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Eduardo Gómez-Bañuelos 1 and Beatriz Teresita Martín-Márquez 1 and Erika Aurora Martínez-García 1,2 and Mauricio Figueroa-Sanchez 3 and Lourdes Nuñez-Atahualpa 3 and Alberto Daniel Rocha-Muñoz 1 and Pedro Ernesto Sánchez-Hernández 4 and Rosa Elena Navarro-Hernandez 1 and Perla Monserrat Madrigal-Ruiz 1 and Adan Alberto Saldaña-Millan 1 and Sergio Duran-Barragan 1 and Laura Gonzalez-Lopez 5 and Jorge Ivan Gamez-Nava 6 and Mónica Vázquez-Del Mercado 1,7

Academic Editor:Miguel A. González-Gay

1, Instituto de Investigación en Reumatología y del Sistema Musculo Esquelético, Centro Universitario de Ciencias de la Salud, Benemérita Universidad de Guadalajara, Sierra Mojada No. 950, Colonia Independencia, 44340 Guadalajara, JAL, Mexico
2, Departamento de Fisiología, Centro Universitario de Ciencias de la Salud, Benemérita Universidad de Guadalajara, Sierra Mojada No. 950, Colonia Independencia, 44340 Guadalajara, JAL, Mexico
3, Servivio de Radiología e Imagen, Hospital Civil de Guadalajara "Fray Antonio Alcalde", Benemérita Universidad de Guadalajara, Hospital No. 278, 44280 Guadalajara, JAL, Mexico
4, Laboratorio de Inmunología, Departamento de Fisiología, Centro Universitario de Ciencias de la Salud, Benemérita Universidad de Guadalajara, Sierra Mojada No. 950, Colonia Independencia, 44340 Guadalajara, JAL, Mexico
5, Departamento de Medicina Interna-Reumatología, Hospital General Regional No. 110, Instituto Mexicano del Seguro Social, Circunvalación Oblatos No. 2212, Colonia Oblatos, 44700 Guadalajara, JAL, Mexico
6, Unidad Médica de Alta Especialidad, Centro Médico Nacional de Occidente, Instituto Mexicano del Seguro Social, Belisario Domínguez No. 1000, Independencia Oriente, 44340 Guadalajara, JAL, Mexico
7, Servicio de Reumatología, Hospital Civil "Dr. Juan I. Menchaca", Benemérita Universidad de Guadalajara, Salvador de Quevedo No. 750, 44100 Guadalajara, JAL, Mexico

Received 20 March 2014; Revised 13 May 2014; Accepted 13 May 2014; 9 June 2014

This is an open access article distributed under the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

1. Introduction

Rheumatoid arthritis (RA) is a chronic autoimmune disease with systemic complications and early cardiovascular death [1]. RA patients are prone to develop atherosclerosis at a relatively young age.

Atherosclerosis and inflammation in RA share several mechanisms in their pathogenesis including proinflammatory cytokine expression, infectious agents, dyslipidemia, and autoantibodies [2-8].

Type B scavenger receptors (SR), like CD36, are molecules possibly involved in the pathogenesis of atherosclerosis. During atherogenesis, blood monocytes are recruited into the intima and subintima layers of blood vessels; were they internalize oxidized low density lipoproteins (ox-LDL) through SR (CD36). This process results in the activation of monocytes and their differentiation into macrophages and foam cells. As a consequence, matrix metalloproteinases, proinflammatory cytokines, and chemoattractants enhance inflammatory infiltrates and vascular remodeling [9, 10]. CD36 has a critical role in the atherosclerotic plaque development [11-14]. However, their role in cardiovascular complications of RA has not been studied.

The aim of this study was to evaluate the association between membrane expressions of CD36 in peripheral blood mononuclear cells (PBMC) with carotid intima-media thickness (cIMT) in patients with RA without known traditional cardiovascular risk factors.

