To the Editor:
In the past several years, adipokines have gained a lot of attention in the field of rheumatic diseases1. Rheumatoid arthritis (RA), for example, is associated with an altered production of adipokines1, and there is some evidence of involvement of adipokines in the pathophysiology of RA as suggested by in vitro1 and in vivo data2,3. The term “adipokines” was originally used to describe cytokine-like factors secreted by adipose tissue, but it turned out that many adipokines are also produced at other sites including the joints1,4,5, where they might have an influence on effector cells of RA or osteoarthritis (OA) pathophysiology.
As an adipokine, omentin was first found in omental adipose tissue from patients with Crohn disease6. Before this, it was identified as a secretory glycoprotein able to bind to galactofuranosyl residue on various microorganisms, suggesting a function in immune recognition of certain pathogens. It has also been described as a lactoferrin-binding protein with lactoferrin being a protein with multiple immunological functions. Omentin is highly abundant in human plasma6. It displayed antiinflammatory and antiatherogenic properties in obese patients7 and is negatively associated with inflammatory bowel disease (IBD)6,8 and metabolic syndrome9. Omentin levels in the synovial fluid (SF) of patients with RA were lower than in patients with OA5, while omentin serum levels were elevated in children with juvenile idiopathic arthritis compared with healthy controls and positively associated with the presence and number of active joints10.
Based on these previous findings, we decided to examine omentin expression in the synovium of patients with RA and OA. Synovial tissue samples obtained from patients with RA (n = 12) and OA (n = 10) undergoing joint surgery were analyzed immunohistochemically with a specific antiomentin antibody to determine the synovial omentin expression pattern. Immunohistochemical staining revealed omentin expression in RA and OA synovium, especially within the lining layer and vessel walls (Figure 1), and the same expression pattern for RA (Figure 1A and Figure 1B) and OA synovium (Figure 1C and Figure 1D). This similar expression pattern may also appear because synovial biopsies were from patients with late- or endstage RA or OA.
The presence of omentin in SF5 and synovial tissue led us to the hypothesis that this adipokine may also be involved in the pathogenesis of RA. Therefore, we analyzed the effects of omentin on the following key cells of RA pathophysiology: human synovial fibroblasts (n = 7), macrovascular endothelial cells (EC) from varicose veins (n = 2), microvascular human umbilical artery EC (n = 1), lymphocytes and monocytes from human blood (n = 1), as well as chondrocytes from human cartilage (n = 1). Because it had previously been shown that within the joint adipokines are particularly expressed by rheumatoid arthritis synovial fibroblasts (RASF)1, which can invade and destroy articular cartilage and subchondral bone, we focused our study on this cell type and started our analyses with RASF. All cell types used were stimulated in vitro with 500 ng/ml omentin (BioVendor) for 15 h. We first screened for potential changes in gene expressions induced by omentin in RASF using Affymetrix microarrays (n = 1; human genome U133A oligonucleotide probe microarrays, Affymetrix) and antibody arrays (n = 1; Human Chemokine Antibody Array I kit, custom human cytokine antibody array, RayBiotech). The array analysis resulted in a small number of genes or proteins showing limited up/downregulation by omentin in RASF (maximum upregulation: 13.1-fold, maximum downregulation: −13.9-fold; Table 1). However, the differential expression could not be confirmed for the genes selected for verification at mRNA level by real-time PCR or at protein level by ELISA (Table 1). For the other cell types, appropriate variables were analyzed by real-time PCR or ELISA; interleukin (IL)-6 was quantified for all cell types. Additionally, the following factors were determined in selected cell types: IL-8 for lymphocytes and monocytes; tumor necrosis factor-α only for lymphocytes; vascular endothelial growth factor and vascular cell adhesion molecule 1 for EC; and aggrecan, cartilage oligomeric matrix protein, and matrix metalloprotease 3 for chondrocytes. Interestingly, none of these factors were changed by omentin stimulation. Of note, the small sample sizes, which were not extended because of the negative characteristic of the results, may be a limitation of our study.
Although omentin is expressed in RA and OA synovium and present in SF, it has no or limited effects on central effector cells of RA pathophysiology, in contrast to the effects observed with other adipokines1,4. Our data suggest that the potentially antiinflammatory effect of omentin in diseases such as obesity7 and IBD8 does not occur in RA and OA, at least regarding the evaluated cell types.
Footnotes
Supported by the German Society for Rheumatology (Deutsche Gesellschaft für Rheumatologie).
REFERENCES
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