Author: Wang, Mengyan; Liu, Mengru; Jia, Jinchao; Shi, Hui; Teng, Jialin; Liu, Honglei; Sun, Yue; Cheng, Xiaobing; Ye, Junna; Su, Yutong; Chi, Huihui; Liu, Tingting; Wang, Zhihong; Wan, Liyan; Meng, Jianfen; Ma, Yuning; Yang, Chengde; Hu, Qiongyi
Title: Association of the Leukocyte Immunoglobulinâ€like Receptor A3 Gene With Neutrophil Activation and Disease Susceptibility in Adultâ€Onset Still’s Disease Cord-id: x7buveu1 Document date: 2021_5_2
ID: x7buveu1
Snippet: OBJECTIVE: Adultâ€onset Still’s disease (AOSD) is a severe autoinflammatory disease. Neutrophil activation with enhanced neutrophil extracellular trap (NET) formation is involved in the pathogenesis of AOSD. Functional leukocyte immunoglobulinâ€like receptor A3 (LIRâ€A3; gene name LILRA3) has been reported to be associated with many autoimmune diseases. We aimed to investigate the association of LILRA3 with disease susceptibility and neutrophil activation in AOSD. METHODS: The LILRA3 deleti
Document: OBJECTIVE: Adultâ€onset Still’s disease (AOSD) is a severe autoinflammatory disease. Neutrophil activation with enhanced neutrophil extracellular trap (NET) formation is involved in the pathogenesis of AOSD. Functional leukocyte immunoglobulinâ€like receptor A3 (LIRâ€A3; gene name LILRA3) has been reported to be associated with many autoimmune diseases. We aimed to investigate the association of LILRA3 with disease susceptibility and neutrophil activation in AOSD. METHODS: The LILRA3 deletion polymorphism and its tagging singleâ€nucleotide polymorphism rs103294 were genotyped in 164 patients with AOSD and 305 healthy controls. The impact of LILRA3 on clinical features and messenger RNA expression was evaluated. Plasma levels of LIRâ€A3 were detected using enzymeâ€linked immunosorbent assay (ELISA), and the correlation between LIRâ€A3 plasma levels and disease activity and levels of circulating NETâ€DNA was investigated. LIRâ€A3–induced NETs were determined using PicoGreen doubleâ€stranded DNA dye and immunofluorescence analysis in human neutrophils and a neutrophilâ€like differentiated NB4 cell line transfected with LIRâ€B2 small interfering RNA. RESULTS: The findings from genotyping demonstrated that functional LILRA3 was a risk factor for AOSD (11% in AOSD patients versus 5.6% in healthy controls; odds ratio 2.089 [95% confidence interval 1.030–4.291], P = 0.034), and associated with leukocytosis (P = 0.039) and increased levels of circulating neutrophils (P = 0.027). Functional LILRA3 messenger RNA expression was higher in the peripheral blood mononuclear cells (P < 0.0001) and neutrophils (P < 0.001) of LILRA3 (+/+) patients. Plasma levels of LIRâ€A3 were elevated in patients with AOSD (P < 0.0001) and correlated with disease activity indicators and levels of circulating NET–DNA complexes. Finally, enhanced NET formation was identified in neutrophils from healthy controls and patients with inactive AOSD after stimulation of the neutrophils with LIRâ€A3. Moreover, NET formation was impaired in NB4 cells after knockdown of LILRB2 gene expression. CONCLUSION: Our study provides the first evidence that functional LILRA3 is a novel genetic risk factor for the development of AOSD and that functional LIRâ€A3 may play a pathogenic role by inducing formation of NETs.
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