Low-dose IL-2 therapy limits the reduction in absolute numbers of circulating regulatory T cells in rheumatoid arthritis.

BACKGROUND: Circulating regulatory T cells (Tregs) are responsible for mediating immune tolerance and maintaining immunological homeostasis. Decreases in Tregs may be involved in the onset of rheumatoid arthritis (RA). Low-dose interleukin-2 (IL-2) has been considered for the treatment of inflammatory diseases mediated by T cells. This study focused on the status of circulating CD4+T subsets and the clinical feasibility of IL-2 therapies in patients with RA.
METHODS: The subjects included 888 patients with RA and 100 healthy controls (HCs); 233 RA patients received IL-2 treatment with 0.5 million international units (MIU)/day from days 1 through 5. The demographic features, disease activity, and levels of CD4+T cells measured by modified flow cytometry were collected in all RA patients before and after treatment.
RESULTS: RA patients had lower absolute Treg counts (but not Th17) compared with HCs, which was associated with disease activity; previously treated RA patients had the fewest circulating Tregs (p < 0.05). Patients treated with low-dose IL-2 had a three-fold increase in absolute anti-inflammatory Treg counts, as well as a two-fold increase in the other CD4+T subsets. Moreover, post-treatment levels of markers of disease activity in RA patients treated with IL-2 were significantly lower than the baseline values (p < 0.001), with no apparent side effects.
CONCLUSION: Decreased absolute counts of circulating CD4+T lymphocyte subsets were observed in patients with RA. Circulating Tregs, which mediate immune tolerance, may be involved in the pathogenesis and progression of RA; however, this was ameliorated by low-dose IL-2, without obvious side effects. PLAIN LANGUAGE
SUMMARY: Low-dose IL-2 treatment for rheumatoid arthritis • Circulating Tregs may be involved in the pathogenesis and progression of RA.• The absolute count of Tregs was significantly correlated with disease activity measures.• Low-dose IL-2 was able to effectively expade Tregs and help for RA patients' symptoms remission without evaluated side effects.

Introduction

Rheumatoid arthritis (RA) is a common chronic and progressive autoimmune inflammatory rheumatic disease of multiple synovial joints, ultimately driven by aberrant immune responses.[1] Without adequate treatment, chronic inflammation can lead to joint damage, severe disability, and even a higher risk of mortality.[2] Disease-modifying antirheumatic drugs (DMARDs), including conventional synthetic DMARDs such as methotrexate, biologic DMARDs such as IL-6R antibodies and JAK inhibitors, and targeted synthetic DMARDs, may improve physical function and inhibit the progression of joint damage by blocking the overwhelming production of pro-inflammatory cytokines that hinder the return to immunological homeostasis.[3,4] Changes in immune-cell function and/or number are mainly responsible for the progressive destruction caused by RA, a T-cell-dependent disease, and promotion of synovial joint articular cartilage degradation and subchondral bone erosion.[5] However, there is no consensus on the levels and function of T cell populations in peripheral blood (PB). Therefore, this should be the priority of research efforts to elucidate the pathogenesis of RA and assess the efficacy of novel therapies.

Several recent studies have focused on the role of impaired immune regulation, resulting mainly from T cells with a regulatory phenotype, in the pathophysiology of RA.[3] Immunoregulation mediated by regulatory T cells (Tregs) derived from CD4+CD25+T cells, with high expression of fork head box protein 3 (FoxP3), is one of the most crucial mechanisms to maintain self-tolerance and immune system homeostasis, and may prevent the production of autoantibodies such as anti-cyclic citrullinated peptide antibodies (anti-CCPs).[6,7] Autoimmune responses can be adjusted by re-establishing the T cell balance in favor of Tregs, as shown in animal models of rheumatic disease.[8] Impaired self-tolerance caused by deficiencies in the function and/or number of Tregs may be an important therapeutic target for RA, and is being investigated extensively in several autoimmune/inflammatory disorders, such as systemic lupus erythematosus, psoriasis, ankylosing spondylitis, and Behçet’s disease.[8,9] However, most previous studies focused on the proportion of Tregs, which can be affected by levels of CD4+T cells and their subsets (such as Th1, Th2, and Th17 cells), rather than the absolute counts, and did not include large amounts of clinical data.[10]

