Rhumatologie, Hôpitaux Universitaires de Strasbourg, Centre de Référence National des Maladies Auto-Immunes Systémique Rares, EA 3432 « Physiopathologie des Arthrites », Strasbourg, France
Institut Pour la Santé et la Recherche Médicale (INSERM) Unité 822, 'Epidémiologie, Démographie et Sciences Sociales', IFR69; Institut National d'Etudes Démographiques (INED); Université Paris 11, Le Kremlin-Bicêtre, France
CHRU de Tours; UMR CNRS 6239, Université de Tours; INSERM CIC-202, Tours, France
Immuno-Rhumatologie, Hôpital Lapeyronie, Université Montpellier 1, UGM 5535, Montpellier, France
Rhumatologie, INSERM U802, Université Paris-Sud 11, Hôpital Bicêtre, Assistance Publique-Hôpitaux de Paris (AP-HP), Le Kremlin Bicêtre, France
Abstract
Introduction
Little is known about systemic B-cell activation in early rheumatoid arthritis (RA). We therefore evaluated the serum levels of markers of B-cell activation in patients included in the ESPOIR early arthritis cohort.
Methods
In the ESPOIR early arthritis cohort (at least 2 swollen joints for more than 6 weeks but less than 6 months), 710 patients were assessed at 1 year and either met the 1987 American College of Rheumatology criteria for RA (n = 578) or had undifferentiated arthritis (n = 132). Baseline serum samples of patients naïve to corticosteroid and disease-modifying antirheumatic drug treatment were assessed for beta2-microglobulin, IgG, IgA, IgM, immunoglobulin free light chains of immunoglobulins, and B-cell activating factor of the tumor necrosis factor family (BAFF). The BAFF gene 871T>C polymorphism was genotyped in all patients.
Results
All markers of B-cell activation except BAFF and IgM were significantly higher in patients with early RA than those with undifferentiated arthritis. Anti-cyclic citrullinated peptide (anti-CCP) and beta2-microglobulin were associated with a diagnosis of early RA in the multivariate analysis. Markers of B-cell activation, except BAFF, were associated with disease activity, rheumatoid factor and anti-CCP secretion. The BAFF gene polymorphism was not associated with early RA.
Conclusions
Markers of B-cell activation are elevated in patients with early RA, compared with undifferentiated arthritis, independently of any systemic increase in BAFF secretion, and correlate with disease activity. This study sheds new light on the early pathogenic role of B-lymphocytes in RA and suggests that targeting them might be a useful therapeutic strategy in early RA.
Introduction
For decades – ever since the discovery of rheumatoid factor (RF) – B cells have been known to play a pathogenic role in established rheumatoid arthritis (RA)
Materials and methods
Patients
The French multicenter prospective cohort of patients with early arthritis (ESPOIR) has included 813 patients with early arthritis between December 2002 and March 2005 and plans to follow them for 10 years. Patients were eligible for inclusion in the cohort if they had a definitive or probable clinical diagnosis of RA or a diagnosis of UA with a potential for progressing to RA. Thus, these patients had at least two swollen joints, present for more than 6 weeks but less than 6 months, and were naïve for DMARDs and corticosteroids at inclusion. Their baseline clinical, immunological, and radiological features were recently published
Serum assessments
Serum samples were collected at enrollment and immediately stored at -80°C. One biological resource center was in charge of centralizing and managing biological data collection. Assessments of serum beta2-microglobulin, IgG, IgA, IgM, immunoglobulin FLCs (nephelometry), and BAFF (enzyme-linked immunosorbent assay, or ELISA; R&D Systems, Lille, France) were centralized. Serum samples of 40 patients were simultaneously thawed daily, and all of their markers of B-cell activation were assessed that day. Serum measurements of IgM and IgA RF (ELISA; Menarini France, Rungis Cedex, France, positive >9 IU/mL) and anti-CCP (anti-CCP2; DiaSorin, Saluggia [Vercelli], Italy, positive >50 U/mL) levels were performed in a central location and determined as previously reported
DNA genotyping
After genomic DNA was isolated from peripheral blood mononuclear cells, the BAFF promoter gene polymorphism 871T>C was genotyped with competitive allele-specific polymerase chain reaction by using FRET (fluoroscence resonance energy transfer) technology. This genotyping was successful for 686 patients and 90 healthy blood donors.