2. Methods

2.1. Patients

We recruited RA patients that met ACR 1987 criteria [15], from the Hospital Civil "Dr. Juan I. Menchaca" at Guadalajara, Jalisco, Mexico. Patients with known cardiovascular risk factors such as history of myocardiopathy, hypertension, diabetes mellitus, hyperlipidemia, malignancy, thyroid, renal or hepatic disease, smokers and steroid treatment >10 mg/day were excluded.

A structured questionnaire was applied to each patient to evaluate demographical and clinical variables. Physical examination, joint assessment, and venous blood drawn were performed at the visit.

2.2. Clinical Assessment

Disease activity was evaluated using Disease Activity Score 28 (DAS28) and C-reactive protein (CRP).

2.3. cIMT

It was assessed according to the recommendations defined by the Mannheim carotid intima-media thickness and plaque consensus (2004-2006-2011) [16] by a single operator using a high-resolution B-mode ultrasound (Philips Saronno, Italy) with a 9 MHz transducer. Two segments from the common carotid artery (CCA), one from the carotid bifurcation (BF), and two from the internal carotid artery (ICA) were evaluated. Mean cIMT values were calculated for each segment. Patients were classified according to the cIMT with a cut-off point of 0.6 mm.

2.4. Laboratory Assessment

Serum was obtained by centrifugation of whole blood at 2,000 rpm for 15 minutes; aliquots with serum were stored at -70°C for no longer than 6 months. Erythrocyte sedimentation rate (ESR) was measured using Wintrobe method and CRP by immunoturbidimetry (assay range 0.3-161 mg/L, Randox laboratories limited); total cholesterol (TC), triglycerides (Tg), high density lipoprotein cholesterol (HDL-c), and low density lipoprotein cholesterol (LDL-c) were measured by routine methods. Cardiovascular risk ratio was calculated using the atherogenic index of plasma (AIP) which was defined as TC/HDL-c. Anticyclic citrullinated peptide (CCP) antibodies (intra-assay variation coefficient (VC) < 9% and interassay VC < 11%, Axis-Shield Diagnostics Ltd.), serum interleukin (IL)-6 (intra-assay VC 5.1%-7.7% and interassay VC 6.5%-9.3%, Invitrogen), tumor necrosis factor (TNF)α (intra-assay VC 4.2%-5.2% and interassay VC 4.6%-7.4%, R&D Systems), and ox-LDL (intra-assay VC 3.9%-5.7% and interassay VC 9.0%-11.0%, ALPCO Diagnostics) were measured by enzyme-linked immunosorbent assay (ELISA).

The flow cytometric analysis was performed using fluorescein isothiocyanate- (FITC-) conjugated mouse monoclonal antibodies against human CD36 and PE conjugated anti-human CD14 (BioLegend). PBMC were obtained by density gradient centrifugation using a lymphocyte separation solution. The cells were washed twice with phosphate buffered saline (PBS) and fixed with 1% paraformaldehyde for 20 minutes at 4°C. After being washed with PBS, 5×¹⁰⁶ cells in 50 μ L PBS were incubated with FITC or PE-conjugated monoclonal antibodies for 30 minutes at 4°C. The cells were then washed twice before being assayed with a flow cytometer (Beckman Coulter, Epic XL, Miami, FL, USA) and analyzed with the software WinMDI 2.9.

2.5. Statistical Analyses

Values are presented as mean ± standard deviation (SD) and percentages as appropriate. Between-group differences were estimated by independent-sample Student's t -test. Chi-square test (or Fisher's exact test) was used to compare categorical variables. Spearman's correlation coefficient was calculated for cIMT, DAS28, CRP, anti-CCP, IL-6, and TNFα . All data were analyzed using SPSS 18.0 software (SPSS Inc., Chicago, IL) and replicated using the software Stata 12.0 (StataCorp LP, Texas, USA), considering a two-tailed level of P<0.05 statistically significant.

