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About the Authors:

Thao H. P. Nguyen

Roles Data curation, Formal analysis, Investigation, Visualization, Writing – original draft

* E-mail: [email protected]

Affiliations Lillehammer Hospital for Rheumatic Diseases, Lillehammer, Norway, University of Oslo, Faculty of Medicine, Institute of Clinical Medicine, Oslo, Norway

ORCID logo https://orcid.org/0000-0003-2597-4031

Ingrid Hokstad

Roles Data curation, Resources, Writing – review & editing

Affiliation: Department of Laboratory medicine, Innlandet Hospital Trust, Lillehammer, Norway

Morten Wang Fagerland

Roles Formal analysis, Methodology, Supervision, Visualization, Writing – review & editing

Affiliation: Oslo Centre for Biostatistics and Epidemiology, Research Support Services, Oslo University Hospital, Oslo, Norway

Tom Eirik Mollnes

Roles Funding acquisition, Investigation, Methodology, Project administration, Resources, Writing – review & editing

Affiliations Department of Immunology, Oslo University Hospital, Oslo, Norway, Research Laboratory, Nordland Hospital, Bodø, and Faculty of Health Sciences, K.G. Jebsen TREC, University of Tromsø, Tromsø, Norway, Centre of Molecular Inflammation Research, Norwegian University of Science and Technology, Trondheim, Norway

Ivana Hollan

Roles Conceptualization, Funding acquisition, Investigation, Project administration, Resources, Visualization, Writing – review & editing

Affiliations Beitostølen Health and Sport Centre, Beitostølen, Norway, Norwegian University of Science and Technology, Gjøvik, Norway

Mark W. Feinberg

Roles Resources, Writing – review & editing

Affiliations Harvard Medical School, Boston, Massachusetts, United States of America, Division of Cardiology, Brigham and Women´s Hospital, Boston, Massachusetts, United States of America

Gunnbjørg Hjeltnes

Roles Data curation, Investigation, Project administration, Writing – review & editing

Affiliation: Department of Internal Medicine, Innlandet Hospital Trust, Lillehammer, Norway

Gro Ø. Eilertsen

Roles Writing – review & editing

Affiliations Faculty of Health Sciences, Department of Clinical Medicine, UIT—The Arctic University of Norway, Tromsø, Norway, Department of Rheumatology, University Hospital of North Norway, Tromsø, Norway

Knut Mikkelsen

Roles Conceptualization, Resources, Writing – review & editing

Affiliation: Volvat Medical Center, Lillehammer, Norway

Stefan Agewall

Roles Conceptualization, Investigation, Project administration, Resources, Supervision, Visualization, Writing – review & editing

Affiliations University of Oslo, Faculty of Medicine, Institute of Clinical Medicine, Oslo, Norway, Department of Cardiology, Oslo University Hospital, Ullevål, Oslo, Norway

Introduction

Rheumatoid arthritis (RA) is associated with a wide range of cardiovascular disease (CVD) manifestations. Of those, accelerated atherosclerosis is of particular importance as it is the main cause of premature CVD mediated morbidity and mortality in RA [1–3]. The exact pathogenetic mechanisms behind increased rates of CVD events in RA are still unclear. However, there is evidence that besides traditional CVD risk factors, systemic inflammation and immune dysregulation play a pathogenic role in the development of accelerated atherosclerosis [4–6]. Inflammation alters metabolic processes, and is involved in all stages of the atherosclerotic disease, from induction of endothelial dysfunction, atheroma formation and destabilization, to thrombogenesis [7–9].

Complement is a key component of innate immunity in addition to bridging to adaptive immune responses [10]. It plays a central role in defense system against microbial invaders, clearance of damaged tissue and apoptotic cells, and modulation of inflammatory processes [10,11]. The complement system can be activated via one of three pathways (classical, alternative or lectin), which converge at C3 and C5 activation and share a common terminal pathway. Activation of complement through any of its three activations pathways results in formation of the terminal C5b-9 complement complex, which may remain in plasma as soluble C5b-9 (TCC) or be inserted in the cell membrane as membrane attack complex [10,11]. Excessive activation of the complement system due to chronic inflammatory rheumatic disease, may cause an immune imbalance and increase systemic and local inflammation, and may lead to vascular tissue damage. Inadequate control of complement activation is suggested to play a major role in pathology of inflammatory and autoimmune diseases, including RA, where the cartilage, bone and synovium are targeted [12,13]. High levels of complement activation products have been demonstrated in the synovial fluid and synovial tissues of patients with RA [14–16]. Additionally, RA patients have been reported to have higher concentrations of TCC in the blood than their non-RA counterparts [17–21].

Furthermore, substantial scientific evidence is now available supporting the strong relationship between several complement components and the pathophysiology of numerous CVD outcomes, including coronary artery disease and heart failure [22–26]. TCC promotes activation of platelets and fibrin formation, facilitating thrombogenesis [23]. The complement system is recognized to play an important role in the formation of atherosclerotic lesions, which might result in plaque rupture and thrombus formation with subsequent development of acute coronary syndrome [24–26]. Compared to healthy arteries, complement activation is more pronounced in atherosclerotic arteries, often activated near cholesterol crystals in lesions [27], and in ruptured compared to stable atherosclerotic lesions [28].

However, in spite of the scattered knowledge about the complement system in RA and CVD, little information is available in relation to complement activation in response to treatment and its importance in the development of premature CVD in RA. Therefore, in this study we wanted to investigate the impact of antirheumatic treatment on complement activation in terms of plasma TCC levels in RA. We further assessed associations between TCC levels and established inflammatory and CVD biomarkers, including endothelial function.

Materials and methods

Patients

In this study, we included sixty-four patients starting with either methotrexate (MTX) monotherapy (n = 34) or TNF inhibitor (TNFi) with or without MTX co-medication (TNFi ± MTX, n = 30) due to active RA. Patients were recruited as part of the Norwegian prospective observational Psoriatic arthritis, Ankylosing spondylitis, Rheumatoid Arthritis (PSARA) study. Recruitment and study procedures have been described in detail previously [29–31]. Patients fulfilled the American Rheumatism Association 1987 revised criteria for the classification of RA [32], and there was a clinical indication for starting treatment with MTX and/or TNFi (adalimumab, etanercept or infliximab). The treatment modality was based on clinical judgment performed by a rheumatologist not involved in this study, and in accordance with the Norwegian guidelines that adhere to the main international recommendations [33]. All patients starting with MTX were MTX naïve, and all patients starting with TNFi had been previously unsuccessfully treated with MTX.

