Early myeloid-derived suppressor cells (HLA-DR−/lowCD33+CD16−) expanded by granulocyte colony-stimulating factor prevent acute graft-versus-host disease (GVHD) in humanized mouse and might contribute to lower GVHD in patients post allo-HSCT

Introduction Myeloid-derived suppressor cells (MDSCs) are proposed to control graft-versus-host disease (GVHD) in allogeneic hematopoietic stem cell transplantation (allo-HSCT). However, the definition of human MDSCs has not yet reached consensus, and the mechanism of MDSCs to control GVHD remains unclear. Methods Immature myeloid cells (HLA-DR−/lowCD33+CD16−) were tested before and after granulocyte colony-stimulating factor (G-CSF) administration in healthy donor and isolated for suppression assays and co-culture with T cells in vitro. Isolated cells were infused in humanized mice for a xenogeneic model of acute GVHD. One hundred allo-HSCT recipients were enrolled prospectively to assess the role of HLA-DR−/lowCD33+CD16− cells in grafts on the occurrence of acute GVHD. Results In the present study, G-CSF mobilized HLA-DR−/lowCD33+CD16− cells with immunosuppressive properties in donor peripheral blood. These cells contained more interleukin-10+ and transforming growth factor-beta (TGF-β)+ cells after G-CSF administration and inhibited the proliferation of autologous donor T cells in a TGF-β-dependent manner. Meanwhile, these immature myeloid cells promoted regulatory T cell expansion and induced Th2 differentiation. Importantly, these cells prevented acute GVHD in a humanized mouse model. Moreover, clinical cohort results showed that the number of HLA-DR−/lowCD33+CD16− cells in the donor graft was the only independent risk factor inversely correlated with the incidence of grade II–IV acute GVHD in the recipients (HR 0.388, 95% CI 0.158–0.954, p = 0.039). Conclusion HLA-DR−/lowCD33+CD16− cells represent functional MDSCs that may control acute GVHD in allo-HSCT. Electronic supplementary material The online version of this article (10.1186/s13045-019-0710-0) contains supplementary material, which is available to authorized users.


Introduction
Allogeneic hematopoietic stem cell transplantation (allo-HSCT) is an effective treatment for patients with most hematological diseases [1]. However, the applications of allo-HSCT are limited by lethal complications, including graft-versus-host disease (GVHD). The increased understanding of the regulatory cells and molecular pathways involved in limiting pathogenic immune responses offers the opportunity for promoting GVHD-relapse-free survival (GRFS), aiming to replace non-specific GVHD control with pharmacological immune suppression [2][3][4][5].
Extensive research has shown that myeloid-derived suppressor cells (MDSCs) have emerged as major immunosuppressive cells in cancer, infection, chronic inflammation, and autoimmune disease, which suggest that MDSCs may help to control GVHD [6,7]. However, the phenotypic, morphological, and functional heterogeneity of MDSCs generates confusion in the investigation and analysis of their roles in immune responses as MDSCs represent a heterogeneous population of immature myeloid cells and are defined by their ability to suppress T cells in vitro [8,9]. In humans, MDSCs most commonly express the common myeloid marker, CD33 [10], but lack the expression of markers of mature myeloid and lymphoid cells as well as the MHC class-II molecule, HLA-DR [11,12]. Lin − (including CD3, CD19, and CD56) CD14-CD15-HLA-DR − CD33 + cells contain mixed groups of MDSCs comprising more immature progenitors (also named early MDSCs, eMDSCs). Furthermore, two other subpopulations with more differentiated surface makers, namely, CD15+ or CD14+, are divided into two groups as follows: G-MDSCs (PMN-MDSCs) and M-MDSCs [8]. However, the definitions of these subsets have not yet reached consensus, and it remains unclear if MDSCs control GVHD in vivo.