Interleukin-2 (IL-2), a soluble T-cell growth factor produced mainly by antigen-activated T cells, has a unique ability to control the proliferation and differentiation of T cells by binding to three different high-affinity receptor subunits, including an IL-2 receptor α chain (CD25 or IL-2Rα), an IL-2 receptor β chain (CD122 or IL-2Rβ), and a γ subunit (CD132 or γc), on target cell membranes in vitro.[11,12] Systemic fatal autoimmune diseases can develop when T cell regulation by IL-2 is deficient.[13] Indeed, the role of IL-2 (as an immunomodulatory cytokine) in the function and differentiation of CD4+T lymphocyte subsets, especially Tregs with high expression of IL-2Rα, has been the focus of extensive studies on immune-mediated diseases in vitro or in vivo.[9,14] Our previous studies found the efficacy and safety of low-dose IL-2 targeted regulation of Tregs levels in patients with psoriatic arthritis (PsA),[15] dermatomyositis/polymyositis (DM/PM),[16] and primary Sjögren’s syndrome (pSS).[17] However, evidence of the clinical efficacy and safety of IL-2 combined treatment in patients with RA is still lacking.

In this retrospective study, we measured the absolute counts of CD4+T subsets using modified flow cytometry in patients with RA and healthy controls (HCs), to elucidate the immune mechanism of RA. All RA patients received DMARDs with or without low-dose IL-2 treatment, to further clarify the clinical feasibility of IL-2 treatment for RA.

Methods

Participants

The participants included 888 patients with RA, seen at the Second Hospital of Shanxi Medical University between January 2016 and September 2018 and who met the 1987 and 2010 RA classification criteria,[18,19] and 100 HCs. The study was approved by the hospital’s Ethics Committee (ethics number: 2016-KY-007). Exclusion criteria included the presence of other autoimmune diseases such as SLE; history of chronic infection and malignancy; severe active infection (such as tuberculosis, hepatitis viruses, HIV or Epstein-Barr virus); severe hepatic and renal dysfunction; pregnant or lactating females.

Treatment

In total, 233 RA patients with informed consent received additional IL-2 treatment with 0.5 million international units (MIU)/day from days 1–5, combined with conventional immunosuppressants treatments (Supplemental Table S1).

Data collection

The demographic and clinical data of the RA patients were recorded before and after treatment, including disease activity, such as the tender joint count (TJC), swollen joint count (SJC), and Disease Activity Score-28 (DAS28); and general laboratory indicators, such as the erythrocyte sedimentation rate (ESR), complete blood count, and liver and kidney function tests.

The absolute counts and proportions of CD4+T subsets, including helper T (Th)1 (CD4+IFN-γ+), Th2 (CD4+IL-4+), Th17 (CD4+IL-17+), and Tregs (CD4+CD25+FOXP3+) (Supplemental Figure S1), were measured by modified flow cytometry in HCs and all RA patients before treatment,[15,17] and only those patients receiving low-dose IL-2 underwent re-evaluation of CD4+ T cell subsets levels within 2 days of treatment completion.

The absolute number of CD4+T subsets has been difficult to assess since most flow cytometers do not directly provide cell concentration or absolute cell counts in a sample, so percentages are probably the most commonly used technique for detecting cell changes. In this study, we used a modified flow-cytometry-based protocol to calculate the absolute number of CD4+ T subsets in fresh peripheral blood using an equation, which is that the absolute number of CD4+ T subsets = the percentage of each CD4+ T subset* the absolute number of total CD4+ T cells. Cells in 80 μl heparin-anticoagulated venous blood were stimulated by 10 μl PMA, 10 μl Ionomycin (final concentration was 750 ng/ml) and 1 μl GolgiStop respectively in 37°C incubator for 5 h before flow cytometry staining.