The study was registered with the following trial registrations: Clinical trials (NCT00902005) and the Norwegian Biobank register (2054). The study was approved by Regional committee for medical and health research ethics in Norway (s-07377b), and all individuals in PSARA gave written informed consent.

Clinical and laboratory tests

Patients were examined at baseline, after 6 weeks and 6 months of treatment. Data collection included demographic data, medical history, life-style parameters, medication, self-reported questionnaires and physical findings. Venous blood samples were drawn after fasting of eight hours.

Endothelial function was assessed by the Reactive Hyperemia Index (RHI), measured by a fingertip plethysmograph (EndoPAT 2000, Itamar Medical Inc., Caesarea, Israel) as described previously [34,35]. An RH-PAT score of ≤ 1.67 signified endothelial dysfunction, as recommended by the manufacturer [36]. This value of 1.67 was also recommended by the Physiological Diagnosis Criteria for Vascular Failure Committee in the Japan Society for Vascular Failure [37], based on a study of Bonetti et al. [38]. Plethysmography was performed after fasting for at least eight hours, including non-allowance for smoking for at least twelve hours.

Blood samples

Routine hematologic and biochemical tests including C-reactive protein (CRP), erythrocyte sedimentation rate (ESR), white blood cells (WBC), anti-citrullinated protein antibody (ACPA) and Rheumatoid Factor IgM (RF-IgM) were performed at the local hospital laboratory on the day of collection at all visits. ACPA and RF-IgM were determined by enzyme-linked immunosorbent assays (ELISA), (QUANTA liteTM CCP3 IgG ELISA and QUANTA LiteTM RF IgM ELISA, both INOVA Diagnostics, Inc; San Diego, CA).

Additional blood samples for later analyses (including TCC) were immediately prepared, divided into small aliquots, and stored at -80°C until analyzed.

Complement activation was detected by TCC in EDTA plasma, using our in-house ELISA, as described in detail by Bergseth et al. [39]. Lower detection limit was 0.3 CAU/mL, intra- and inter-assay coefficients of variability were 14% and 15% respectively. The upper reference limit was < 0.7 CAU/mL based on samples form healthy blood donors. The units were designated as Complement Activation Unit (CAU)/mL based on an international standard as described in Bergseth et al. [39].

Statistical analyses

Continuous data were expressed as median (interquartile range [IQR]) and categorical data by number (percentage) as appropriate. As most continuous variables were not normally distributed, and particularly because the TCC measurements contained several extreme values, median regression was applied for comparisons between and within groups. Median regression is analogous to linear regression but provides inference about medians instead of means. The median regression models used the Hall-Sheather bandwidth method as the nonparametric density estimator under the assumption that the residuals are independent and identically distributed. Spearman’s rank-order coefficients, with 95% confidence intervals based on the Fisher Z transformation, were calculated to evaluate correlations between TCC, RA- and CV related variables at baseline, after 6 weeks and 6 months of antirheumatic treatment. The multiple regression models were adjusted for age and gender and for the baseline characteristics that were statistically significantly related to TCC in simple regression analysis. Chi-squared tests were used for comparisons of categorical data between groups.

A two-tailed probability value of p < 0.05 was considered statistically significant. For statistical calculations we used Stata/SE 16 (StataCorp LLC, College Station, TX).

Results

Baseline characteristics of all the patients

Baseline clinical and cardiovascular characteristics of patients are presented in Tables 1 and 2, respectively.

[Figure omitted. See PDF.]

Table 1. Baseline clinical characteristics.

https://doi.org/10.1371/journal.pone.0264628.t001

[Figure omitted. See PDF.]

Table 2. Baseline cardiovascular characteristics.

https://doi.org/10.1371/journal.pone.0264628.t002

About half of the patients started with MTX monotherapy, while in the other half, TNF±MTX were initiated due to insufficient MTX response. Disease activity was high with a median DAS28-ESR of 5. Patients on TNF±MTX treatment were 4.9 years older than those treated with MTX monotherapy (median disease duration 5.0 versus 0.1 year). More patients in TNF±MTX treatment group had subcutaneous rheumatoid nodules as compared to MTX only treatment group (Table 1).

One third of all the patients smoked, and the number of smokers in the MTX only treatment group did not differ from the TNF±MTX treatment group. No further substantial differences were noted when comparing MTX only treatment group to patients treated with TNFi regimens. (Table 2).

TCC and RA- and other CVD-related risk factors at baseline

The median baseline TCC level was 1.10 CAU/mL, and 57 (89%) patients had TCC above the upper limit of the estimated reference range with no difference between patients treated with MTX monotherapy and those treated with TNFi regimens (Table 1). No differences in plasma levels of TCC were noted between smokers and non-smokers, neither at baseline (p = 0.19), nor at 6-week (p = 0.21) or 6-month visit (p = 0.47).

Patients with endothelial dysfunction had significantly higher TCC compared to those without (median 1.4 versus 1.0 CAU/mL, p = 0.023) (Fig 1). However, TCC was not related to RHI at any point of time (pbaseline = 0.08, p6-week = 0.82, and p6-month = 0.50), although there was a modestly negative correlation between baseline TCC and baseline RHI in MTX only treatment group (Spearman´s rho = -0.38 [95% CI = -0.63 to -0.04], p = 0.031).

[Figure omitted. See PDF.]

Fig 1. Baseline TCC in patients with and without endothelial dysfunction.

Boxplots presenting the distribution of the baseline values of TCC in patients with and without endothelial dysfunction. The lines inside the boxes show the median, bottom and top of the box represent 25 and 75 percentile and whiskers represent minimum and maximum values. Endothelial dysfunction defined as reactive hyperemia index ≤ 1.67. Values are given in median. TCC: Soluble terminal complement complex.

https://doi.org/10.1371/journal.pone.0264628.g001

Associations between TCC and selected variables at baseline are presented in Table 3.