Though granulocyte colony-stimulating factor (G-CSF) has been routinely used to mobilize stem cells to the peripheral blood from healthy donors, it is also recognized as a novel mediator of T cell tolerance [13,14]. Increasing evidences suggest that G-CSF affects different immune cells [13,15], which modulate T cell response directly by inducing Th2 differentiation [16,17] or mobilizing functional regulatory T cells [18], or indirectly through monocytes [19][20][21], DC [22], and neutrophils [23] to prevent GVHD. Previous results have suggested that G-CSF-mobilized donor cells also contain MDSCs, which are closely associated with GVHD in allo-HSCT [24]. Antonio et al. reported that systemic treatment with G-CSF induces expansion of myeloid cells displaying the phenotype of M-MDSCs (Lin low/neg HLA-DR − CD11b + CD33 + CD14 + ), which is the only graft parameter to predict acute GVHD (aGVHD) [25]. Lv showed that monocytic MDSCs (Lin − HLA-DR −/low CD33 + CD11b + CD14 + CD1 5 dim CD16 − ) and promyelocytic MDSCs (Lin − H-LA-DR −/low CD33 + CD11b −/low CD14 − CD15 − CD16 − ) in the graft are correlated with the incidence of cGVHD without significant influence on relapse and survival [26]. Fan demonstrated that higher frequency of Lin low/neg HLA-DR − CD33 + CD11b + MDSCs in the G-CSF-primed bone marrow (G-BM) than in the G-CSF peripheral blood stem cell (G-PBSC) harvest grafts leads to a better GRFS and less GVHD [27]. In contrast, the frequency of CD14 + HLA-DR low/ neg M-MDSCs is significantly increased in the peripheral blood after allo-HSCT, especially in patients with acute graft-versus-host disease [28]. Though clinical relevance between MDSCs and GVHD has been observed in humans, there is no data available to identify if human MDSCs prevent GVHD in vivo and there was limited data about the eMDSCs in allo-HSCT. In addition, as positive CD16 represents the relatively mature marker of myeloid cells, whether negative CD16 could better define MDSCs remains to be explored [26,29].
Based on a humanized mouse model and a prospective cohort study, the present study demonstrated that HLA-DR −/low CD33 + CD16 − cells expanded by G-CSF represent subsets of more immature progenitors and immune regulatory properties in donor PBSC have the immunosuppressive potential of eMDSCs, which suppress aGVHD in the allo-HSCT settings.

Materials and methods
Experimental model NOD-SCID-IL-2Rg−/− mice (NSG mice) were purchased from Vitalstar. All mice were bred and housed in a specific pathogen-free facility in microisolator cages and used at 8 to 12 weeks of age in protocols approved by the local Ethical Committee. Each experimental group included six to eight mice, and the experiment is repeated twice.

Donor PB and BM samples
This study was approved by the Ethics Committee of Peking University People's Hospital, Beijing, in accordance with the Declaration of Helsinki. Healthy donors were enrolled from the related donors of patients who had undergone either haplo-identical or HLA-matched allogeneic blood and marrow transplantation at the Peking University People's Hospital between April 2017 and May 2018. Peripheral blood and BM samples (10 ml in EDTA tube) from recombinant human G-CSF (rhG-CSF)-non-treated or recombinant human G-CSF-treated (filgrastim, 5 μg/ kg/day, five consecutive days) healthy allogeneic donors (randomly selected at Peking University People's Hospital in Beijing) were collected after informed consent was obtained.
Human HLA-DR −/low CD33 + CD16 − isolation HLA-DR −/low CD33 + CD16 − cells were isolated from GPBSC using fluorescence-activated cell sorting (FACS)-sorted (FACS Aria II, BD Biosciences) with antibodies of HLA-DR, CD33, and CD16 (eBioscience or BD Bioscience) according to the manufacturer's instructions, which included one step of positive selection for CD33 + cells and two steps of negative selection for HLA-DR − and CD16 − cells.

Morphology
HLA-DR −/low CD33 + CD16 − morphology was studied on cytospins after May-Grünwald-Giemsa staining. Photographs were taken using × 1000 magnification with a smart V350Df digital camera mounted on an OLYMPUS CX31 microscope.

