly patients benefited from the combination of CHOP and rituximab, and their clinical outcome significantly improved.17,18 However, there are still a considerable number of patients who show no response to rituximab-based therapy or who relapse early, and the outcome of these patients to second-line or salvage therapies is not satisfactory. The IPI remains the most successful clinical prognostic instrument for DLBCL. However, the IPI score is no longer considered as a strong prognostic indicator for R-CHOP-treated patients, and a recent analysis revealed that it failed to recognize subgroups with a long-term survival rate lower than 50%.5,6 Biomarkers seem to contribute to perfect risk stratification in DLBCL and to identify high-risk subgroups of patients benefiting from intensified or novel therapies.2 Currently there is no a reliable system that could effectively identify such patients prospectively, which needs to identify a more effective prognostic evaluation system for patients treated with R-CHOP.

CD40 is a member of the tumor necrosis factor receptor family and is expressed on non-immune cells and on tumor cells–mostly in B-cell malignancies – as well as on several immune cells including normal B cells.19 It has been demonstrated that agonistic CD40 antibodies may mediate antitumor activity through the activation of CD40-positive antigen-presenting cells, including dendritic cells.20,21 A recent report showed that in the help of CD40-independent natural killer (NK) cells, the immunity against endogenous B-cell lymphoma by dendritic cell vaccine-induced T-cell was enhanced. Hömberg et al22 showed that exogenous dendritic cells can trigger endogenous NK cells, resulting in the generation of interferon-γ and initiating a cascade that eventually leads to cytotoxic T-lymphocyte responses. This pathway depends on a preceding maturation step to obviate CD4(+) T-cell help and CD40 signaling.22 A Phase I study of the agonistic IgG1 chimeric anti-CD40 antibody ChiLob7/4 in patients with CD40-expressing solid tumors and DLBCL was conducted. The authors found that ChiLob7/4 can activate B and NK cells at doses that can be administered safely, and ChiLob7/4 should be tested in combination with other antibodies and chemotherapy agents.23 In addition, another Phase I and Phase II study of dacetuzumab was conducted in patients with refractory or recurrent B-cell Non-Hodgkin’s lymphoma (NHL), including DLBCL.24,25 CD40L/CD154 mainly expressed on activated helper T cells is the ligand of CD40 and interacts with it. This interaction leads to the B cells guided by their differentiation program – a process that mainly takes place within the germinal centers.26,27 CD40 signal has been shown to be associated with B-cell proliferation, growth, and differentiation; however, several recent studies have shown that it plays an important role in a diverse array of biological processes. CD40 engagement may be associated with weakening the ability of survival and malignancy in tumor cells. It can promote apoptosis and stimulate angiogenesis and transcription/secretion of matrix metalloproteinase.28,29 In addition, it has been reported that CD40 upregulates the expression of ICAM-1,30 a cell-adhesion molecule important for cell–cell interactions. These programs are closely related to the migration and invasion of tumor cells. However, how the expressions of CD40 affect the malignant cells of DLBCL are not well established. Some studies have found that the expression of CD40 defined by IHC in DLBCL results in a favorable prognosis.10,11,29

Therefore, we analyzed the expression of CD40 in specimens of DLBCL. In our study, all the 186 patients with DLBCL were treated with R-CHOP and the expression of CD40 was found to be higher in patients with CR compared to patients with PR, and in patients with PR compared to patients with no response. Therefore, high CD40 expression can predict DLBCL patients’ response to R-CHOP regime. The preliminary results demonstrate that the long-term survival rate including 3-year OS and 3-year PFS in patients with high CD40 expression was superior compared with patients with low expression. The expression level of CD40 positively correlates with the prognosis of DLBCL patients. So if we formulate more adequate regimen based on CD40 expression, the long-term survival rate can be improved in DLBCL patients with different risk factors. In order to minimize the inherent biases of the study, we selected only patients with de novo DLBCL treated with standard first-line chemotherapy and excluded other presentations of DLBCL such as HIV-positive, primary mediastinal, central nervous system, intravascular and testicular lymphomas, transformed NHL, and cutaneous LBCL.31

Conclusion

In conclusion, this study demonstrates that in routine pathologic specimens, CD40 expression can be detected by IHC. Low levels of CD40 expression indicate a poor prognosis, since R-CHOP produces limited benefits. These results have shown that we can effectively identify DLBCL patients with poor clinical outcome, which guides us to adopt more intensive treatment for those patients. Our finding was based on the analysis of a small cohort of DLBCL patients and is a retrospective study. Patients with DLBCL should be classified based on the effective prognostic factors such as CD40 and treatment including upfront hematopoietic stem cell transplantation should be aggressively administered to patients with an unfavorable prediction. To further advance the detection of CD40 expression for clinical application, larger-scale, prospective studies on DLBCL patients are required.

Disclosure

The authors declare no conflicts of interest in this work.


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