[Figure omitted. See PDF.]

Table 3. Associations between TCC levels and selected variables at baseline.

https://doi.org/10.1371/journal.pone.0264628.t003

In crude analyses, TCC levels positively correlated with inflammatory markers like CRP, ESR and interleukin 6 (IL-6). However, only association with IL-6 remained significant after adjustment for age and gender (Table 3).

Changes in TCC levels with antirheumatic treatment

Compared to baseline, TCC levels reduced significantly already after 6 weeks of antirheumatic therapy in both treatment groups. After 6 months on antirheumatic therapy, reduction in TCC persisted only after administration of TNFi±MTX compared to baseline, whereas no significant change was observed in patients treated with MTX only (Figs 2 and S1). However, there were no statistically significant differences in changes in TCC between MTX only group and TNFi±MTX treatment group at any point of time (pbaseline-6weeks = 1.00; p6weeks- i6months = 0.34; pbaseline-6months = 0.49).

[Figure omitted. See PDF.]

Fig 2. Changes in TCC with MTX monotherapy and TNFi±MTX treatment.

Boxplot displaying the difference in TCC at baseline and post-treatment with MTX monotherapy and TNFi±MTX for the whole population. The lines inside the boxes show the median, bottom and top of the box represent 25 and 75 percentile and whiskers represent minimum and maximum values. Values are given in median. MTX: Methotrexate, TNFi: Tumor necrosis factor inhibitors, TCC: Soluble terminal complement complex.

https://doi.org/10.1371/journal.pone.0264628.g002

Percentage of patients with TCC above the upper limit of the estimated reference range at 6-week and 6-month visit reduced to 75% and 72%, respectively, as compared to baseline (89%).

In patients with higher TCC levels, antirheumatic treatment led to significant improvement in RHI after 6 weeks, compared to baseline (median 1.84 vs 2.01 CAU/mL, p = 0.029). After 6 months of treatment, a marginal improvement in RHI was observed in MTX only treatment group, as compared to baseline (median 1.80 vs 2.09, p = 0.057).

Changes in TCC and some selected clinical and laboratory variables are shown in Table 4.

[Figure omitted. See PDF.]

Table 4. Changes in TCC and some selected clinical and laboratory variables.

https://doi.org/10.1371/journal.pone.0264628.t004

Associations of changes in TCC with markers related to arthritis activity and CVD

Associations of changes in TCC with selected clinical and laboratory variables after 6 weeks and 6 months of antirheumatic treatment are shown in Tables 5 and 6, respectively.

[Figure omitted. See PDF.]

Table 5. Associations between changes in TCC and changes in selected markers of arthritis activity after 6 weeks of treatment.

https://doi.org/10.1371/journal.pone.0264628.t005

[Figure omitted. See PDF.]

Table 6. Associations between changes in TCC and changes in selected variables after 6 months of treatment.

https://doi.org/10.1371/journal.pone.0264628.t006

Reductions in TCC from baseline to 6 weeks and from baseline to 6 months were related to decreased CRP, ESR and IL-6.

Reduction in TCCC after 6 months on antirheumatic treatment was correlated with decrease of some clinical markers of RA activity (e.g., DAS28-ESR, PtGA and MHAQ), and with increased levels of all types of cholesterol, and triglycerides (Table 6).

At 6-month visit, it was observed a marginal elevation in total cholesterol level (median difference = 0.20 [95% CI = -0.006 to 0.41], p = 0.056), and a statistically significant increase in HDL-C (median difference = 0.10 [95% CI = 0.02 to 0.18], p = 0.012) in the whole population. Changes in LDL-C and triglyceride did not reach statistical significance level (median difference = 0.10 [95% CI = -0.05 to 0.25], p = 0.20 and median difference = -0.02 [95% CI = -0.13 to 0.09], p = 0.72, respectively)

Discussion

In this study, complement activation as detected by plasma TCC was increased in the majority of patients with active RA, and the complement activation reduced rapidly and sustainably after initiation of antirheumatic treatment. Notably, during the 6-month follow-up period, sustained reduction in TCC was achieved only after administration of TNFi±MTX, whereas treatment with MT alone reduced TCC after 6 weeks, but not after 6 months. TCC positively correlated to inflammatory markers at baseline, and reductions in TCC with treatment were related to decreased inflammatory markers and increased total cholesterol, high-density lipoprotein (HDL-C) and low-density lipoprotein cholesterol (LDL-C) values. Moreover, baseline TCC levels were significant lower in RA patients with normal endothelial function compared to those with disturbed endothelial function.

The presence of increased complement activation in autoimmune arthritis, such as RA and spondyloarthropathies, has been reported before [14–16,40], and is confirmed by the results of the present study. This might point to the contribution of complement activation in the pathogenesis of RA.

Concordant with previous studies, our data showed a clear association between complement activation and markers of RA disease activity, and that initiation of TNFi brought on sustained reduction in complement activation in form of TCC, as well as these inflammatory markers [40,41–43]. However, the exact pathogenetic mechanisms regarding complement activation in response to TNFi therapy are still incompletely understood. Several explanations may partly account for this.

First, up to 90% of plasma complement components are produced by hepatocytes [44], and hepatic synthesis is upregulated in response to various cytokines, e.g., TNF [45–47], which is a pivotal mediator and driver of inflammation in RA [48]. This may explain the finding of increased soluble complement products in our patients, reverted by inhibition of TNF.

Second, former studies have demonstrated that the classical pathway of complement is in part activated by CRP [42,49,50], a routinely assessed marker of systemic inflammation in RA [51]. Therefore, reduction in CRP induced by antirheumatic therapy, could be associated with decreased complement activation.

Third, antirheumatic therapy exert their effect partly by inhibition of IL-6-production, leading to downregulation of CRP synthesis by hepatocytes and subsequently reduced activation of the classical pathway [52–54].