Radiological data
At enrollment, radiographs of the hands and wrists (anteroposterior view) and of the feet (anteroposterior and oblique views) were taken. Their interpretation was standardized as described previously
Statistical analysis
Continuous data are presented as medians with interquartile ranges. In spite of the high number of patients and because of the uneven frequency of early RA and UA data, we used nonparametric tests for statistical analysis of continuous variables. The Mann-Whitney
Results
Characteristics of the study population
The median age of the 710 patients (76.5% of whom were female) was 49 (40 to 64) years. At enrollment, 48.3% of the patients were IgM-RF-positive and 40.0% were anti-CCP-positive. Median DAS28 was 5.1 (4.3 to 5.9), and median HAQ was 0.9 (0.4 to 1.4). Radiographic erosions on hands or feet were seen at inclusion in 22.5% of the patients. Five hundred seventy-eight patients (79.2%) had met the 1987 ACR criteria for RA at any time since their inclusion and were classified as having early RA, and 132 patients still had UA at the 1-year follow-up visit. Baseline characteristics of the 710 patients are summarized in Table
Baseline characteristics of 710 patients with early rheumatoid arthritis or undifferentiated arthritis
Patients with early RA or UA
Early RA
UA
Univariate analysis:
Multivariate analysis:
OR (95% CI),
(1)
(2)
(1) versus (2)
(1) versus (2)
n = 710
n = 578
n = 132
Percentage of females
76.5%
77%
74%
0.8
Age, years
49.0 (40.0–64.0)
50.1 (42.3–65.2)
47.4 (39.5–62.4)
0.6
ESR, mm at 1st hour
22.0 (11.2–38)
23.0 (12.0–40.1)
17.0 (10.0–32.0)
0.01
0.9 (0.9–1.0), 0.6
CRP, mg/L
9.0 (0–24.0)
9.5 (3.0–25.0)
6.0 (0–16.0)
0.002
1.0(0.9–1.1), 0.3
Positivity for anti-CCP
40.3%
47.4%
13.2%
<0.0001
5.8 (3.4–10.0), 0.001
BAFF, ng/mL
0.7 (0.5–1.0)
0.7 (0.5–1.0)
0.7 (0.5–0.9)
0.5
Beta2–microglobulin, mg/L
1.9 (1.7–2.3)
2.0 (1.7–2.4)
1.8 (1.6–2.1)
0.0002
1.5 (1.0–2.0), 0.03
Total IgG, g/L
13.5 (11.5–16.1)
13.5 (11.7–16.1)
12.9 (10.9–16.0)
0.03
0.9 (0.9–1.0), 0.4
Total IgA, g/L
2.6 (1.9–3.5)
2.8 (1.9–3.5)
2.2 (1.7–3.1)
<0.0001
1.2 (0.9–1.5), 0.06
Total IgM, g/L
1.5 (1.1–2.0)
1.5 (1.1–2.0)
1.4 (1.1–1.9)
0.5
Kappa free light chain, mg/L
13.8 (10.5–17.9)
14.3 (10.9–18.7)
11.7 (9.6–14.9)
<0.0001
1.0 (0.9–1.0), 0.6
Lambda free light chain, mg/L
16.4 (12.8–21.6)
17.5 (13.2–22.5)
14.5 (11.6–18.8)
<0.0001
0.9 (0.9–1.0), 0.9
Ratio of kappa to lambda
0.8 (0.3–0.99)
0.8 (0.7–1.0)
0.8 (0.7–0.9)
0.9
Results are expressed as median values (25th–75th values) or as percentages. Comparison of proportions of presence of anti-cyclic citrullinated peptide (anti-CCP) used chi-square test, and comparison of the other variables used Mann-Whitney
Elevated markers of B-cell activation in patients with early rheumatoid arthritis
Comparison of markers of B-cell activation, except RF, which belongs to ACR criteria used to define RA, was performed between patients with early RA and patients with UA. Patients with early RA had significantly elevated serum levels of beta2-microglobulin, IgG, IgA, and immunoglobulin kappa and lambda FLCs. Anti-CCP, ESR, and CRP were also associated on univariate analysis with the diagnosis of early RA (Table