Statistical analysis

Categorical data are expressed as frequencies and were analyzed using the chi-squared test. Non-normally distributed data are expressed as the median (range) and were analyzed using the Mann–Whitney U test or Kruskal–Wallis H test. Normally or near-normally distributed data are described as mean ± standard deviation (SD) and were analyzed using the independent samples t test or ANOVA test. The paired samples t test was used to analyze changes in disease activity and laboratory indices after IL-2 treatment in RA patients. The correlations between the absolute counts of Tregs and disease activity parameters were analyzed using Pearson’s correlation. The correlations of autoantibodies with markers of disease activity and Tregs were analyzed using Spearman’s correlation. SPSS 22.0 software (IBM Corp., Armonk, NY, USA) was used for the statistical analyses. A two-tailed p-value <0.05 was considered statistically significant.

Results

Baseline characteristics of all subjects

A total of 888 RA patients (618 females and 270 males) with a mean age of 55.8 ± 13.0 years, and 100 HCs (65 females and 35 males) with a mean age of 54.4 ± 8.0 years were enrolled. The RA patients included 188 new patients (129 females and 59 males, without any immunosuppressants or steroids) with a mean age of 54.4 ± 14.0 years, and 700 patients already treated with immunosuppressants or corticosteroid (489 females and 211 males) with a mean age of 56.2 ± 12.7 years. There was no statistically significant difference in gender or age among the groups (p > 0.05) (Table 1). In total, 233 patients with RA received the IL-2 treatment (0.5 MIU/day for 5 days) and their absolute counts and proportions of peripheral CD4+T subgroups were measured.

Table 1.

Baseline characteristics of all subjects (mean ± SD).

n	Healthy controls	RA	t	P
	100	888
Age (years)	54.4 ± 8.0	55.8 ± 13.0	1.600	0.112
Gender (female/male)	65/35	618/270	0.889	0.346
CD4+T (cells/μl)	701.91 ± 219.73	673.07 ± 295.95	1.196	0.234
Th1 (cells/μl)	124.70 ± 80.77	88.68 ± 77.23	4.401	< 0.001
Th2 (cells/μl)	8.89 ± 5.45	9.58 ± 6.52	1.012	0.312
Th17 (cells/μl)	7.22 ± 4.04	7.17 ± 6.01	0.103	0.918
Treg (cells/μl)	35.20 ± 12.98	27.98 ± 16.71	4.182	< 0.001
CD4+T%	39.01 ± 7.06	41.77 ± 9.65	3.548	0.001
Th1%	17.96 ± 9.97	13.65 ± 10.02	4.080	<0.001
Th2%	1.32 ± 0.79	1.56 ± 1.06	2.210	0.027
Th17%	1.06 ± 0.57	1.18 ± 1.07	1.758	0.080
Treg%	5.12 ± 1.46	4.38 ± 2.01	4.581	<0.001
Th1/Th2	19.97 ± 25.10	11.34 ± 10.31	3.407	0.001
Th17/Treg	0.23 ± 0.15	0.35 ± 0.47	5.485	<0.001

RA, rheumatoid arthritis; SD, standard deviation; Th, helper T cells; Treg, regulatory T cells.

Differences in CD4+T subset levels between RA patients and healthy controls

The absolute number of peripheral CD4+T cells was not significantly altered in overall, previously treated, and new RA patients, compared with healthy individuals, while levels of CD4+T cells were lower in previously treated RA patients than in new RA patients. Both new and previously treated RA patients had decreased absolute counts of Tregs, but not Th17 or Th2 cells, compared with HCs (p < 0.001); the fewest Tregs were in PB from patients already treated with immunosuppressive therapies (p < 0.05). The counts of circulating Th1 cells were also lower in RA patients overall, and in the previously treated RA patients, compared with the HCs, but there was no significant difference between the new RA patients and HCs. Compared with HCs, RA patients (both new and previously treated) had a lower proportion of Treg cells but no difference in that of Th17; thus, the Th17/Treg ratio was significantly higher in RA patients (p < 0.05) (Table 1, Figure 1). The proportions of Th1 and Th2 decreased and increased, respectively (Supplemental Figure S2) and, as a result, the ratio of Th1/Th2 decreased, in overall and previously treated RA patients, compared with healthy controls (p < 0.05) (Table 1, Figure 1, Supplemental Figure S2). New RA patients had a higher level of Th1 cells than previously treated RA patients (p < 0.05) (Supplemental Figure S2). Peripheral Tregs were the only CD4+T subset that showed a significant decrease in absolute counts in both previously treated and new RA patients compared with HCs, which suggested that Tregs may be involved in the onset of RA (Figure 1).