It is worth mentioning that MTX monotherapy also led to rapid reduction in TCC already within 6 weeks, but at 6 months, the change in TCC did not reach statistical significance. There are few studies suggesting any direct effect of MTX on complement system. The anti-inflammatory effects of MX are broad, and the mechanisms are not fully understood. MTX, via its metabolite adenosine, exerts inhibitory effect on production of TNF and promote secretion of IL-6, and thus might attenuate the complement cascade [55]. Moreover, MTX exposure has been shown to be associated with higher expression of complement genes, and increased complement activation products C3 and C5 in liver in patients with inflammatory arthritis [56].

Thus, the observed data in our study are consistent with the conclusion that reduction of complement system could be one of the mechanisms by which TNFi exert their effectiveness on RA. Our findings suggest that TCC could be an attractive biomarker for measurement of disease activity and also effect of TNFi in RA.

There is strong scientific evidence for the involvement of inflammation in endothelial dysfunction, the subclinical precursor to overt CVD [57,58]. Mechanistically, TCC activation and the membrane attack complex can initiate NLRP3 inflammasome activation triggering induction of IL-1ß, IL-6, and IL-18 secretion in endothelial cells, vascular smooth muscle cells, or leukocytes in the vessel wall [59,60]. Our result ties well with previous studies wherein patients with endothelial dysfunction had significant higher circulating levels of TCC in the blood [61,62], and that endothelial function improved with antirheumatic treatment (data not completely shown) [63,64].

Taken together, our findings support the notion that complement activation is involved in chronic inflammation and in endothelial dysfunction, and suggest that better control of complement activation might also control atherogenesis and ameliorate CVD risk.

However, in the present study, we did not find correlation between change in TCC and change in endothelial function after treatment. This might reflect the complexity and not fully elucidated pathophysiological mechanisms of endothelial dysfunction in our patients. The lack of association between TCC and endothelial function after 6 months on antirheumatic treatment could be due to our method of endothelial function assessment. Several tools have been validated for assessing vascular endothelial function, and the most commonly performed and best validated method is brachial artery ultrasound scanning (BAUS), evaluating flow-mediated dilatation (FMD) [65]. This technique, recommended by the international Brachial Artery Reactivity Task Force, is based on the percentage change of the brachial artery diameter during reactive hyperemia. Nevertheless, accurate assessment of FMD is technically challenging to perform, and this method is strongly operator-dependent, and therefore prone to operator bias and high variability [66]. The reactive hyperemia-peripheral arterial tonometry (RH-PAT) test, based on the same principle of reactive hyperemia as BAUS, is relatively simple, easy to perform in a standardized manner, less operator-dependent than that of FMD, and with comprehensive automatic analysis. Another benefit of RH-PAT is that this technique evaluates vascular dilatation in both arms–using contralateral arm as its internal control to correct for systemic changes during testing [34,35]. However, the main disadvantage of this technique is that it could be difficult to obtain stable measurements because RH-PAT recordings have shown to be sensitive to mental stress, anxiety, smoking and hyperglycemia [67–69]. To minimize the impact of confounding factors on the RH-PAT results, our patients were examined in tightly controlled environments, including rest period of 15 minutes, fasting for at least eight hours and refraining from tobacco for at least twelve hours before examination.

Moreover, no associations were observed between TCC and circulating markers for CVD, including coronary artery disease and heart failure, such as high-sensitivity troponin T, N-terminal pro-brain natriuretic peptide and pentraxin 3.

High levels of systemic inflammation in RA are associated with suppression of total cholesterol, LDL-C and HDL-C levels, partly due to impaired cholesterol efflux capacity of HDL-C [70,71]. Our data showed that reductions in TCC after 6 months of antirheumatic treatment were correlated with increased levels of all types of cholesterol and triglycerides. The results are in accordance with a former study demonstrating an inverse correlation of TCC and HDL-C [70], and that disease modifying antirheumatic drugs are associated with increased LDL cholesterol and triglyceride levels, possibly due to inhibition of inflammation [72,73]. Nonetheless, the increased cholesterol levels after treatment do not indicate increased atherogenicity as cholesterol quality and cholesterol transport, including HDL-C efflux capacity, may improve with treatment [73,74]. Increase of HDL-C level after antirheumatic treatment may also contribute to reduction in TCC as HDL-C carries many proteins that inhibit complement activation [75], and HDL-C can impair the cytolytic activity of TCC [27].

Cigarette smoking is supposed to enhance complement cleavage products, as it induces a pro-inflammatory environment specifically by generating complement factors C3a and C3b [76,77]. Nevertheless, in our study, there was no association between TCC and tobacco smoke, neither pre- nor post antirheumatic treatment. The results are in line with former study showing no change in TCC expression in sera exposed to tobacco smoke extract, despite signs of upstream complement activation [78]. Our patients were instructed not to smoke in at least twelve hours prior to examination, and it is unclear whether temporary smoking cessation affects outcomes.

The findings of this study have to be seen in lights of some limitations including the relatively small sample size and the observational design. The former may increase the risk of Type-II errors, and might lead to underestimation of real differences and associations. Moreover, it is not ethically appropriate to withhold treatment with beneficial effect from clinically eligible patients. The statistical approach utilized in our research paper also suffers from the limitation that multiple testing of longitudinal data amplifies the probability of a false-positive finding.

An advantage of our study is the comprehensive characterization of patient population and the design that makes it possible to compare the effect of the two antirheumatic treatment regimens on TCC levels in RA.

In conclusion, RA patients had elevated TCC, which decreased rapidly and sustainably with TNFi±MTX treatment during the 6-month period. Exaggerated complement activation due to chronic inflammation in RA, seems to be associated with endothelial dysfunction–the initial step in the pathogenesis of atherosclerosis. Our findings support further investigations to determine if the cardioprotective effects of antirheumatic drugs might be associated to ameliorating effects of TNFi on complement activation, and whether the complement system might be a target for therapy in RA.

Supporting information

S1 Fig. Scatterplots.

Changes in TCC with MTX monotherapy and TNFi±MTX treatment.

https://doi.org/10.1371/journal.pone.0264628.s001

(TIF)

S1 File. Stata file.