T cell proliferation and suppression assays
T cells from GPBSC were purified by positive selection using CD3 cell isolation via flow cytometry. Purified CD3 + T lymphocytes were labeled with 5 μM 5,6-carboxy-fluorescein diacetate succinimidyl ester (CFSE) (eBioscience) and thereafter were co-cultured with isolated HLA-DR −/ low CD33 + CD16 − at a HLA-DR −/low CD33 + CD16 − to CD3 + T cell ratio of 0.25:1 to 2:1 in the presence of anti-CD3/ CD28 beads (Thermo) in RPMI 1640 (Biological Industries) supplemented with 10% FBS, penicillin/streptomycin, and 2 mM L-glutamine. 10 5 T cells were seeded in 96-well U-bottom plates. After 4 days, cells were harvested for flow cytometry analysis. To neutralize IL-10 and TGF-β, blocking antibodies were used at 10 to 20 μg/ml concentrations (blocking antibody for IL-10 and TGF-β from R&D Systems). To inhibit arginase activity, nor-NOHA (Calbiochem) was used at a concentration of 300 μM. For the inhibition of iNOS, L-NMMA (Sigma) was used at a concentration of 300 μM. To inhibit IDO, indoximod (NLG8189) (Selleck) was used at a concentration of 500 μM. To inhibit Cox2, NS398 (Selleck) was used at a concentration of 10 μM. All the in vitro experiment was repeated at least three times.
Xenogeneic model of graft-versus-host disease NSG mice were sublethally irradiated using 180-cGy total body irradiation by X-ray on day − 1, followed by the intravenous infusion in the caudal vein of 5 × 10 6 GPBSC and different dose of HLA-DR −/low CD33 + CD16 − on day 0. Control groups were transplanted with GPBSC alone. Engraftment of human white blood cell was detected from peripheral blood samples of mice at 7 days, 14 days, and 21 days after transplantation. Engraftment of human eMDSC was detected in the peripheral blood, spleen, and bone marrow of humanized mice at 14 days and 21 days after transplantation. Human Treg (CD4 + CD25 + Foxp3 + ), Th1 (CD4 + T-bet + ), Th2 (CD4 + GATA3 + ), Th17 (CD4 + RORγt + ), and the cytokine levels were detected from peripheral blood samples of mice at 21 days after transplantation. Levels of cytokines were assessed with pre-designed sets of Luminex immunoassays from eBioscience (for all cytokines measured in supernatants [Human ProcartaPlex Panel #EPX180-12165-901] according to the recommended protocols, using Magpix detection platform (Luminex Corp., Austin, TX) and xPonent software (Luminex). Mice were monitored for survival, weight, and acute GVHD score three times a week. The clinical scoring system was based on six parameters: weight loss, posture, activity, fur texture, skin integrity, and diarrhea. A severity scale of 0 to 1 was used for each parameter, with a maximum score of 6. Mice that had died or had been sacrificed at 1.5 months after HSCT and the tissues were kept in 4% paraformaldehyde. Tissues from GVHD target organs (liver, intestine, and skin) were embedded in paraffin, sectioned, and stained with hematoxylin, eosin, and Safran. Photographs were taken using × 200 or × 400 magnifications with Basler Microscopy ace 2.3 MP Mono camera mounted on an OLYM-PUS BX43 microscope.

Survival analysis of allo-HSCT recipients
The risk stratification for recipients of hematological malignancies is followed by Disease Risk Index (DRI) [35]. The survival functions were estimated by the Kaplan-Meier method using the log-rank test with asymmetric 95% confidence intervals, and the cumulative incidences of aGVHD or cGvHD and TRM/Relapse were calculated using competing risks with 95% confidence intervals. Diagnosis of GVHD was also evaluated with classic and the National Institutes of Health (NIH) consensus criteria [36,37]. Univariate probabilities of survival were calculated using a left-truncated approach. A bivariable analysis was applied to check with two-way interactions between variables (Spearman correlation for non-normally distributed values; Pearson correlation for normally distributed values). All variables included in the multivariable analysis were tested with time-dependent covariates and constructed in a proportional hazards (Cox) model if PH ≥ 0.05 or a Cox w/Time-Dep Cov model if PH < 0.05, which included patient age, sex, donor-patient sex mismatch, graft components, etc. Variables included in the multivariate analysis were selected by backward elimination process with a criterion of p < 0.10 for retention.