Figure 1.

Changes in the absolute counts of peripheral CD4+T subsets among new (n = 188) and previously treated (n = 700) patients with RA and healthy controls (n = 100). (a) The absolute count of CD4+T cells was significantly decreased in previously treated patients with RA compared with new RA patients. (b) The absolute count of Th1 cells from previously treated patients with RA was significantly lower than that of healthy individuals and new RA patients. New RA patients had a similar level of Th1 cells as healthy controls. (c, d) There were no significant differences in the absolute counts of Th2 or Th17 cells between RA patients and healthy controls. (e) RA patients, both new and previously treated, had decreased absolute counts of Tregs compared with healthy controls; the fewest circulating Tregs were from previously treated RA patients. (f, g) The Th1/Th2 ratio was significantly lower, and the Th17/Treg ratio significantly higher, in patients with RA. Previously treated patients had the lowest Th1/Th2 ratio. *p < 0.05, **p < 0.01, ***p < 0.001. Significance values are asymptotic (two-sided tests) and the significance level is p < 0.05.

RA, rheumatoid arthritis; Tregs, regulatory T cells.

Changes in CD4+T subset levels in RA patients varying in disease activity level

Based on DAS28-ESR, all patients with RA were divided into remission (DAS28 ⩽ 2.6, n = 47), low activity (2.6 < DAS28 ⩽ 3.2, n = 56), moderate activity (3.2 < DAS28 ⩽ 5.1, n = 361), and high activity groups (5.1 < DAS28, n = 424) (Table 2). The clinical remission rate of RA was only 5%, whereas nearly half of all RA patients had high disease activity. As the condition of the RA patients deteriorated, a gradual decline in the absolute counts of CD4+T subsets, especially Tregs, was observed, although the proportions of those subsets and the Th17/Treg and Th1/Th2 ratios did not change significantly (Table 2, Supplemental Figure S3). The fewest Tregs, Th17, Th1, and Th2 cells were seen in the PB of patients with high disease activity (p < 0.05) (Table 2). The absolute count of Tregs was significantly correlated with the disease duration (p < 0.05) and markers of disease activity (p < 0.001), including ESR, C-reactive protein (CRP), TJC, SJC, and DAS28 (Figure 2).

Table 2.

Differences in absolute counts of CD4+T subgroups among patients with different disease activity levels (mean ± SD).

	Healthy controls	RA - remission	RA - low	RA - moderate	RA - high
		DAS28<2.6	2.6⩽DAS28<3.2	3.2⩽DAS28<5.1	DAS28⩾5.1
n	100	47	56	361	424
Gender (female/male)	65/35	30/17	34/22	245/116	309/115
Age (years)	54.39 ± 8.00	51.64 ± 12.62	52.86 ± 13.26	54.94 ± 13.54	57.48 ± 12.38[abcd]
CD4+T (cells/μl)	701.91 ± 219.73	786.27 ± 305.18	747.58 ± 325.06	712.33 ± 287.29	617.26 ± 288.02[abcd]
Th1 (cells/μl)	124.70 ± 80.77	111.64 ± 100.63	100.07 ± 99.01	99.28 ± 81.15[a]	75.61 ± 64.69[abd]
Th2 (cells/μl)	8.89 ± 5.45	12.35 ± 7.62[a]	10.90 ± 6.87	9.91 ± 6.33[b]	8.82 ± 6.39[bcd]
Th17 (cells/μl)	7.22 ± 4.04	9.03 ± 7.01	7.63 ± 5.92	7.68 ± 6.30	6.47 ± 5.56[bd]
Treg (cells/μl)	35.20 ± 12.98	31.03 ± 15.22	30.86 ± 19.55	29.57 ± 16.59[a]	25.91 ± 16.36[abd]
Th1/Th2	19.97 ± 25.10	12.71 ± 14.01	11.43 ± 11.14[a]	11.90 ± 10.73[a]	10.69 ± 9.30[a]
Th17/Treg	0.23 ± 0.15	0.46 ± 0.76[a]	0.33 ± 0.32[a]	0.33 ± 0.42[a]	0.35 ± 0.48[a]