Stata file containing all data underlying the findings described in the present study.

https://doi.org/10.1371/journal.pone.0264628.s002

(DTA)

Acknowledgments

We thank all the patients who gave their voluntary consent to participate in the study. We thank all the medical staff involved in the study research and the administration of our hospital for their valuable contributions, especially to Research Laboratory, Nordland Hospital for handling lab procedures, and to Chevy Stubberud for assisting with finger plethysmography.

Citation: Nguyen THP, Hokstad I, Fagerland MW, Mollnes TE, Hollan I, Feinberg MW, et al. (2022) Antirheumatic therapy is associated with reduced complement activation in rheumatoid arthritis. PLoS ONE 17(2): e0264628. https://doi.org/10.1371/journal.pone.0264628

References

1. England BR, Thiele GM, Anderson DR, Mikuls TR. Increased cardiovascular risk in rheumatoid arthritis: mechanisms and implications. BMJ 2018;361:k1036. pmid:29685876

2. Nurmohamed MT, Heslinga M, Kitas GD. Cardiovascular comorbidity in rheumatic diseases. Nat. Rev. Rheumatol. 2015;11:693–704. pmid:26282082

3. Avina-Zubieta JA, Thomas J, Sadatsafavi M, Lehman AJ, Lacaille D. Risk of incident cardiovascular events in patients with rheumatoid arthritis: a meta-analysis of observational studies. Ann Rheum Dis. 2012; 2012 Sep;71(9):1524–9. pmid:22425941

4. Libby P. Role of Inflammation in Atherosclerosis Associated with Rheumatoid Arthritis. Am. J. Med. 2008;121(10): S21–S31. pmid:18926166

5. Geovanini GR and Libby P. Atherosclerosis and inflammation: overview and updates. Clin. Sci. 2018;132(12):1243–1252. pmid:29930142

6. Crowson CS, Rollefstad S, Ikdahl E, Kitas GD, van Riel PLCM, Gabriel SE et al. Impact of risk factors associated with cardiovascular outcomes in patients with rheumatoid arthritis. Ann Rheum Dis. 2018 January; 77(1): 48–54. pmid:28877868

7. Hollan I, Ronda N, Dessein P, Agewall S, Karpouzas G, Tamargo J et al. Lipid management in rheumatoid arthritis: a position paper of the Working Group on Cardiovascular Pharmacotherapy of the European Society of Cardiology. Eur Heart J Cardiovasc Pharmacother. 2020 Apr 1;6(2):104–114. pmid:31397840

8. Skeoch S, Bruce IN. Atherosclerosis in rheumatoid arthritis: is it all about inflammation? Nat Rev Rheumatol. 2015 Jul;11(7):390–400. pmid:25825281

9. Bordy R, Totoson P, Prati C, Marie C, Wendling D, Demougeot C. Microvascular endothelial dysfunction in rheumatoid arthritis. Nat Rev Rheumatol. 2018; 14:404–420. pmid:29855620

10. Dunkelberger JR, Song W-C. Complement and its role in innate and adaptive immune responses. Cell Research. 2010; 20:34–50. pmid:20010915

11. Ricklin D, Lambris JD. Complement in immune and inflammatory disorders: pathophysiological mechanisms. J Immunol. 2013 Apr 15;190(8):3831–8. pmid:23564577

12. Galindo-Izquierdo M, Alvarez JLP. Complement as a Therapeutic Target in Systemic Autoimmune Diseases. Cells. 2021 Jan 13;10(1):148. pmid:33451011

13. Holers M, Banda NK. Complement in the Initiation and Evolution of Rheumatoid Arthritis. Front. Immunol. 2018 May; 9:1057. pmid:29892280

14. Neumann E, Barnum SR, Tarner IH, Echols J, Fleck M, Judex M et al. Local Production of Complement Proteins in Rheumatoid Arthritis Synovium. Arthritis Rheum. 2002 Apr;46(4):934–45. pmid:11953970

15. Brodeur JP, Ruddy S, Schwartz LB, Moxley G. Synovial fluid levels of complement SC5b-9 and fragment Bb are elevated in patients with rheumatoid arthritis. Arthritis Rheum. 1991 Dec;34(12):1531–7. pmid:1747138

16. Konttinen YT, Ceponis A, Meri S, Vuorikoski A, Kortekangas P, Sorsa T, et al. Complement in acute and chronic arthritides: assessment of C3c, C9, and protectin (CD59) in synovial membrane. Ann Rheum Dis. 1996; 55(12):888–94. pmid:9014582

17. Bemis EA, Norris JM, Seifert J, Frazer-Abel A, Okamoto Y, Feser ML et al. Complement and its Environmental Determinants in the Progression of Human Rheumatoid Arthritis. Mol. Immunol. 2019; 112: 256–265. pmid:31207549

18. Corallini F, Bossi F, Gonelli A, Tripodo C, Castellino G, Mollnes TE et al. The soluble terminal complement complex (SC5b-9) up-regulates osteoprotegerin expression and release by endothelial cells: implications in rheumatoid arthritis. Rheumatology 2009; 48:293–298. pmid:19168833

19. Morgan B. P., Daniels R. H. & Williams B. D. Measurement of terminal complement complexes in rheumatoid arthritis. Clin. Exp. Immunol. 1988; 73(3), 473–478. pmid:3208454

20. Mollnes TE, Paus A. Complement activation in synovial fluid and tissue from patients with juvenile rheumatoid arthritis. Arthritis Rheum. 1986 Nov;29(11):1359–64. pmid:3778542

21. Mollnes TE, Lea T, Mellbye OJ, Pahle J, Grand O, Harboe M. Complement activation in rheumatoid arthritis evaluated by C3dg and the terminal complement complex. Arthritis Rheum. 1986 Jun;29(6):715–21. pmid:3718564

22. Lappegård KT, Garred P, Jonasson L, Espevik T, Aukrust P, Yndestad A. A vital role for complement in heart disease. Mol Immunol. 2014 Oct;61(2):126–34. pmid:25037633

23. Engelmann B, Massberg S. Thrombosis as an intravascular effector of innate immunity. Nat Rev Immunol. 2013 Jan;13(1):34–45. pmid:23222502