Subsequently, the inhibition of CD3 + T cell proliferation by HLA-DR −/low CD33 + CD16 − cells was markedly reduced in the presence of an anti-TGF-β antibody but not an anti-IL-10 antibody, indicating that the immunosuppressive activity relied more on the presence of TGF-β (Fig. 2c, d).

modulate Th cell balance and induce Treg generation
The present study demonstrated that CD4 + CD25 + Foxp3 + Treg cells increased in the HLA-DR −/ low CD33 + CD16 − cell co-culture group (Fig. 3a, c). Th cell subsets were analyzed after co-culture with or without HLA-DR −/low CD33 + CD16 − cells. Though the expression of IFN-γ and IL-17A increased, co-culture with HLA-DR −/low CD33 + CD16 − cells led to a significantly higher ratio of Th2/Th1 and Th2/Th1+Th17 cells than the control group (Fig. 3b, d, e).
HLA-DR −/low CD33 + CD16 − MDSCs prevent aGVHD in humanized mouse model Because G-CSF expanded HLA-DR −/low CD33 + CD16 − cells into the peripheral blood and exerted a strong regulatory effect on T cell immune response, we next investigated if such population prevents aGVHD in vivo. To mimic aGVHD after allo-HSCT in humans, a humanized xenogeneic aGVHD model was established by injection of 5 × 10 6 donor G-PBSC into irradiated non-obese diabetic (NOD)-severe combined immune deficient (SCID)-IL-2Rg−/− mice (NSG mice) [38,39] (Fig. 4a). Human white blood cell engraftment was detected by CD45 + cells at 7, 14, and 21 days after transplantation, and there was no significant difference of human cells engraftment intragroup (14 days, p = 0.486; 21 days, p = 0.4012) (Additional file 1: Figure S4). We failed to detect the engraftment of HLA-DR −/ low CD33 + CD16 − MDSCs in PB as these cells could be detected in the spleen and bone marrow at 14 days after transplantation; however, they decreased quickly and almost could not be detected at 21 days after co-transplantation (Additional file 1: Figure S5). Acute GVHD occurred in the humanized mice receiving donor G-PBSC during 2 to 4 weeks after transplantation as evidenced by weight loss, disease score (hunching, activity, ruffling, and diarrhea), and death. Similar to humans [40,41], humanized mice with aGVHD showed severe inflammation, leukocyte infiltration, necrosis, and tissue damage in target organs, such as the skin, liver, and gut in the G-PBSC group (Fig. 4e). On the base of this model, a prevention model was established by one-time co-infusion of 2.5 × 10 6 , 1 × 10 6 , and 5 × 10 5 human G-CSF-mobilized HLA-DR −/low CD33 + CD16 − cells sorted from the same donor with graft at the same day. All of these cell doses reduced weight loss (Fig. 4b), improved overall survival (Fig. 4c), improved pathological score (Fig. 4d), and lessened tissue damage in target organs in medium and high doses of HLA-DR −/low CD33 + CD16 − cells compared to mice grafted without or with low-dose human HLA-DR −/low CD33 + CD16 − cells (Fig. 4e). For human Treg detected at 21 days after transplantation, a significant difference was found between the high-dose HLA-DR −/low CD33 + CD16 − cells and GPBSC control (p = 0.0498); there was no disparity between medium dose vs. control (p = 0.6825) and low dose vs. control (p > 0.9) (Fig. 4a, Additional file 1: Figure S6); there were no disparity of Th2/(Th1+Th17) ratio between the different groups (Fig. 4b, Additional file 1: Figure S6). For cytokines detected at 7, 14, and 21 days after transplantation, there were significantly less INF-γ and IL-6 at days 7, 14, and 21 and   2 The percentage of IL-10 + and TGF-β + cells increased in HLA-DR −/low CD33 + CD16 − cells in GPBSC and HLA-DR −/low CD33 + CD16 − cells suppressed T cell proliferation in a TGF-β-dependent manner. a, b IL-10 and TGF-β were analyzed by cytometry in HPB and GPBSC from eight healthy donors. IL-10 + and TGF-β + cells were gated on HLA-DR −/low CD33 + CD16 − cells. c HLA-DR −/low CD33 + CD16 − cells sorted from GPBSC and co-cultured with autologous CD3 + T cells, with or without anti-IL-10 antibody or anti-TGF-β antibody in culture system in the presence of anti-CD3/CD28 beads. The ratio of HLA-DR −/low CD33 + CD16 − to CD3 + T cells was 1:1. Co-cultured for 4 days, T cell proliferation was evaluated using CFSE labeling. Unstimulated T cells were used as a negative control. Stimulated T cells were used as a positive control. d The percentage of T cell suppression was shown in a different group. Data were compared using Student's unpaired t test (ns, not significant; *p ≤ 0.05). d Percentages of T cell suppression in different groups. Data were compared using Student's unpaired t test (ns, not significant; *p ≤ 0.05) ratios were higher at days 7 and 14, while IL-4/IL-17A ratio was higher at day 21 (Fig. 5c, d). These results confirmed that immune-suppressive activity of HLA-DR −/ low CD33 + CD16 − cells which might contribute to alleviating aGVHD in NSG model.

Negative correlations between the frequency of HLA-DR −/low CD33 + CD16 − cells among donor PBSCs and the development of aGVHD in recipients
In a prospective study (registered at www.chictr.org as ChiCTR-OCH-10000940), 100 allo-HSCT recipients were enrolled to assess the role of HLA-DR −/low CD33 + CD16 − in graft on the occurrence of aGVHD. Of these patients, 76 patients received a combination of G-BM and G-PBSC grafts from haplo-donors, and 24 patients received grafts from MSDs. The indications for allo-HSCT were as follows: AML (n = 39), ALL (n = 29), MDS (n = 8), SAA (n = 14), and lymphoma (n = 10). Ninety-nine (99%) patients reached full donor chimerism before day 30 after transplantation as assessed by the analysis of a variable number of tandem repeats on the peripheral blood. Platelet recovery (count > 20,000/ml) was achieved at a median of day 32 post-transplantation, whereas neutrophils reached values greater than 500/ml on day 12. Only 1 patient died due to transplant-related mortality at day 11 post-HSCT. The median follow-up period of the enrolled patients was 11 months. The cell components in the graft were listed in Additional file 1: Table S1. Patients were divided into 2 groups according to the median absolute counts of HLA-DR −/low CD33 + CD16 − MDSCs in grafts (1.88 × 10 7 / Fig. 3 HLA-DR −/low CD33 + CD16 − cells could affect the balance of Th subsets induce Treg generation. a Treg (CD4 + CD25 + Foxp3 + ) generation was detected through flow cytometry. CD3 + T cells were co-cultured with or without HLA-DR −/low CD33 + CD16 − cells for 4 days. b The percentage of Treg in CD4 + T cell, group HLA-DR −/low CD33 + CD16 − vs. control, p = 0.0048. c Flow cytometry analysis of Th1 (CD4 + IFN-γ + ), Th2 (CD4 + IL-4 + ), Th17 (CD4 + IL-17a + ). CD3 + T cells were co-cultured with or without HLA-DR −/low CD33 + CD16 − cells sorted from GPBSC in the presence of CD3/CD28 for 4 days. Red for CD4+ cell fraction and blue for CD4-negative part. d Th2/Th1 ratio fold change compared with the control group, p = 0.0159. e Th2/(Th1+Th17) ratio fold change compared with the control group, p = 0.0095 kg) as follows: 53 patients were in the high MDSCs group (≥ 1.88 × 10 7 /kg), and 47 patients were in the low MDSCs group ( Table 2).