Serum BAFF levels in patients with early rheumatoid arthritis and with undifferentiated arthritis
BAFF was a possible explanation for the higher levels of markers of B-cell activation in early RA. The median BAFF levels were 0.7 (0.5 to 1.0) ng/mL in the 710 patients with arthritis and 0.5 (0.4 to 0.6) ng/mL in the 80 healthy blood donors (
Association of the BAFF 871T>C gene promoter polymorphism with early rheumatoid arthritis and undifferentiated arthritis
We analyzed the distribution of the BAFF 871T>C polymorphism among patients with early RA and patients with UA. The two groups did not differ significantly for any allelic or genotypic frequencies (Table
Allelic and genotypic distribution of BAFF -871T/C among patients with early rheumatoid arthritis, undifferentiated arthritis, and controls
BAFF -871T/Caia
Early RA
UA
Controls
Odds ratio (95% CI)
Odds ratio (95% CI)
Allele frequencies
n = 1,112
n = 260
n = 180
Early RA versus UA
Early RA versus controls
-871C (%)
603 (54)
146 (56)
90 (50)
NS
1.00 (0.77–1.30)
NS
1.18 (0.86–1.62)
-871T (%)
509 (46)
114 (44)
90 (50)
Genotype frequencies
n = 556
n = 130
n = 90
CC (%)
171 (31)
43 (33)
21 (23)
NS
1.02 (0.68–1.53)
CC versus CT and TT
NS
1.46 (0.87–2.46) CC versus CT and TT
CT (%)
261 (47)
60 (46)
48 (54)
TT (%)
124 (22)
27 (21)
21 (23)
NS
1.02 (0.66–1.60)
TT versus CT and CC
NS
0.94 (0.56–1.60) TT versus CT and CC
Comparisons used chi-square test. BAFF, B-cell activating factor of the tumor necrosis factor family; CI, confidence interval; NS, not significant; RA, rheumatoid arthritis; UA, undifferentiated arthritis.
Association of markers of B-cell activation with initial disease activity, Health Assessment Questionnaire, autoantibody secretion, and early erosion in patients with early rheumatoid arthritis
We subsequently investigated whether an elevated level of markers of B-cell activation was associated with a specific clinical, immunological, or radiological pattern in patients with early RA. The initial DAS28 was slightly but significantly correlated with serum levels of beta2-microglobulin (
Association between baseline B-cell activation biomarkers and immunological features of the 578 patients with early rheumatoid arthritis
IgM RF +
IgM RF -
Anti-CCP +
Anti-CCP -
n = 321
n = 257
n = 274
n = 304
BAFF
0.7 (0.5–0.9)
0.7 (0.5–1.0)
0.18
0.7 (0.5–0.9)
0.7 (0.5–0.9)
0.18
Beta2–microglobulin
2.1 (1.8–2.4)
1.9 (1.6–2.3)
0.01
2.0 (1.7–2.4)
1.9 (1.6–2.4)
0.30
Total IgG
14.0 (12.0–16.9)
13.0 (11.1–15.1)
<10-4
14.4 (12.4–17.1)
12.9 (11.1–15.9)
<10-4
Total IgA
2.9 (2.1–3.7)
2.5 (1.9–3.3)
<10-4
3.1 (2.3–3.8)
2.4 (1.8–3.2)
<10-4
Total IgM
1.6 (1.2–2.2)
1.3 (1.1–1.8)
<10-4
1.6 (1.2–2.3)
1.4 (1.0–1.9)
<10-4
Kappa free light chain
15.8 (12.2–20.6)
12.7 (9.5–16.8)
<10-4
16.3 (12.7–20.6)
12.7 (9.7–17.1)
<10-4
Lambda free light chain
18.6 (14.4–25.0)
15.0 (11.8–19.6.)
