Background
Multiple myeloma (MM) is a common hematologic malignancy characterized by renal insufficiency, osteolytic lesions, anemia and hypercalcemia [
1]. Almost all MM cases were progressed from a premalignant condition called monoclonal gammopathy of undetermined significance (MGUS) [
2]. So far, the pathogenesis of myeloma is not yet clear [
3]. Changes in tumor microenvironment and genetic alterations synergically promote disease occurrence and progression [
4,
5]. The immune cells in the tumor microenvironment, such as T and B cells, play a crucial part in myelomagenesis. As the major suppressors of immune responses, Tregs can regulate the proliferation and function of other immune cells, such as CD4
+ and CD8
+ T cells, natural killer cells, dendritic cells [
6,
7]. Tregs can be further classified into three subpopulations based on their different phenotypes and functions [
8]. The three distinct subpopulations are as follows: (1) CD45RA
+FoxP3
lo resting Treg cells (rTregs) (2) CD45RA
−FoxP3
hi activated Treg cells (aTregs), both of which are suppressive in vitro; (3) non-suppressive CD45RA
−FoxP3
lo T cells (non-Tregs) which can secret immunoregulatory cytokines, such as IL-10, TGF-β and so on.
Several studies have shown that CD4
+ Tregs are increased and functionally immunosuppressive in the peripheral blood of MM patients [
9‐
11]. However, these results were strongly debated due to different gating strategies of Treg, lack of analysis based on Treg cell subsets. Besides, using peripheral blood rather than bone marrow as study subject cannot truly interpret the real size and function of Treg pools in tumor microenvironment since bone marrow is a possible priming site for T cell responses which represents the immediate tumor environment of myeloma [
12,
13]. Therefore, we conducted our study based on precisely Treg subset analysis in both peripheral blood and bone marrow from MGUS to MM patients.
CD28 is the main co-stimulatory molecule of T cells and plays a key role in proliferation, differentiation and activation of T cells with CD3 synergistically [
14]. Prolonged antigen stimulation and T cell senescence may cause the downregulation of CD28, leading to T cell anergy [
15]. Recent studies found that immune abnormalities in MM patients are inseparable from functional failure caused by T cell aging [
16], especially defective expression of CD28 in T cells, which has close relationship with clinical stage, disease progression and prognosis [
17,
18]. CD4
+CD28
−FoxP3
+ Treg-like cell is a novel senescent regulatory T cell subset with impaired suppressive function and early aging features [
19]. In some connective tissue diseases, for example rheumatoid arthritis (RA), CD28
− Treg-like cells revealed an increased number and abnormal cytokine secretion which might contribute to pathogenic immune response. Thus we assumed these aging Treg-like cells might participate in immune dysfunction during myelomagenesis to some extent.
In this study, we performed a comprehensive analysis to investigate the frequencies and function of Treg cell subsets and aging Treg-like cells in both peripheral blood and bone marrow of newly diagnosed MM and MGUS patients, trying to provide new ideas for immunodeficiency of multiple myeloma.
Methods
Patients and healthy donors
In this study, patients were included after signing informed consent form, and the study was approved by Peking Union Medical College Hospital research ethics committee. A total of 20 MGUS and 26 untreated MM patients were recruited for this study. A group of 18 healthy adults (10 males and 8 females) who did not have any systemic disorders was studied in parallel and used as normal controls. Mononuclear cells from additional 8 MM patients and additional 3 volunteers were used for immunosuppressive assays.
Flow cytometry analysis
PB and BM samples were collected and used for analysis within 24 h. Both PB and BM were lysed to remove erythrocytes using BD lysing solution (BD Biosciences, USA) according to manufacturer’s instructions. After lysis of erythrocytes, 1 × 106 cells were labeled with the following fluorochrome conjugated monoclonal antibodies (BD Biosciences, USA): Fluorescein isothiocyanate (FITC) anti-hCD4 (clone RPA-T4), phycoerythrin-cyanin (PE-Cy™7) anti-hCD45RA (clone HI100), APC-Vio770 anti-hCD28 (clone 15E8) and Peridinin Chlorophyll Protein Complex-Cy™5.5 (PerCP-Cy™5.5) anti-hCD25 (clone M-A251), and incubated at 4 °C for 20–30 min.