24. Hovland A, Jonasson L, Garred P, Arne Yndestad, Aukrust P, Lappegård K et al. The complement system and toll-like receptors as integrated players in the pathophysiology of atherosclerosis. Atherosclerosis. 2015;241 (2):480–494. pmid:26086357

25. Hansson G, Hermansson A. The immune system in atherosclerosis. Nat Immunol. 2011; 12:204–212. pmid:21321594

26. Weber C, Noels H. Atherosclerosis: current pathogenesis and therapeutic options. Nat Med. 2011 Nov;17(11):1410–22. pmid:22064431

27. Niyonzima N, Samstad EO, Aune MH, Ryan L, Bakke SS, Rokstad AM et al. Reconstituted High-Density Lipoprotein Attenuates Cholesterol Crystal-Induced Inflammatory Responses by Reducing Complement Activation. J Immunol. 2015 Jul 1;195(1):257–64. pmid:26026058

28. Shields KJ, Mollnes TE, Eidet JR, Mikkelsen K, Almdahl SM, Bottazzi B et al. Plasma complement and vascular complement deposition in patients with coronary artery disease with and without inflammatory rheumatic diseases. PLoS ONE. 2017; 2(3): e0174577. pmid:28362874

29. Hjeltnes G, Hollan I, Førre Ø, Wiik A, Lyberg T, Mikkelsen K et al. Serum levels of lipoprotein(a) and E-selectin are reduced in rheumatoid arthritis patients treated with methotrexate or methotrexate in combination with TNF-α-inhibitor. Clin Exp Rheumatol. May-Jun 2013;31(3):415–21. Epub 2013 Mar 4. pmid:23465067

30. Deyab G, Hokstad I, Whist JE, Småstuen MC, Agewall S, Lyberg T, et al. Anti-rheumatic treatment is not associated with reduction of pentraxin 3 in rheumatoid arthritis, psoriatic arthritis and ankylosing spondylitis. PLoS ONE 12(2): e0169830. pmid:28225768

31. Nguyen THP, Fagerland MW, Deyab G, Hjeltnes G, Hollan I, Feinberg MW, et al. (2021) Antirheumatic therapy is not associated with changes in circulating N-terminal pro-brain natriuretic peptide levels in patients with autoimmune arthritis. PLoS ONE 16(6): e0253793. pmid:34170978

32. Arnett FC, Edworthy SM, Bloch DA, McShane DJ, Fries JF, Cooper NS et al. The American Rheumatism Association 1987 revised criteria for the classification of rheumatoid arthritis. Arthritis Rheum. 1988 Mar;31(3):315–24. pmid:3358796

33. Smolen JS, Landewé RBM, Bijlsma JWJ, Burmester GR, Dougados M, Kerschbaumer A et al. EULAR recommendations for the management of rheumatoid arthritis with synthetic and biological disease-modifying antirheumatic drugs: 2019 update. Ann Rheum Dis. 2020 Jun;79(6):685–699. pmid:31969328

34. Bonetti PO, Barsness GW, Keelan PC, Schnell TI, Pumper GM, Kuvin JT et al. Enhanced external counterpulsation improves endothelial function in patients with symptomatic coronary artery disease. J Am Coll Cardiol. 2003;41(10):1761–8. pmid:12767662

35. Rozanski A, Qureshi E, Bauman M, Reed G, Pillar G, Diamond GA. Peripheral arterial responses to treadmill exercise among healthy subjects and atherosclerotic patients. Circulation 2001;103:2084–9. pmid:11319199

36. https://www.itamar-medical.com/pat-technology-peripheral-arterial-tone/.

37. Tanaka A, Tomiyama H, Maruhashi T, Matsuzawa Y, Miyoshi T, Kabutoya T et al. Physiological Diagnosis Criteria for Vascular Failure Committee.Physiological Diagnostic Criteria for Vascular Failure. Hypertension. 2018 Nov;72(5):1060–1071. pmid:30354826

38. Bonetti PO, Pumper GM, Higano ST, Holmes DR, Kuvin JT, Lerman A. Noninvasive identification of patients with early coronary atherosclerosis by assessment of digital reactive hyperemia. J Am Coll Cardiol. 2004 Dec; 44(11):2137–41. pmid:15582310

39. Bergseth G, Ludviksen JK, Kirschfink M, Giclas PC, Nilsson B, Mollnes TE. An international serum standard for application in assays to detect human complement activation products. Mol Immunol. 2013 Dec 15;56(3):232–9. pmid:23787367

40. Hokstad I, Deyab G, Wang Fagerland M, Lyberg T, Hjeltnes G, Førre Ø, et al. (2019) Tumor necrosis factor inhibitors are associated with reduced complement activation in spondylarthropathies: An observational study. PLoS ONE 14(7): e0220079. pmid:31335881

41. Ballanti E, Perricone C, di Muzio G, Kroegler B, Chimenti MS, Graceffa D et al. Role of the complement system in rheumatoid arthritis and psoriatic arthritis: Relationship with anti-TNF inhibitors. Autoimmun. Rev. 2011; 10(10): 617–623. pmid:21549221

42. Familian A, Voskuyl AE, van Mierlo GJ, Heijst HA, Twisk JWR, Dijkmans BAC et al. Infliximab treatment reduces complement activation in patients with rheumatoid arthritis. Ann Rheum Dis 2005; 64:1003–1008. pmid:15958758

43. Di Muzio G, Perricone C, Ballanti E, Kroegler B, Greco E, Noevll L, et al. Complement system and rheumatoid arthritis: relationships with autobodies, serological, clinic features and anti-TNF treatment. Int J Immunopathol Pharmacol. 2011; 24(2): 357–366. pmid:21658310

44. Qin X, Gao B. The complement system in liver diseases. Cell Mol Immunol. 2006; 3:333‐340. pmid:17092430

45. Zhou Z, Xu M-J, Gao B. Hepatocytes: a key cell type for innate immunity. Cell Mol Immunol. 2016; 13:301–315. pmid:26685902

46. Perissutti S, Tedesco F. Effect of cytokines on the secretion of the fifth and eighth complement components by HepG2 cells. Int J Clin Lab Res. 1994; 24:45–48. pmid:8180423

