Rheumatoid arthritis–associated autoantibodies in non–rheumatoid arthritis patients with mucosal inflammation: a case–control study

Serum autoantibody levels were measured in adult patients without RA with PD) (n = 114), non-CF patients with BR (n = 80) and patients with CF (n = 41). Subjects without systemic disease and without PD served as the HC group (n = 36). Patients with established RA without lung disease and with known periodontal status served as a reference group (RA group, n = 86).

Patients with untreated severe PD were recruited from a referral practice for periodontology (Clinic for Periodontology Groningen). The inclusion criterion was >30 % of sites involved with clinical attachment loss ≥5 mm on the basis of full-mouth oral measurements [34]. The exclusion criteria were antibiotic use <3 months before inclusion and having systemic disease other than PD. To assess the inflammatory burden exerted by the periodontium, the periodontal inflamed surface area (PISA) [35] was quantified.

Sera from patients with BR without CF and without RA from a previously conducted randomized controlled trial were included [36]. Baseline serum samples were used to avoid a possible influence of treatment on antibody levels. Sera from a cohort of patients with CF without RA who visited the Department of Pulmonology of the University Medical Center Groningen for routine checkups were included. For BR and CF patients, the number of exacerbations was based on the number of antibiotic courses received 12 months before inclusion. The percentage predicted forced expiratory volume in 1 second (%FEV₁) at inclusion was used as a disease activity measure.

HC subjects were recruited from among subjects planned for first consultation at the dental department of the University Medical Center Groningen. Periodontal health was assessed using the Dutch periodontal screening index (DPSI) [37]. An inclusion criterion was DPSI score ≤2 (absence of PD), and exclusion criteria were antibiotic use <3 months before inclusion and presence of systemic disease.

Patients with established RA without lung disease at the time of inclusion and with known periodontal status as assessed by the DPSI served as a reference group for serological measurements. RA disease activity was assessed using the Disease Activity Score 28 tender and swollen joint count (DAS28).

In PD, RA and HC subgingival microbiological samples were tested for presence of P. gingivalis by using anaerobic culture techniques (for details, see [38]).

Participants provided written informed consent before study enrollment according to the Declaration of Helsinki. This study was conducted with the approval of the Medical Ethical Committee of the University Medical Center Groningen (METC UMCG 2009/356, METC UMCG 2011/010) and Medical Ethical Committee Noord-Holland (METC Noord-Holland M07-002).

IgG anti-cyclic citrullinated protein antibody (anti-CCP) levels were measured using a commercial anti-CCP2 kit (Euro Diagnostica, Malmö, Sweden) according to the manufacturer’s protocol. Samples with a value <25 U/ml were measured again with an adjusted protocol in which samples were diluted 1:10 instead of 1:50. The diagnostic cutoff value was defined as >25 U/ml according to the manufacturer’s instruction. However, IgG anti-CCP was not used as a diagnostic test for RA in this study; therefore, seropositivity was defined as >2 SD above the mean of HC (2.2 U/ml), analogous to the other autoantibodies measured.

IgA anti-CCP measurements were performed using a modification of the anti-CCP2 kit (Euro Diagnostica). Sera were diluted 1:50 using the dilution buffer provided by the manufacturer. The secondary antibody was horseradish peroxidase (HRP)-conjugated polyclonal goat anti-human IgA (SouthernBiotech, Birmingham, AL, USA), diluted 1:20,000 in phosphate-buffered saline (PBS) with 1 % bovine serum albumin (BSA) and 0.05 % Tween-20 (Sigma-Aldrich, St. Louis, MO, USA). The color reaction was performed using tetramethylbenzidine (Sigma-Aldrich) and hydrogen peroxide. A pool of four sera from RA patients with high levels of IgA anti-CCP served as a calibrator for the standard curve expressed in arbitrary units per milliliter (AU/ml) and starting at 200 AU/ml. Seropositivity was defined as >2 SD above the mean of HC.

To assess the citrulline-specific nature of the response, sera were tested on plates coated with the arginine-containing counterpart of CCP2: cyclic arginine peptide (CAP, kindly provided by Euro Diagnostica), following almost the same protocol as described for the IgG and IgA CCP2 enzyme-linked immunosorbent assay (ELISA). A dilution of patient serum with high levels of IgG anti- CAP served as a calibrator for the standard curve, starting at 100 AU/ml. Similarly, IgA anti-CAP reactivity was measured with a dilution of a high-level responding serum serving as a standard curve, starting at 100 AU/ml. Seropositivity was defined as >2 SD above the mean of HC.

