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AI-17 Response gene to complement-32 expression is upregulated in lupus T cells and promotes IL-17A expression

分子生物学 流式细胞术 生物 系统性红斑狼疮 狼疮性肾炎 下调和上调 免疫学 医学 内科学 基因 生物化学 疾病
作者
Anamaria Talpos-Caia,Alexandru Tatomir,Vinh Nguyen,Cornelia Cudrici,Simona Rednic,Horea Rus,Violeta Rus
标识
DOI:10.1136/lupus-2018-lsm.17
摘要

Background

RGC (Response Gene to Complement)-32 is a cell cycle regulator widely expressed in normal tissues including brain, kidney, spleen, thymus, multiple tumors and in a variety of cell lines. RGC-32 is localized in the cytoplasm and translocates to the nucleus upon upregulation by complement activation, growth factors and cytokines. RGC-32 is induced by TGFβ in fibroblasts, astrocytes and human renal proximal tubular cells and mediates TGFβ dependent profibrotic pathways. RGC-32 is preferentially upregulated in murine Th17 cells and promotes their differentiation. Patients with Systemic Lupus Erythematosus (SLE) display increased serum levels, expanded frequency of IL-17 producing cells. Whether RGC-32 plays a role in human Th17 differentiation pathway and in Th17 abnormalities in lupus patients has not yet been investigated.

Methods

RGC-32 expression in naïve CD4+ T cells from normal controls stimulated with cytokines alone or under Th0, Th1, Th2, Th17 and Treg conditions was determined by flow cytometry and RT-PCR. RGC-32 mRNA expression in PBMCs of lupus patients was assessed with the Autoimmune Disease Profiling cDNA Array spotted with cDNA from CD3+, CD19+ and CD14+ cells and by RT-PCR and flow cytometry. RGC-32 nuclear translocation after stimulation under Th17 conditions was assessed by Western blotting. RGC-32 overexpression and silencing was performed by nucleofection and the effect on IL-17A mRNA levels in CD4+ T cells under Th17 conditions was determined by RT-PCR.

Results

RGC-32 mRNA expression was upregulated by TCR stimulation and TGFβ and was more robust under Th17 (3.2±fold) and Treg (2.6±0.8 fold) vs Th1 (1.3±0.4 fold) and Th2 (1.8±0.1 fold) conditions. Moreover, upon stimulation with anti-CD3/CD28 and TGFβ, RGC-32 was translocated into the nucleus. Other cytokines such as IFNα, IL-1β, TNFα did not upregulate RGC-32 mRNA either alone or in combination with TCR stimulation. Overexpression or silencing of RGC-32 in CD4+ T cells upregulated, respectively downregulated IL-17A transcript levels and protein secretion. RGC-32 mRNA and protein level were significantly increased in CD19+ B cells and CD3+ T from lupus patients compared to controls.

Conclusions

These results suggest that RGC-32 promotes the differentiation of human Th17 cells. Furthermore, T cells from patients with SLE exhibit increased expression of RGC-32 compared to controls. These data support the idea that RGC-32 signaling may enhance disease expression in SLE by promoting abnormalities in the Th17 pathway and provide a compelling rationale for further investigating the therapeutic potential of blocking RGC-32 in SLE.
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