Then, cells were permeabilized according to eBioscience recommendations (eBioscience, USA). Finally, cells were labeled with anti-hFoxP3 (clone 3G3) conjugated with allophycocyanin (APC) from Miltenyi Biotec (Germany) and incubated at 4 °C for 30–40 min. All prepared samples were measured on BD FACS Canto II. FlowJo software (Version 10.0, TreeStar) was used for analysis of the cytometric data. At least 50,000 events were acquired from each sample.
Definition of activated Treg, resting Treg and non-suppressive T cells
As in the previous study [
8], we defined activated Treg (aTreg) as CD4
+CD45RA
−FoxP3
hi or CD4
+CD45RA
−CD25
++ T cells, resting Treg (rTreg) as CD4
+CD45RA
+ FoxP3
lo or CD4
+CD45RA
+CD25
+ T cells and non- suppressive T cells (non-Treg) as CD4
+CD45RA
−FoxP3
lo or CD4
+CD45RA
−CD25
+ T cells (Additional file
1: Figure S1). Similarly, we defined aging Treg cells as CD4
+CD28
−FoxP3
+ based on previous findings [
19] (Additional file
2: Figure S2).
Isolation of T regulatory cell subsets
9 ml blood samples were collected and used for analysis within 12 h. At first, mononuclear cells were isolated by Ficoll-Hypaque density gradient centrifugation (GE Healthcare company, USA), then resuspended in PBS supplemented with 1% penicillin and streptomycin (Sigma, USA) at a concentration of 1 × 10
6 cells/ml. To isolate Treg cell subsets, purified mononuclear cells were labeled with PE anti-hCD4 (clone RPA-T4), APC anti-hCD25 (clone M-A251) and PE-Cy™7 anti-hCD45RA (clone HI100). Then, these labeled cells were sorted using a BD FACS Aria™ Cell Sorter (BD Bioscience, USA) into four different subpopulations as described previously [
8,
20]: CD4
+CD25
+CD45RA
−, CD4
+CD25
+CD45RA
+, CD4
+CD25
++CD45RA
−, and CD4
+CD25
− fractions sorted as responder cells. Purity of sorted cells was 95% for all samples. The CD25
++ gate was adjusted to contain CD4
+ T cells that express CD25 more brightly than CD4
+CD25
+ cells.
Assessment of T regulatory cells subsets immunomodulatory function
Cell stimulation and suppression assay
RPMI 1640 medium supplemented with 10% fetal bovine serum, 100 IU/ml penicillin and 100 mg/ml streptomycin (Sigma, USA) was used for T cell cultures. For the carboxyfluorescein diacetate succinimidyl ester (CFSE) dilution assay, CD4+CD25− responder T cells were labeled with 1 mmol/ml CFSE (Invitrogen, USA) for 20 min at 37 °C. 1 × 104 CD4+CD25− T cells were co-cultured in the presence or absence of sorted Treg subsets cells (aTregs, rTregs or non-Tregs) for assessing their suppressive capacity at 1:1 ratio. Subsequently, mixed T cell cultures were stimulated with anti-CD3/CD28 coated beads (cell: beads = 1:1) (Dynabeads human T-activator CD3/CD28, Life Technologies, USA) in 96-well plates for 90–96 h. Proliferation of CFSE-labeled cells was analyzed by flow cytometry. Suppression percentage = (number of proliferating CFSE-labeled responder cells when co-cultured with suppressor cells/number of proliferating responder cells when cultured alone) × 100%. FlowJo software (Version 10.0, TreeStar) was used for analysis of the cytometric data.