2.6. Ethics

Protocol was approved by the IRB committee (register number 1068/10) of the Hospital Civil "Dr. Juan I. Menchaca" of the Benemérita Universidad de Guadalajara.

3. Results

Sixty-seven patients were included in this study; 60 (89.5%) were female, with a mean (SD) age of 44.2 (11.9) years old; 29 (43.28%) had evidence of increased cIMT. Table 1 shows the comparison of RA subgroups with and without increased cIMT. No statistical differences in age, disease duration, and disease activity were observed between higher and lower cIMT groups. The increased cIMT group (>0.6 mm) showed higher serum levels of TC (P<0.001 ), Tg (P=0.002 ), ox-LDL (P<0.001 ), and AIP (P<0.001 ) and lower serum levels of HDL-c (P<0.001 ) compared with the cIMT group (<0.6 mm). Serum levels of CRP, TNFα , IL-6, and anti-CCP also were higher in the increased cIMT group (P<0.001 ).

Table 1: Characteristics and comparison of RA subgroups with and without increased cIMT.

RA: rheumatoid arthritis; cIMT: carotid intima-media thickness; DAS28: disease activity score; TC: total cholesterol; Tg: triglycerides; HDL-c: high density lipoprotein cholesterol; LDL-c: low density lipoprotein cholesterol; VLDL-c: very low density lipoprotein cholesterol; AIP: atherogenic index of plasma; ESR: erythrocyte sedimentation rate; RF: rheumatoid factor; CRP: C-reactive protein; TNFα : tumor necrosis factor alpha; IL: interleukin; anti-CCP: anticyclic citrullinated peptides; MFI: mean fluorescence intensity; DMARDs: disease-modifying antirheumatic drugs.

Qualitative variables are expressed as frequencies (%); quantitative variables are expressed as means ± standard deviations (SD). Comparisons between proportions were computed using Chi-square or Fisher exact test. Comparisons between medians were computed with unpaired Student's t -test.

3.1. CD36 PBMC Membrane Expression

RA patients with increased cIMT showed lower levels of CD36 compared with no increased cIMT (67.09 ± 27.50 versus 170.43 ± 38.80, P<0.001 ).

The PBMC membrane expression of CD36 MFI was significantly lower in patients with moderate and high disease activity (n=22 , 64.31 ± 16.72), when compared to patients with low disease activity (n=11 , 129.78 ± 13.73) or in remission (n=34 , 158.2 ± 13.66) (P<0.05 ).

3.2. Correlations Coefficients between cIMT, Clinical, and Laboratory Characteristics of RA Patients

Correlation coefficients between cIMT and characteristics of RA patients are shown in Table 2. cIMT was negatively correlated with CD36 MFI and HDL-c and positively correlated with age, TC, Tg, AIP, anti-CCP, TNFα , IL-6, CRP, and ox-LDL.

Table 2: Correlation coefficients between cIMT and characteristics of the groups evaluated.

cIMT: carotid intima-media thickness; RA: rheumatoid arthritis; DAS28: disease activity score; TC: total cholesterol; Tg: triglycerides; HDL-c: high density lipoprotein cholesterol; LDL-c: low density lipoprotein cholesterol; VLDL-c: very low density lipoprotein cholesterol; AIP: atherogenic index of plasma; ESR: erythrocyte sedimentation rate; RF: rheumatoid factor; CRP: C-reactive protein; TNFα : tumor necrosis factor alpha; IL-6: interleukin 6; anti-CCP: anticyclic citrullinated peptide antibodies; MFI: mean fluorescence intensity. Spearman r test.

Figure 1 showed a negative correlation between CD36 MFI with TNFα (r=-0.729 , P<0.001 ) and IL-6 (r=-0.822 , P<0.001 ). In data not shown, we observed a negative correlation of CD36 MFI with ox-LDL (r=-0.841 , P<0.001 ).

Figure 1: Correlation between serum TNFα , IL-6, and CD36 MFI.