The cumulative incidences for different grades of aGVHD at 100 days after transplantation for the total cohort were as follows: 50% of patients developed grade I-IV aGVHD; 28% of patients developed grade I aGVHD (61.8% for haplo-HSCT and 12.5% for MSD-HSCT); 17% of patients had grade II aGVHD (25% for haplo-HSCT and 12.5% for MSD-HSCT); and 5% of patients developed grade III-IV aGVHD (5.3% for haplo-HSCT and 4.2% for MSD-HSCT). Patients who received a high number of MDSCs exhibited lower incidence of grade II-IV aGVHD compared to the low MDSC groups in allo-HSCT (11.3% vs. 31.9%, p = 0.0287) and comparable of grade III-IV aGVHD in allo-HSCT (1.9% vs. 8.5%, p = 0.127) (Fig. 6a, b). In the bivariable analysis, high MDSC dose and CD34 + cells in the graft were interacted; for consideration of collinearity in multiple variable analysis (MVA), backward elimination process was applied to choose one factor (high MDSC dose) which was taken into the final MVA model. In the multivariate analysis, absolute counts of MDSCs in allografts emerged as the only Fig. 4 HLA-DR −/low CD33 + CD16 − cells could inhibit the development of aGVHD in humanized mouse model. a Protocol for the establishment of aGVHD model through injecting human GPBSC. Sublethally irradiated NSG mice received 5 × 10 6 human GPBSC with or without 2.5 × 10 6 , 1 × 10 6 , and 5 × 10 5 G-CSF-mobilized HLA-DR −/low CD33 + CD16 − sorted from GPBSC. b Weight Loss, c median survival, and d pathological score in xenografted mice were shown. Mice co-transplanted with HLA-DR −/low CD33 + CD16 − (pink, green, and blue, eight mice each group) had improved survival after transplant as compared with GPBSC-injected group (red). For survival, weight change, and disease score: GPBSC + high dose versus GPBSC, GPBSC + medium dose versus GPBSC, and GPBSC + low dose versus GPBSC, p < 0.05. e Representative histology of the target organs harvested on day 22 after transplantation. All results were derived from two pooled independent experiments. Each experiment was performed with G-PBSC from one donor for all recipients. Results were presented and compared with Kaplan-Meier survival curves independent factor that reduced the occurrence of grades II-IV (HR 0.388, 95% CI 0.158-0.954, p = 0.039). Age, patient gender, HLA disparity, ABO disparity, patient-donor relationship, and CD3/CD4/ CD8/CD14/CD34 cells in grafts were not correlated to grades II-IV in the analysis.
For patients with leukemia-free survival (LFS) above 100 days post-transplantation, the estimated 1-year cumulative incidences for chronic GVHD (cGVHD) of the total cohort were as follows: 25.5% patients developed cGVHD, 8.2% patients with extensive cGVHD, and 15.3% patients with moderate to severe cGvHD with NIH criteria. There were trends that patients who received a high number of MDSCs exhibited a lower incidence of cGVHD (17.6% vs. 36.9%, p = 0.067) and NIH moderate to severe cGvHD (10.3% vs. 24.5%, p = 0.045) (Fig. 6c, d). In the univariate analysis, high-vs. low-dose MDSCs are identified as a potential factor that reduced the occurrence of cGVHD (HR 0.481, 95% CI 0.213-1.089, p = 0.072). In the multivariate analysis, no independent risk factor was found.

Discussion
The present study characterized a previously unidentified immature monocytic cell population defined by the cell surface expression of HLA-DR −/low CD33 + CD16 − in healthy donors after G-CSF treatment. These cells represented an eMDSC population. Compared with the same b Th2/(Th2+Th17) ratios between intragroup. c IL-4/INF-γ ratios between intragroup. d IL-4/IL-17A ratios between intragroup. *p < 0.05; **p < 0.01 compartment in non-mobilized PB, the percentage of IL-10 + cells and TGF-β + cells significantly increased, suggesting that G-CSF not only expanded these cells but also endowed them immunosuppressive properties and regulatory function dependent on TGF-β. Importantly, these cells prevented aGVHD in a humanized mouse model. Moreover, the prospective cohort suggested that these eMDSCs in the donor graft inversely correlated with the incidence and severity of aGVHD in recipients. These cells may be a potential treatment for immunomodulatory prevention and therapy for aGVHD in allo-HSCT (Fig. 7).