p < 0.05: a versus healthy; b versus remission; c versus low; d versus moderate.

RA, rheumatoid arthritis; SD, standard deviation; Th, helper T cells; Treg, regulatory T cells.

Figure 2.

Correlation between the absolute count of circulating Tregs and disease activity. (a–e) The absolute count of Tregs in peripheral blood was negatively correlated with markers of disease activity, including TJC, SJC, ESR, CRP, and DAS28, in patients with RA. Significance values are asymptotic (2-sided tests) and the significance level is p < 0.05.

CRP, C-reactive protein; DAS28, disease activity score-28; ESR, erythrocyte sedimentation rate; SJC, swollen joint counts; RA, rheumatoid arthritis; TJC, tender joint counts; Treg, regulatory T cells.

Changes in antibody levels in RA patients varying in disease activity levels

Levels of autoantibodies, such as rheumatoid factor (RF), anti-CCP, and anti-mutated citrullinated vimentin antibody (anti-MCV), were recorded in 774 patients with RA. The levels of RF and anti-MCV were lower in RA patients in remission than in patients with active RA, whereas the anti-CCP level was not significantly different among RA patients with different disease activity levels (Supplemental Figure S4). The level of RF was significantly correlated with indicators of disease activity, such as DAS28, ESR, and CRP, while anti-MCV was significantly correlated only with DAS28 and ESR. In addition, only RF was significantly correlated with the absolute count of peripheral Tregs (Supplemental Figure S5).

Changes in disease activity parameters and general biochemical indicators in RA patients with low-dose IL-2 treatment

After low-dose IL-2 treatment, indicators of disease activity, including ESR, CRP, TJC, SJC, and DAS28, decreased significantly compared with baseline values (p < 0.001) (Table 3). Compared with baseline values, white blood cell (WBC), neutrophilic granulocyte, and lymphocyte counts increased significantly (p < 0.001), platelet (PLT) counts decreased (p < 0.001), and red blood cell (RBC) counts did not change (p > 0.05) in the PB of RA patients with IL-2 treatment; however, the levels of these indicators fell within the normal range. Liver function, assessed by aspartate aminotransferase (AST), alanine aminotransferase (ALT), and γ-glutamine transferase (GGT) concentrations, was not affected; AST was lower than baseline (p < 0.05) but still within the normal range. Blood urea nitrogen (BUN) and serum creatinine (CREA), which indicate renal function, significantly increased and decreased, respectively, relative to baseline (p < 0.05) but were within the normal range (Table 3).

Table 3.

Indicators of the efficacy and safety of IL-2 treatment (mean ± SD).

	Before IL-2	After IL-2	t	p
ESR (mm/h)	59.85 ± 36.62	28.88 ± 25.40	13.798	<0.001
CRP (mg/l)	41.98 ± 47.88	10.26 ± 21.64	8.078	<0.001
TJC	10.07 ± 7.97	3.94 ± 4.76	14.636	<0.001
SJC	6.40 ± 7.63	1.70 ± 3.32	11.212	<0.001
DAS28	5.44 ± 1.34	3.66 ± 1.09	22.611	<0.001
WBC (×109/l)	6.87 ± 2.89	9.62 ± 4.99	7.995	<0.001
RBC (×1012/l)	4.16 ± 0.55	4.29 ± 1.21	1.518	0.131
PLT (×109/l)	299 ± 101	270 ± 90	5.586	<0.001
Neutrophilic granulocyte (×109/l)	4.82 ± 2.53	6.31 ± 3.07	6.905	<0.001
Lymphocyte (×109/l)	1.57 ± 0.64	2.41 ± 1.15	10.959	<0.001
ALT (U/l)	24.71 ± 17.27	30.49 ± 34.05	1.457	0.150
AST (U/l)	27.06 ± 19.66	21.02 ± 14.91	2.428	0.018
GGT (U/l)	38.72 ± 39.83	39.73 ± 36.39	0.218	0.828
BUN (mmol/l)	5.46 ± 1.95	6.01 ± 2.21	2.124	0.038
CREA (µmol/l)	57.75 ± 14.90	55.36 ± 15.66	2.306	0.025