[figure omitted; refer to PDF]

4. Discussion

In this study, we showed that RA patients with subclinical atherosclerosis showed low membrane expression of CD36 in PBMC and increased serum proinflammatory cytokines (Table 1). The CD36 PBMC membrane expression was negatively correlated with cIMT, ox-LDL, TNFα , and IL-6 (data not shown). We described a positive correlation between age, TC, Tg, ox-LDL, AIP, CRP, TNFα , IL-6, and anti-CCP antibodies with cIMT (Table 2).

In endothelial cell cultures exposed to IL-6 and TNFα , upregulation of the scavengers receptors- (SR-) A and ox-LDL receptor- (LOX-) 1 was shown but not CD36 expression. Endothelial cells stimulated with human sera rich in IL-6 and TNFα from RA patients; the CD36 expression increased and was not modified by IL-6 or TNFα antagonists. This suggests that a different factor present in the serum of these patients, like ox-LDL, may be responsible for the upregulation of CD36 [17].

TNFα promotes atherosclerosis through the inhibition of cholesterol efflux, favoring the cholesterol uptake by CD36 and other SR via protein kinase pathway. In THP-1 cells in the presence of ox-LDL, TNFα impaired the cholesterol efflux by downregulation of ATP-binding cassette (ABCA) proteins [18].

Boyer et al. showed the downregulation of membrane expression and mRNA levels of CD36 in culture of fresh PBMC from healthy donors in the presence of human recombinant TNFα . In other experiment incubating PBMC with a humanized TNFα blocker (Adalimumab), the membrane and mRNA CD36 increased [19]. The authors concluded that different pathways were involved in the regulation of CD36. When TNFα was used, the signaling was mediated by a reduction in activated peroxisome proliferator-activated receptor gamma, whereas Adalimumab increased CD36 through redox signaling.

In our report, the membrane CD36 in PBMC was decreased in RA patients with higher cIMT; besides, a negative correlation between TNFα and membrane CD36 MFI was found. These support the findings observed in endothelial cells and PMBC cultures reported by Boyer et al. [19]. However, these results must be corroborated by further studies using similar approaches as described before.

In our patients, another possible explanation for the low levels of CD36 might be the proteolytical cleavage by ADAM17, which might result in more soluble CD36 [20]. It has been reported the protective role of the CD36 polymorphism, G573A, in plaque thickness in patients with early coronary artery disease [21].

In a more detailed analysis of our results, we looked for the influence of disease duration and treatment. We found that, RA patients with normal cIMT had longer disease duration and lower levels of TNFα and IL-6 (Table 1) probably due to the benefit of prolonged use of antirheumatic drugs in the prevention of subclinical atherosclerosis [22]. In vitro studies using methotrexate (MTX) favor the cholesterol efflux through activation of adenosine A2 receptor, which in turn prevents the foam cell differentiation and atherosclerosis plaque formation [23, 24]. MTX might downregulate serum TNFα in RA [25]. A large study that enrolled more than 8,000 patients using synthetic DMARDS compared with anti-TNFα users (11,000 approximately) showed a reduction in cardiovascular risk in both groups, even though the reduction was greater in the anti-TNFα treated patients [26, 27].

Based on our results, low PBMC CD36 membrane expression showed a negative correlation with cIMT, ox-LDL, TNFα , IL-6, and DAS28. From the clinical standpoint, the interaction between these factors might reflect the importance of CD36 in the development of atherosclerosis in RA.

5. Conclusion

RA patients with subclinical atherosclerosis showed low membrane expression of CD36 in PBMC and increased serum proinflammatory cytokines. Translation of the results from these studies to the clinical field is difficult since the functional role of CD36 depends on the target cell. Further studies are needed to validate our findings and clarify the downregulation of CD36 in RA.

Acknowledgment

The authors thank Professor Minoru Satoh, M.D. and Ph.D., for reviewing this paper.

Conflict of Interests

The authors declare that they do not have conflict of interests.