Antibodies against specific extractable nuclear antigens (ENAs) as diagnostic and prognostic tools and inducers of a profibrotic phenotype in cultured human skin fibroblasts: are they functional?

被引:17
|
作者
Corallo, Claudio [1 ]
Cheleschi, Sara [2 ]
Cutolo, Maurizio [3 ,4 ]
Soldano, Stefano [3 ,4 ]
Fioravanti, Antonella [2 ]
Volpi, Nila [2 ]
Franci, Daniela [1 ]
Nuti, Ranuccio [1 ]
Giordano, Nicola [1 ]
机构
[1] Univ Siena, Dept Med Surg & Neurosci, Scleroderma Unit, Siena, Italy
[2] Univ Siena, Dept Med Surg & Neurosci, Rheumatol Unit, Siena, Italy
[3] Univ Genoa, Res Lab, Genoa, Italy
[4] Univ Genoa, Dept Internal Med, Acad Div Clin Rheumatol, Genoa, Italy
关键词
Systemic sclerosis; Fibrosis; Autoantibodies; Fibroblasts; Centromeric protein B; Topoisomerase I; ANTIENDOTHELIAL CELL ANTIBODIES; TOPOISOMERASE-I AUTOANTIBODIES; 2013 CLASSIFICATION CRITERIA; SYSTEMIC-SCLEROSIS; RHEUMATOLOGY/EUROPEAN LEAGUE; ANTINUCLEAR ANTIBODIES; AMERICAN-COLLEGE; INVOLVEMENT; BINDING;
D O I
10.1186/s13075-019-1931-x
中图分类号
R5 [内科学];
学科分类号
1002 ; 100201 ;
摘要
BackgroundThe importance of systemic sclerosis (SSc) autoantibodies for diagnosis has become recognized by their incorporation into the 2013 ACR/EULAR classification criteria. Clear prognostic and phenotypic associations with cutaneous subtype and internal organ involvement have been also described. However, little is known about the potential of autoantibodies to exert a direct pathogenic role in SSc. The aim of the study is to assess the pathogenic capacity of anti-DNA-topoisomerase I (anti-Topo-I) and anti-centromeric protein B (anti-Cenp-B) autoantibodies to induce pro-fibrotic markers in dermal fibroblasts.MethodsDermal fibroblasts were isolated from unaffected and affected skin samples of (n=10) limited cutaneous SSc (LcSSc) patients, from affected skin samples of diffuse cutaneous (DcSSc) patients (n=10) and from healthy subjects (n=20). Fibroblasts were stimulated with anti-Topo-I, anti-Cenp-B IgGs, and control IgGs in ratios 1:100 and 1:200 for 24h. Cells were also incubated with 10% SSc anti-Topo-I+ and anti-Cenp-B+ whole serum and with 10% control serum for 24h. Viability was assessed by MTT test, while apoptosis was assessed by flow cytometry. Activation of pro-fibrotic genes ACTA2, COL1A1, and TAGLN was evaluated by quantitative real-time PCR (qPCR), while the respective protein levels alpha-smooth-muscle actin (-SMA), type-I-collagen (Col-I), and transgelin (SM22) were assessed by immunocytochemistry (ICC).ResultsMTT showed that anti-Cenp-B/anti-Topo-I IgGs and anti-Cenp-B+/anti-Topo-I+ sera reduced viability (in a dilution-dependent manner for IgGs) for all the fibroblast populations. Apoptosis is induced in unaffected LcSSc and control fibroblasts, while affected LcSSc/DcSSc fibroblasts showed apoptosis resistance. Basal mRNA (ACTA2, COL1A1, and TAGLN) and protein (-SMA, Col-1, and SM22) levels were higher in affected LcSSc/DcSSc fibroblasts compared to LcSSc unaffected and to control ones. Stimulation with anti-Cenp-B/anti-Topo-I IgGs and with anti-Cenp-B+/anti-Topo-I+ sera showed a better induction in unaffected LcSSc and control fibroblasts. However, a statistically significant increase of all pro-fibrotic markers is reported also in affected LcSSc/DcSSc fibroblasts upon stimulation with both IgGs and sera.ConclusionsThis study suggests a pathogenic role of SSc-specific autoantibodies to directly induce pro-fibrotic activation in human dermal fibroblasts. Therefore, besides the diagnostic and prognostic use of those autoantibodies, these data might further justify the importance of immunosuppressive drugs in the early stages of the autoimmune disease, including SSc.
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页数:11
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