ALT, alanine aminotransferase; AST, aspartate aminotransferase; BUN, blood urea nitrogen; CREA, serum creatinine; CRP, C-reactive protein; DAS28, disease activity score-28; ESR, erythrocyte sedimentation rate; GGT, γ-glutamine transferase; IL-2, interleukin-2; PLT, platelet; RBC, red blood cells; SD, standard deviation; SJC, swollen joint count; TJC, tender joint count; WBC, white blood cells.

Patients treated with low-dose IL-2 showed a three-fold increase in the absolute counts of anti-inflammatory Tregs (26.26 ± 15.51 to 92.80 ± 64.92), and a two-fold increase in CD4+T cells and its subsets, such as Th1, Th2, and Th17 cells (p < 0.001) (Figure 3); however, peripheral Tregs were the only CD4+T subset that showed a significant increase in proportion (p < 0.05) (Supplemental Figure S6). After IL-2 treatment, the Th17/Treg ratio decreased significantly, down to the level of HCs, whereas the Th1/Th2 ratio did not change significantly (Figure 3).

Figure 3.

Efficacy of short-term, low-dose IL-2 treatment in regulating levels of CD4+T subsets. (a–e) Absolute counts of peripheral CD4+T and its subsets, especially Tregs, were significantly higher in RA patients after IL-2 treatment compared with baseline. (f, g) The Th17/Treg ratio decreased significantly in RA patients after IL-2 treatment, whereas the ratio of Th1/Th2 was not significantly different. Within-group comparisons were made using the paired samples t test before and after IL-2 therapy. ***p < 0.001. Significance values are asymptotic (two-sided tests) and the significance level is p < 0.05.

IL-2, interleukin-2; RA, rheumatoid arthritis; Tregs, regulatory T cells.

Safety

Low-dose IL-2 was well tolerated in all patients with RA. None of them displayed severe adverse effects. Non-severe adverse events were characterized by skin rashes at the injection site that healed spontaneously without special treatment.

Discussion

CD4+CD25+FOXP3+T cells, also known as Tregs, can modulate the immune system, maintain self-tolerance and immunological homeostasis, and suppress the proliferation of effector T cells and the production of pro-inflammatory cytokines and autoantibodies. In human and animal studies, dysfunction or reduction of circulating Tregs has been observed in autoimmune diseases, including systemic lupus erythematosus,[20] dermatomyositis/polymyositis (DM/PM),[16] primary Sjögren’s syndrome (pSS),[17] and RA.[21,22] However, results from several studies regarding the levels of peripheral Tregs in RA are controversial.[23] Thus, large amounts of data pertaining to the absolute counts of Tregs in PB have been needed to confirm whether lack or dysfunction of circulating Tregs is crucial to the immune mechanism of RA.