47. Perlmutter DH, Dinarello CA, Punsal PI, Colten HR. Cachectin/tumor necrosis factor regulates hepatic acute-phase gene expression. J Clin Invest 1986; 78:1349–54. pmid:2429991

48. McInnes I, Schett G. The Pathogenesis of Rheumatoid Arthritis. N Engl J Med. 2011 Dec 8;365(23):2205–19. pmid:22150039

49. Volanakis JE. Complement activation by C-reactive protein complexes. Ann N Y Acad Sci. 1982; 389:235–50. pmid:7046577

50. Molenaar ETH, Voskuyl AE, Familian A, van Mierlo GJ, Dijkmans BAC et al. Complement activation in patients with rheumatoid arthritis mediated in part by C-reactive protein. Rheumatol. 2009; 48:293–298. pmid:19168833

51. Pope JE, Choy EH. C-reactive protein and implications in rheumatoid arthritis and associated comorbidities. Semin Arthritis Rheum. 2021; 51(1): 219–229. pmid:33385862

52. Tanka T, Narazaki M, Kishimoto T. IL-6 in Inflammation, Immunity, and Disease. Cold Spring Harb Perspect Biol 2014;6:a016295. pmid:25190079

53. Eng GP, Bouchelouche P, Bartels EM, Bliddal H, Bendtzen K, Stoltenberg M. Anti-Drug Antibodies, Drug Levels, Interleukin-6 and Soluble TNF Receptors in Rheumatoid Arthritis Patients during the First 6 Months of Treatment with Adalimumab or Infliximab: A Descriptive Cohort Study. PLoS One. 2016 Sep 8;11(9):e0162316. pmid:27606615

54. Ridker PM. C-Reactive Protein: Eighty Years from Discovery to Emergence as a Major Risk Marker for Cardiovascular Disease. Clin Chem. 2009 Feb;55(2):209–15. pmid:19095723

55. Cutolo M, Seriolo B, Pizzorni C, Craviotto C, Sulli A. Methotrexate in psoriatic arthritis. Clin Exp Rheumatol. Nov-Dec 2002;20(6 Suppl 28):S76–80. pmid:12463453

56. Belinsky GS, Parke AL, Huang Q, Blanchard K, Jayadev S, Stoll R et al. The Contribution of Methotrexate Exposure and Host Factors on Transcriptional Variance in Human Liver. Toxicol Sci. 2007 Jun;97(2):582–94. pmid:17400583

57. Libby P. History of Discovery: Inflammation in Atherosclerosis. Arterioscler Thromb Vasc Biol. 2012 September; 32(9): 2045–2051. pmid:22895665

58. Bäck M, Yurdagul A Jr, Tabas I, Öörni K, Kovanen PT. Inflammation and its resolution in atherosclerosis: mediators and therapeutic opportunities. Nat. Rev. Cardiol. 2019; 16:389–406. pmid:30846875

59. Suresh R, Chandrasekaran P, Sutterwala FS, Mosser DM. Complement-mediated ‘bystander’ damage initiates host NLRP3 inflammasome activation. J Cell Sci. 2016 May 1;129(9):1928–39. pmid:27006116

60. Viedt C, Hänsch G-M, Brandes RP, Kübler W, Kreuzer J. The terminal complement complex C5b-9 stimulates interleukin-6 production in human smooth-muscle cells through activation of transcription factors NF-κB and AP-1. FASEB J. 2000 Dec;14(15):2370–2. pmid:11024008

61. Hertle E, van Greevenbroek MMJ, Arts ICW, van der Kallen CJH, Feskens EJM, Schalkwijk CG et al. Complement activation products C5a and sC5b-9 are associated with low-grade inflammation and endothelial dysfunction, but not with atherosclerosis in a cross-sectional analysis: The CODAM study. Int. J. Cardiol. 2014,174(2):400–403. pmid:24794956

62. Corallini F, Bossi F, Gonelli A, Tripodo C, Castellino G, Mollnes TE et al. The soluble terminal complement complex (SC5b-9) up-regulates osteoprotegerin expression and release by endothelial cells: implications in rheumatoid arthritis. Rheumatology 2009; 48:293–298. pmid:19168833

63. Hjeltnes G, Hollan I, Førre Ø, Wiik A, Lyberg T, Mikkelsen K et al. Endothelial function improves within 6 weeks of treatment with methotrexate or methotrexate in combination with a TNF-α inhibitor in rheumatoid arthritis patients. Scand J Rheumatol. 2012 May;41(3):240–2. pmid:22401496

64. Deyab G, Hokstad I, Whist JE, Smastuen MC, Agewall S, Lyberg T et al. Methotrexate and anti-tumor necrosis factor treatment improves endothelial function in patients with inflammatory arthritis. Arthritis Res. Ther. 2017 Oct 17;19(1):232. pmid:29041979

65. Deanfield J, Donald A, Ferri C, Giannattasio C, Halcox J, Halligan S, et al. Endothelial function and dysfunction. Part I: Methodological issues for assessment in the different vascular beds: a statement by the Working Group on Endothelin and Endothelial Factors of the European Society of Hypertension. J Hypertens. 2005 Jan;23(1):7–17. pmid:15643116

66. Corretti MC, Anderson TJ, Benjamin EJ, Celermajer D, Charbonneau F, Creager MA. Guidelines for the ultrasound assessment of endothelial-dependent flow-mediated vasodilation of the brachial artery: a report of the International Brachial Artery Reactivity Task Force. J Am Coll Cardiol. 2002 Jan 16;39(2):257–65. pmid:11788217

67. Martin EA, Nelson RE, Felmlee-Devine MD, Brown TE, Lerman A. Comparing EndoPAT and BIOPAC measurement of vascular responses to mental stress. Cell Biochem Funct. 2011 Jun;29(4):272–8. pmid:21671245

68. Bo’ CD, Campolo J, Porrini M, Fracassetti D, Parolini M, Klimis-Zacas D et al. Acute cigarette smoking impairs microvascular function in young moderate smokers: A potential model for studying vasoactive properties of food bioactives. PharmaNutrition. 2014;2(1):1–7.