MDSCs represent a heterogenic population of immature myeloid cells, and the definition of these subsets has not yet reached consensus [42][43][44]. Currently, most MDSC phenotypes have been reported to be generated in the tumor state [29,45]. There are fewer reports about the generation and function of MDSCs in regions other than tumors and chronic inflammation. GM-CSF is considered as a major growth factor driving myelopoiesis [46,47]. In combination with IL-6, IL-1β, prostaglandin (PG) E2, TNF-α, or VEGF, GM-CSF has been reported to mediate the generation of highly suppressive MDSCs from CD33 + peripheral blood mononuclear cells isolated from healthy donors [48]. Importantly, GM-CSF and IL-6 allow a rapid and efficient generation of MDSCs with strong tolerogenic activity from the precursors present in mouse and human bone marrow [49]. Solito demonstrated that the GM-CSF, G-CSF, and IL-6 cytokines allow a rapid generation of MDSCs from precursors present in human BM in vitro and that the CD11b low/− /CD16 − -immature subset is the only subset responsible for immune suppression in BM-MDSCs [29]. As G-CSF is more widely applied in an allo-HSCT demonstrated that G-CSF-expanded myeloid cells display the phenotype of M-MDSCs and suppress alloreactive T cells [25]. However, these MDSCs have not been tested in an in vivo model. In contrast, the present study demonstrated that HLA-DR −/low CD33 + CD16 − eMDSCs Fig. 6 Association of HLA-DR −/low CD33 + CD16 − cells and clinical outcomes. The cumulative incidences of aGvHD for patients were calculated according to competitive risk. Gray's test was used in the cumulative incidence analyses. The "low" and "high" groups were separated according to the median of HLA-DR −/low CD33 + CD16 − MDSC absolute numbers in the graft (< vs. ≥ 1.88 × 10 7 /kg). a II-IV aGvHD in total allo-HSCT cohort (n = 100). b III-IV aGVHD in allo-HSCT cohort. c cGvHD in allo-HSCT cohort. d NIH moderate to severe cGvHD in allo-HSCT cohort. e LFS in hematological malignancies. f OS in allo-HSCT cohort. g CIR in hematological malignancies. h TRM in allo-HSCT cohort prevented acute GVHD in a humanized mouse model in vivo. As G-CSF treatment alone is significantly associated with the generation of HLA-DR −/ low CD33 + CD16 − eMDSCs in both frequency and absolute number compared to only increasing number in total MDSCs (Lin − HLA-DR −/low CD11b + CD33 + ), M-MDSCs (HLA-DR -low CD11b + CD33 + CD14 + CD15 − ), and G-MDSCs (HLA-DR −/low CD11b + CD33 + CD14 − CD15 + ), we speculated that G-CSF-expanded HLA-DR −/low CD33 + CD16 − eMDSCs accumulated in G-PBSC may play an important role in the G-CSF-induced immune tolerance in allo-HSCT.
