Pathological autoantibody internalisation in myositis

医学 自身抗体 肌炎 转录组 核糖核酸 病理 免疫学 生物 抗体 基因 基因表达 遗传学
作者
Iago Pinal‐Fernandez,Sandra Muñoz-Braceras,María Casal-Domínguez,Katherine Pak,Jiram Torres-Ruíz,Jon Musai,Stefania Dell’Orso,Faiza Naz,Shamima Islam,Gustavo Gutierrez-Cruz,Maria‐Dolores Cano,Ana Matas-García,Joan Padrosa,Ester Tobías-Baraja,Glòria Garrabou,Ibán Aldecoa,Gerard Espinosa,Carmen Pilar Simeón‐Aznar,Alfredo Guillén‐Del‐Castillo,Albert Gil‐Vila,Ernesto Trallero‐Araguás,Lisa Christopher‐Stine,Thomas E. Lloyd,Teerin Liewluck,Elie Naddaf,Werner Stenzel,Steven A. Greenberg,Josep María Grau,Albert Selva-O’Callaghan,José C. Milisenda,Andrew L. Mammen
出处
期刊:Annals of the Rheumatic Diseases [BMJ]
卷期号:: ard-225773 被引量:1
标识
DOI:10.1136/ard-2024-225773
摘要

Objectives Autoantibodies targeting intracellular proteins are common in various autoimmune diseases. In the context of myositis, the pathologic significance of these autoantibodies has been questioned due to the assumption that autoantibodies cannot enter living muscle cells. This study aims to investigate the validity of this assumption. Methods Confocal immunofluorescence microscopy was employed to localise antibodies and other proteins of interest in myositis muscle biopsies. Bulk RNA sequencing was used to examine the transcriptomic profiles of 669 samples, including those from patients with myositis, disease controls and healthy controls. Additionally, antibodies from myositis patients were introduced into cultured myoblasts through electroporation, and their transcriptomic profiles were analysed using RNA sequencing. Results In patients with myositis autoantibodies, antibodies accumulated inside myofibres in the same subcellular compartment as the autoantigen. Bulk RNA sequencing revealed that muscle biopsies from patients with autoantibodies targeting transcriptional regulators exhibited transcriptomic patterns consistent with dysfunction of the autoantigen. For instance, in muscle biopsies from patients with anti-PM/Scl autoantibodies recognising components of the nuclear RNA exosome complex, an accumulation of divergent transcripts and long non-coding RNAs was observed; these RNA forms are typically degraded by the nuclear RNA exosome complex. Introducing patient antibodies into cultured muscle cells recapitulated the transcriptomic effects observed in human disease. Further supporting evidence suggested that myositis autoantibodies recognising other autoantigens may also disrupt the function of their targets. Conclusions This study demonstrates that, in myositis, autoantibodies are internalised into living cells, causing biological effects consistent with the disrupted function of their autoantigen.
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