69. Title LM, Cummings PM, Giddens K, Nassar BA. Oral glucose loading acutely attenuates endothelium-dependent vasodilation in healthy adults without diabetes: an effect prevented by vitamins C and E. J Am Coll Cardiol. 2000 Dec;36(7):2185–91. pmid:11127459

70. Pasqui AL, Puccetti L, Bova G, Di Renzo M, Bruni F, Pastorelli M, et al. Relationship between serum complement and different lipid disorders. Clin Exp Med. 2002 May;2(1):33–8. pmid:12049187

71. Charles-Schoeman C, Lee YY, Grijalva V, Amjadi S, FitzGerald J, Ranganath VK et al. Cholesterol efflux by high density lipoproteins is impaired in patients with active rheumatoid arthritis. Ann Rheum Dis 2012;71:1157–1162. pmid:22267330

72. Navarro-Millán I, Charles-Schoeman C, Yang S, Bathon JM, Bridges SL Jr, Chen L et al. Changes in lipoproteins associated with methotrexate or combination therapy in early rheumatoid arthritis: results from the treatment of early rheumatoid arthritis trial. Arthritis Rheum. 2013 June; 65(6): 1430–1438. pmid:23460074

73. Myasoedova E. Lipids and lipid changes with synthetic and biologic disease modifying antirheumatic drug therapy in rheumatoid arthritis: implications for cardiovascular risk. Curr Opin Rheumatol 2017;29(3):277–284. pmid:28207495

74. Liao KP, Playford MP, Frits M, Coblyn JS, Iannaccone C, Weinblatt ME et al. The association between reduction in inflammation and changes in lipoprotein levels and HDL cholesterol efflux capacity in rheumatoid arthritis. J Am Heart Assoc. 2015;30;4(2):e001588. pmid:25637346

75. Gordon SM, Remaley AT. High density lipoproteins are modulators of protease activity: Implications in inflammation, complement activation, and atherothrombosis. Atherosclerosis. 2017 April; 259: 104–113. pmid:28242049

76. Wang L, Kondo N, Cano M, Ebrahimi K, Yoshida T, Barnett PB et al. Nrf2 Signaling Modulates Cigarette Smoke Induced Complement Activation in Retinal Pigmented Epithelial Cells. Radic Biol Med. 2014 May; 70: 155–166. pmid:24440594

77. Robbins RA, Nelson KJ, Gossman GL, Koyama S, Rennard SI. Complement activation by cigarette smoke. Am J Physiol Cell Mol Physiol. 1991 Apr; 260(4): L254–9. pmid:1902064

78. Yin W, Ghebrehiwet B, Weksler B, Peerschke EIB. Regulated complement deposition on the surface of human endothelial cells: effect of tobacco smoke and shear stress. Thromb Res. 2008;122(2):221–8. pmid:18166221

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© 2022 Nguyen et al. This is an open access article distributed under the terms of the Creative Commons Attribution License: http://creativecommons.org/licenses/by/4.0/ (the “License”), which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited. Notwithstanding the ProQuest Terms and Conditions, you may use this content in accordance with the terms of the License.

Abstract

Background

The complement system plays an important role in pathophysiology of cardiovascular disease (CVD), and might be involved in accelerated atherogenesis in rheumatoid arthritis (RA). The role of complement activation in response to treatment, and in development of premature CVD in RA, is limited. Therefore, we examined the effects of methotrexate (MTX) and tumor necrosis factor inhibitors (TNFi) on complement activation using soluble terminal complement complex (TCC) levels in RA; and assessed associations between TCC and inflammatory and cardiovascular biomarkers.

Methods

We assessed 64 RA patients starting with MTX monotherapy (n = 34) or TNFi with or without MTX co-medication (TNFi±MTX, n = 30). ELISA was used to measure TCC in EDTA plasma. The patients were examined at baseline, after 6 weeks and 6 months of treatment.

Results

Median TCC was 1.10 CAU/mL, and 57 (89%) patients had TCC above the estimated upper reference limit (<0.70). Compared to baseline, TCC levels were significantly lower at 6-week visit (0.85 CAU/mL, p<0.0001), without significant differences between the two treatment regimens. Notably, sustained reduction in TCC was only achieved after 6 months on TNFi±MTX (0.80 CAU/mL, p = 0.006). Reductions in TCC after treatment were related to decreased C-reactive protein (CRP), erythrocyte sedimentation rate (ESR) and interleukin 6, and increased levels of total, high and low-density lipoprotein cholesterol. Similarly, baseline TCC was significantly related to baseline CRP, ESR and interleukin 6. Patients with endothelial dysfunction had higher baseline TCC than those without (median 1.4 versus 1.0 CAU/mL, p = 0.023).

Conclusions

Patients with active RA had elevated TCC, indicating increased complement activation. TCC decreased with antirheumatic treatment already after 6 weeks. However, only treatment with TNFi±MTX led to sustained reduction in TCC during the 6-month follow-up period. RA patients with endothelial dysfunction had higher baseline TCC compared to those without, possibly reflecting involvement of complement in the atherosclerotic process in RA.

Details

Title
Antirheumatic therapy is associated with reduced complement activation in rheumatoid arthritis
Author
Nguyen, Thao H P; Hokstad, Ingrid; Morten Wang Fagerland; Mollnes, Tom Eirik; Hollan, Ivana; Feinberg, Mark W; Hjeltnes, Gunnbjørg; Eilertsen, Gro Ø; Mikkelsen, Knut; Agewall, Stefan
First page
e0264628
Section
Research Article
Publication year
2022
Publication date
Feb 2022
Publisher
Public Library of Science
e-ISSN
19326203
Source type
Scholarly Journal
Language of publication
English
DOI
https://doi.org/10.1371/journal.pone.0264628
ProQuest document ID
2633248820
Copyright
© 2022 Nguyen et al. This is an open access article distributed under the terms of the Creative Commons Attribution License: http://creativecommons.org/licenses/by/4.0/ (the “License”), which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited. Notwithstanding the ProQuest Terms and Conditions, you may use this content in accordance with the terms of the License.