Cytokine determination
Concentration of IL-10 from the co-culture supernatants of proliferation assays were measured using Human IL-10 ELISApro Kit (Mabtech biotec, Sweden) according to the manufacturer’s instructions.
Statistical analysis
Data were expressed in median and range percentages for Treg cells and their subsets. Non-parametric analyses were used including Mann–Whitney U test and Kruskal–Wallis test to evaluate the difference between two and more independent groups. To evaluate the difference between groups, P value<0.05 was considered as significant.
Discussion
Treg cells play an essential role in maintaining immunological homeostasis and exert major immunosuppressive activity. Elevated FoxP3 expression and Treg cell expansion are generally considered to poor prognosis markers in various cancers, including breast cancer, gastric malignancies, lymphoma and so on [
21,
22]. FoxP3
+ regulatory T cells could be divided into three different subpopulations: activated Treg cells (aTregs), resting Treg cells (rTregs) and non-suppressive Treg cells (non-Tregs) [
8,
23]. rTreg is generated in the thymus and remain a resting state. After being stimulated by various antigens and activation signals in the body, it can be transformed into a terminally differentiated state called aTreg cell which has a stronger immunosuppressive function than rTreg cell [
24]. In addition, Tregs contain a kind of non-Treg cells that have no immunosuppressive effect but can exert immunoregulatory function by secreting proinflammatory cytokines (IL-17, IL-10, TGF-β, etc.) [
25].
Our study found that, no matter in PB or BM, the frequency of aTregs increased in newly diagnosed MM and MGUS patients, which indicated severe immunosuppressive state. However, changes of rTreg cells in peripheral blood and bone marrow of patients with MM or MGUS were not consistent. In MGUS and MM cohort, the proportion of rTreg cells in peripheral blood gradually decreased, which corresponded to the increasing proportion of aTreg cells. It may be explained that rTregs were transformed into aTregs by tumor antigen stimulation [
26]. While in BM, the extent of rTreg decline in MGUS and newly diagnosed MM patients was more pronounced than in peripheral blood, suggesting bone marrow is more sensitive to reflect disease severity and progression. It’s worth mentioning that the proportion of aTreg cells in MGUS patients was significantly higher than that in control. Similarly, in the bone marrow of patients with MGUS, we also found that the proportion of rTreg cells was significantly lower than that of healthy people, indicating that there were already immunologic abnormalities in patients with precancerous lesions of myeloma. These results, from a side, support Dhodapkar’s view that patients in MGUS phase have experienced changes in the tumor microenvironment, including immune cells, osteoclasts, and stromal cells [
27]. However, due to the short duration of our projects and limited samples, it was difficult to further analyze MM and MGUS patient based on risk stratification and disease severity.
For functional study, we found the inhibition rate of aTregs and rTregs on effective T cells was slightly higher than that of healthy controls, indicating the immune suppressive ability of Treg subsets in NDMM patients was basically normal. In addition, our results showed that the ability of Treg cell subsets to secrete IL-10 in untreated myeloma patients was not different from that of healthy controls. These results were partially consistent with previous studies [
10,
28] that immunosuppressive function of CD4
+CD25
hiFoxP3
+ cells in MM patients was intact compared with healthy controls.
In our study, we noticed that the proportion of CD28− aging Treg-like cells in PB and BM from MGUS and MM patients was significantly higher than that of healthy controls, and gradually increased with disease progression. This also corresponds to our result of Treg subsets, suggesting that patient’s immunologic state is deteriorating during progression from MGUS to MM. The significant difference between MGUS patients and healthy controls revealed that in the early stage of myelomagenesis, phenotypic abnormalities of immune cells have appeared in the body of patients, leading to cellular senescence and functional failure.
Authors’ contributions
Conceived and designed experiments: WJN, CH, LJ. Performed experiments and analyzed data: WJN, WX. Collected and interpreted patient data: WJN, CXX, ZAL. Contributed reagents/materials/analysis tools: CH, WX. Wrote the paper: WJN, LJ. All authors read and approved the final manuscript.