<10-4
19.3(14.9–24.9)
15.1 (11.9–19.9)
<10-4
Results are expressed as median values (25th–75th values). B-cell activating factor of the tumor necrosis factor family (BAFF) values are expressed in nanograms per milliliter, total immunoglobulin values in grams per liter, and free light chain of immunoglobulins in milligrams per liter. Comparisons used Mann-Whitney
Baseline clinical and biological features in patients with early rheumatoid arthritis according to the presence of radiological erosions at enrollment
Early erosions
Absence of early erosion
Univariate analysis:
Multivariate analysis:
OR (95% CI),
n = 138
n = 377
Initial DAS28
5.4 (4.6–6.4)
5.2 (4.3–6.5)
0.1
ESR, mm at 1st hour
29.5 (13.0–54.0)
20.5 (11.0–36.0)
0.002
1.1 (0.9–1.3), 0.4
CRP, mg/L
11.0 (4.0–33.1)
9.0 (0–22.0)
0.1
IgM-RF-positive
63.7%
52.5%
0.03
0.7 (0.4–1.3), 0.2
IgA-RF-positive
64.5%
45.9%
0.0003
1.7 (1.1–2.7), 0.01
Anti-CCP-positive
61.6%
41.6%
<0.0001
2.3 (1.2–4.3), 0.008
BAFF, ng/mL
0.7 (0.5–0.9)
0.8 (0.5–1.0)
0.5
Beta2–microglobulin, mg/L
2.1 (1.7–2.4)
1.9 (1.7–2.4)
0.08
Total IgG, g/L
13.7 (12.0–15.6)
13.3 (11.5–15.9)
0.2
Total IgA, g/L
3.0 (2.1–3.7)
2.6 (1.9–3.4)
0.003
1.1 (0.9–1.2), 0.4
Total IgM, g/L
1.4 (1.1–2.1)
1.5 (1.1–2.1)
0.9
Kappa free light chain, mg/L
15.3 (11.9–20.7)
13.9 (10.4–17.9)
0.007
1.0 (0.9–1.1), 0.2
Lambda free light chain, mg/L
18.3 (13.5–23.4)
16.9 (12.8–21.9)
0.1
Results are expressed as median values (25th–75th values) or as percentages. Comparison of proportions of presence of IgM-RF, IgA-RF, and anti-cyclic citrullinated peptide (anti-CCP) used chi-square test, and comparison of the other variables used Mann-Whitney
Discussion
These findings from ESPOIR, the prospective French multicenter cohort of early arthritis patients, demonstrate that serum markers of B-cell activation are elevated in patients with early RA compared with undifferentiated early arthritis. They also show that markers of B-cell activation are correlated with disease activity. Lastly, they indicate that serum BAFF might not drive the specific B-cell activation we observed in early RA. ESPOIR offered us the opportunity to investigate markers of B-cell activation in patients with early arthritis who had not yet been exposed to corticosteroids or DMARDs at enrollment. The disease-related increase of markers of B-cell activation might otherwise have been masked by these treatments, which can modulate these marker levels
The main limitations of this study were the short duration of follow-up (1 year) so far, since ACR criteria for RA might be fulfilled later, and the absence of validated criteria for early RA. Although the 1987 ACR criteria lack specificity for early RA diagnosis
The ESPOIR cohort confirms the pathogenic activation of autoreactive B cells in early RA, reflected by the association between anti-CCP and IgA-RF with early radiological erosions, also observed in previous early RA cohorts
The first important finding is that serum level markers of alloreactive B-lymphocyte activation are higher in early RA than in UA. Some features of B-cell activation were nonetheless observed in patients with UA, including BAFF levels that were higher than in healthy donors, elevated IgG in 55% of the patients, and elevated levels of immunoglobulin FLCs in 22% (compared with 0% in healthy donors, according to previous studies
Our second important finding was the absence of an association between the BAFF gene polymorphism and either RA or any of the baseline clinical, immunological, or radiological characteristics of RA. The lack of an association with RA is consistent with a previous Japanese genetic study
Serum BAFF level was higher than in healthy blood donors, as previously reported for patients with established disease
Thus, the specific increase of markers of B-cell activation in early RA might not be related to the increase of BAFF secretion. Membrane-bound BAFF or post-translational changes of BAFF (glycosylation, trimerization with a proliferation-inducing ligand [APRIL] or delta BAFF) might affect serum B-cell activation independently of the quantity of BAFF secreted and detected in the serum. The role of local BAFF production in arthritic joints cannot be ruled out either since BAFF levels are reported to be higher in synovial fluid than in serum
Our results thus suggest that serum BAFF does not drive B-cell activation in early RA, at least not directly or solely. The triggering forces of B-cell activation in early RA may depend on T lymphocytes. A specific pattern of T-lymphocyte activation was recently reported in RA, with Th2 (interleukin [IL]-4, IL-13) and IL-17 expression increasing temporarily in the synovial fluid of patients with very early RA
Interestingly, our results showed elevated serum IgA levels in early RA. This might be related to synovial, T cell-independent activation of B lymphocytes, which might be locally triggered by resident cells of autoimmunity, like synoviocytes, as described in mucosa
Lastly, one of the important results of the study was the association observed between the increase in some markers of B-cell activation and disease activity (assessed by DAS28) and between the increase in some markers of B-cell activation (total IgA and kappa FLCs) and disease severity (early radiological erosion at inclusion). The relevance of markers of B-cell activation as prognostic markers will be further investigated throughout the cohort study, planned to last for 10 years to ensure assessment of patients' long-term clinical and radiological course. From a therapeutic perspective, these results suggest the potential value of B-cell depletion in early RA, which is currently under evaluation in controlled trials.