Immune-suppressive activity contributes to the definition of MDSCs; though the activity of HLA-DR −/ low CD33 + CD16 − eMDSCs was lower compared with M/ G-MDSCs, it suggested the underlining mechanism of the immunosuppressive effects of HLA-DR −/low CD33 + CD16 − eMDSCs on T cells in vitro might be distinct from M/ G-MDSCs [24,25]. Mougiakakos suggested that indoleamine 2,3-dioxygenase (IDO) plays a critical role in the immunosuppressive effects of CD14 + HLA-DR low/neg M-MDSCs [28]. In contrast, the present study showed that the inhibition of CD3 + T cell proliferation by HLA-DR −/low CD33 + CD16 − eMDSCs was abolished in the presence of an anti-TGF-β antibody rather than an anti-IL-10 antibody. This result should be interpreted carefully as there were 10% IL-10 + while 60% TGF-β + HLA-DR −/low CD33 + CD16 − cells in G-PBSC. These results implied that the immunosuppressive activity of HLA-DR −/low CD33 + CD16 − eMDSCs might depend more on TGF-β, which may further strengthen this new set of eMDSCs compared to traditional MDSCs. Acute GVHD is mediated by donor-derived T cells and activation with alloantigens expressed on host tissues. Donor-derived naive CD4 + T cells differentiate into Th cell subsets of effector T cells, such as Th1 and Th17, expressing distinct sets of transcriptional factors and cytokines, which mediate organ-specific GVHD. Previous studies have demonstrated that Th2 cells alleviate aGVHD in mouse models [50,51]. While playing key roles in suppressing autoimmunity and maintaining immune homeostasis, Treg reduce the severity of GVHD. The effects of Treg on inhibiting aGVHD have been reported in several previous studies [52][53][54]. The present study suggested that the Treg induction and polarization of T cells from Th1/Th17 to Th2 should be primarily regulated by the HLA-DR −/low CD33 + CD16 − eMDSCs. Although, the inverse ratio of Th2/(Th1+Th17) might be interpreted with caution as there was an increase in all cytokines measured including IFN-γ and IL-17 in vitro; there were significantly less INF-γ, IL-17A, IL-6, and Fig. 7 Summary of study. Early myeloid-derived suppressor cells (HLA-DR −/low CD33 + CD16 − ) expanded by granulocyte colony-stimulating factor derived from G-CSF-mobilized donor PBSCs. This MDSC population suppressed T cell proliferation in vitro and in humanized mouse model, potentially by TGF-β-dependent manner, and promoted Treg generation, which also prevents acute graft-versus-host disease (GVHD) in humanized mouse and might contribute to lower GVHD in patients post-allo-HSCT TNF-α at days 14 and 21 in NSG mice after infusion of high-dose HLA-DR −/low CD33 + CD16 − eMDSCs, with increased IL-4/INF-γ and IL-4/IL-17 ratio. In the present study, HLA-DR −/low CD33 + CD16 − eMDSCs were demonstrated to prevent aGVHD by evaluating weight loss, overall survival, pathological score, and less tissue damage of the gut and liver; it should be noticed that the lung and bone marrow are also the main target organs of GVHD in NSG model and might be evaluated in the future [55]. In summary, it is anticipated that donor-derived HLA-DR −/low CD33 + CD16 − eMDSCs may prevent aGVHD via TGF-β activity, inducing Treg generation, and possibly by modulating Th cell balance.
In addition, several studies have reported that MDSCs modulate the function of alloreactive T cells and prevent GVHD without impairing the graft-versus-leukemia (GVL) effects in murine models [15,56]. In our prospective cohort study, high dose of HLA-DR −/ low CD33 + CD16 − eMDSCs was identified as independent risk factor for II-IV aGVHD, while it is also associated with lower risk of NIH moderate to severe cGVHD while did not affect CIR and LFS. As the high MDSC group also had significantly more CD34 + cells in the graft, though backward elimination process had been applied to reduce collinearity, high CD34 + cells might promote platelet engraftment and lymphocyte recovery after allo-HSCT and have mixed influence on the association of MDSCs with clinical outcome. In addition, as the median follow-up is still relatively short, it is also important to further understand if the donor-derived cells in the present study can prevent cGVHD without impairing the GVL effects in the future.
In conclusion, the present study identified and confirmed a population of previously unreported immature myeloid regulatory cells derived from G-CSF-mobilized donor PBSCs. This MDSC-like population suppressed T cell proliferation in a TGF-β-dependent manner, modulated the T helper cell balance from Th1 to Th2, and promoted Treg generation. These effects are beneficial for establishing immune tolerance in HSCT and may prevent aGVHD. Therefore, the mechanisms underlying the prevention of aGVHD in recipients and the immunomodulatory function of these donor-derived cells need to be studied in the future. Such work might improve the transplantation outcomes with allo-HSCT and facilitate the potential use of these cells in the clinic.