Levels of IgG anti-CarP antibodies against carbamylated fetal calf serum were assessed using a protocol described by Shi et al. [8]. Seropositivity was defined as >2 SD above the mean of a distinctive HC cohort [8].

The specificity of the response against citrullinated proteins was assessed by testing reactivity against four synthetic citrullinated peptides that are known autoantigens in RA: fibrinogen-1 (Fib1, β-chain amino acids 36–52, NEEGFFSACitGHRPLDKK), fibrinogen-2 (Fib2, β-chain amino acids 60–74, CitPAPPPISGGGYCitACit), α-enolase (CEP-1, KIHACitEIFDSCitGNPTVE) and vimentin (Vim1, VYATCitSSAVCitLCitSSV). Every peptide was linked with its N terminus to biotin with a spacer (SGSG) in between. Reactivity against the citrullinated and native forms of the peptides was measured according to the method of van de Stadt et al. [39] with some modifications. In short, 96-well Costar plates (Corning, Corning, NY, USA) were coated overnight with 5 μg/ml streptavidin (Rockland Immunochemicals, Limerick, PA, USA) in PBS. Subsequently, plates were blocked for at least 1 hour with 2 % BSA and 0.05 % Tween-20 in PBS followed by incubation with the biotin-labeled peptides (0.5 μg/ml in PBS). Next, serum samples were diluted 1:100 in high-performance ELISA buffer (Sanquin, Amsterdam, the Netherlands) and incubated on the plates. Reactivity was detected with HRP-conjugated monoclonal mouse anti-human IgG (clone JDC-10; SouthernBiotech) diluted 1:2000 in PBS with 1 % BSA and 0.05 % Tween-20 or with HRP-conjugated polyclonal goat anti-human IgA (SouthernBiotech) diluted 1:4000 in the same dilution buffer. Bound antibodies were visualized by using tetramethylbenzidine and hydrogen peroxide. Reactivity against a citrullinated peptide and its native counterpart was measured on the same plate. Every serum sample was measured in duplicate, and a positive control serum sample was applied on each plate. The citrulline-specific response was expressed as the difference in optical density (ΔOD) between the citrullinated peptide and its native form, and it was considered positive when ΔOD was >2 SD above the mean of HC. Likewise, the arginine-specific response was expressed as ΔOD between the native peptide and its citrullinated form, and it was considered positive when ΔOD was >2 SD above the mean of HC.

IgM and IgA RF levels were assessed using a validated in-house ELISA [40]. Levels were expressed in international units (IU) per milliliter, and seropositivity was defined as >10 IU/ml for IgM RF and >25 IU/ml for IgA RF [40].

C-reactive protein levels were measured by performing ELISA (DuoSet; R&D Systems, Minneapolis, MN, USA).

Absorbance was read at 450 nm in an EMax microplate reader, and antibody levels were calculated by using SoftMax PRO software (Molecular Devices, Sunnyvale, CA, USA).

Statistical analysis was performed using GraphPad Prism software (version 5.00 for Windows; GraphPad Software, La Jolla, CA, USA) and IBM SPSS Statistics for Windows software (version 20.0; IBM, Armonk, NY, USA). Normality was tested using D’Agostino-Pearson omnibus K2 test. For group comparisons, a Mann–Whitney U test was used for continuous variables and Fisher’s exact test for categorical variables. Comparison of RA-AAB levels between the groups was done with Kruskal–Wallis one-way analysis of variance with Dunn’s multiple-comparisons post-test compared with HC if overall p < 0.05. A logistic regression model was used to analyze the association of the diseases with seropositivity for anti-CCP and RF. The model was adjusted for age, sex and smoking (former and current versus never). A logistic regression model appeared to be better than a linear regression model owing to non-normally distributed residuals. Associations of anti-CCP, RF and anti-CarP with disease activity were assessed by using a Mann–Whitney U test or an unpaired t-test with or without Welch’s correction, depending on normality and equality of variances. Correlations between different parameters were assessed by Spearman’s ρ.