Conclusions
The elevation of markers of B-cell activation in very early RA demonstrates that B-cell activation is an early pathogenic event in RA. B-cell activation is not directly driven by a systemic increase of BAFF in early RA. The increase of some markers of B-cell activation is associated with disease activity, autoantibody secretion, and early radiological erosion. This study thus sheds new light on the early pathogenic role of B lymphocytes in RA and suggests that targeting these cells might be a useful therapeutic strategy in early RA.
Abbreviations
ACR: American College of Rheumatology; anti-CCP: anti-cyclic citrullinated peptide; APRIL: a proliferation-inducing ligand; BAFF: B-cell activating factor of the tumor necrosis factor family; CRP: C-reactive protein; DAS28: disease activity score using 28 joint counts; DMARD: disease-modifying antirheumatic drug; ELISA: enzyme-linked immunosorbent assay; ESR: erythrocyte sedimentation rate; FLC: free light chain; HAQ: Health Assessment Questionnaire; IL: interleukin; OR: odds ratio; RA: rheumatoid arthritis; RF: rheumatoid factor; SLE: systemic lupus erythematosus; TNF: tumor necrosis factor; UA: undifferentiated arthritis; VAS: visual analog scale.
Competing interests
The authors declare that they have no competing interests.
Authors' contributions
J-EG and XM analyzed the data and wrote the manuscript. CM-R analyzed BAFF gene polymorphism. BD performed statistical analyses. PG and BC contributed to the analysis and revised the manuscript. All authors read and approved the final manuscript.
Acknowledgements
We thank all of the investigators who recruited and followed the patients: Francis Berenbaum, Paris-Saint Antoine; Marie-Christophe Boissier, Paris-Bobigny; Alain Cantagrel, Toulouse; Maxime Dougados, Paris-Cochin; Patrice Fardelonne, Amiens; Bruno Fautrel and Pierre Bourgeois, Paris-La Pitié; Rene-Marc Flipo, Lille; Frederic Liote, Paris-Lariboisière; Xavier Le Loet, Rouen; Olivier Meyer, Paris-Bichat; Alain Saraux, Brest; Thierry Schaeverbeke, Bordeaux; Jean Sibilia, Strasbourg; Valerie Devauchelle, Brest, for expert radiograph interpretation; Sylvie Martin, Paris-Bichat, who performed all of the assays of CRP, IgA and IgM rheumatoid factor, and anti-CCP antibodies; and Laurence Meyer (Epidemiology, INSERM U 569, Le Kremlin Bicêtre), who reviewed the statistical procedures. We want to acknowledge the tremendous work of Nathalie Rincheval, who supervised the data collection of the ESPOIR cohort. An unrestricted grant from Merck Sharp & Dohme (Whitehouse Station, NJ, USA) was allocated for the first 5 years of the ESPOIR cohort. Two additional grants from INSERM were obtained to support part of the biological database. The French Society of Rheumatology, Abbott Laboratories (Abbott Park, IL, USA), Amgen (Thousand Oaks, CA, USA), and Wyeth (Madison, NJ, USA) have provided funding for the ESPOIR cohort study. J-EG received a grant from the French Society of Rheumatology to perform the assessment of markers of B-cell activation. The other authors did not receive any grants for the study.