The present study investigated the levels of peripheral Tregs in a large sample of RA patients. Compared with HCs, patients with RA had fewer Tregs and Th1 (CD4+IFN-γ+T) cells, but not Th17 (CD4+IL-17+T) cells, which are important immune cells previously thought to be involved in the onset of RA. The reduced absolute count of Tregs rather than Th1 cells was the only difference in immune cells between new RA patients (i.e., recent onset or without previous immunosuppressive therapies) and healthy individuals. In addition, the absolute count of Tregs was clearly associated with disease activity and RF, and gradually decreased with disease progression in RA patients. These observations suggested that Tregs play an indispensable role in the pathogenesis and progression of RA. Evidence that Tregs may be involved in the progression of arthritis comes primarily from experimental mouse studies, in which disease was exacerbated with treatment by anti-25-depleting antibody to deplete Tregs[24]; conversely, adaptive transplantation of Tregs could lead to reduced disease activity.[25-27] We previously reported that the absolute count of Tregs was significantly lower in patients with DM/PM (both new and previously treated patients) compared with healthy subjects, while there was no significant difference between new and previously treated patients.[16] In other autoimmune diseases similar to RA, deficient immune tolerance mediated by depletion of circulating Tregs also contributes to the disease.[17,20,28] In addition, autoantibodies, such as RF and anti-MCV, were higher in patients with active RA, and were significantly correlated with markers of disease activity. Follicular Th cells are involved in the generation of high-affinity antibodies characteristic of RA, such as RF, anti-CCP, and anti-MCV, which can be suppressed with elevated expression of Tregs.[29] The mechanism of deficient immune tolerance mediated mainly by peripheral Tregs in RA patients has been unclear in previous studies, possibly due to decreased absolute counts of peripheral Tregs caused by Tregs migrating and presenting in inflamed joints during inflammatory responses,[30] or to the dysfunction of Tregs induced by IL-2 deficiency in patients with RA.[13,31,32] In addition, previous immunosuppressive drugs, such as methotrexate and leflunomide, as well as glucocorticoid, can lead to, or exacerbate, deficiency in Tregs or other CD4+T lymphocyte subpopulations, thereby increasing the risk of infections and tumors.[33-35] Therefore, immunoregulation regimens targeting Tregs, such as supplementation with exogenous IL-2 (or transfer of Tregs) to restore self-tolerance, may provide a new avenue for treating Treg-mediated diseases, such as RA. IL-2 has been shown to influence T cell differentiation in a dose-dependent way.[9] In our previous studies, the efficacy and safety of low-dose IL-2 for peripheral Tregs proliferation and disease remission were confirmed in patients with PsA,[15] DM/PM,[16] and primary SS,[17] without evaluated side effects.

Low-dose IL-2 in patients with RA can reduce disease activity by restoring immune tolerance and promoting the proliferation of circulating Tregs, without obvious adverse reactions or side effects. When the disease was gradually relieved, pro-inflammatory markers, such as Th17 cells, also increased significantly, which further confirmed that Tregs were the main lymphocyte subgroup involved in the pathogenesis of RA. Rosenzwajg reported that all autoimmune and inflammatory diseases are associated with insufficient Tregs[9]; low-dose IL-2 selectively and safely activated and increased Tregs in 11 autoimmune diseases, although only three subjects with RA were enrolled. Other studies have reported that low-dose IL-2 may also amplify Tregs and natural killer cells, thus sustaining cellular immunity, and is a well-tolerated treatment for SLE,[20,36] consistent with the results of Rosenzwajg.[9] Thus, the safety and efficacy of IL-2 has been demonstrated in different diseases without serious adverse treatment-related effects; however, the mechanism of IL-2 still needs further study. Although the present study included a large number of samples, long-term follow up is needed to further confirm the efficacy and safety of low-dose IL-2 combination treatment.

In conclusion, decreased absolute counts of circulating CD4+T lymphocyte subsets were observed in patients with RA. Moreover, circulating Tregs, which mediate immune tolerance, may be involved in the pathogenesis and progression of RA and can be restored by low-dose IL-2 without obvious side effects.

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Supplemental material, sj-pdf-1-tab-10.1177_1759720X211011370 for Low-dose IL-2 therapy limits the reduction in absolute numbers of circulating regulatory T cells in rheumatoid arthritis by Sheng-Xiao Zhang, Jia Wang, Cai-Hong Wang, Rui-Huan Jia, Ming Yan, Fang-Yuan Hu, Guang-Ying Liu, Xue-Yu Liu, Jing Luo, Chong Gao and Xiao-Feng Li in Therapeutic Advances in Musculoskeletal Disease