人超氧化物歧化酶（SOD） 1 G93A和氯病毒ATCV-1 SOD的表达增加了巨噬细胞对炎症刺激物的反应，包括ATCV-1主要衣壳蛋白聚糖

IF 2.5 4区医学 Q3 IMMUNOLOGY

Immunobiology Pub Date : 2025-02-12 DOI:10.1016/j.imbio.2025.152881

Thomas M. Petro , Ahmed Esmael , Gary L. Pattee , Fiyad Al-Sarmi , Fabrizio Chiodo , Irina V. Agarkova , David D. Dunigan , James L. Van Etten

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引用次数: 0

摘要

家族性肌萎缩性侧索硬化症（ALS）的一个原因是超氧化物歧化酶1 （SOD1）突变，其中氨基酸93是丙氨酸而不是甘氨酸（SOD1- g93a）。表达人SOD1-G93A致病变异的转基因小鼠可发生类似ALS的运动神经元病（MND）。ALS患者和SOD1-G93A小鼠的炎性细胞因子如IL-6的产生升高，这可能会促进MND。我们之前的研究表明，感染了编码SOD1的绿病毒棘囊藻小球藻病毒1 (ATCV-1)，加速了这些小鼠MND的发病，并诱导巨噬细胞产生高水平的IL-6。我们在此证实，与健康对照相比，ALS患者的血浆IL-6和干扰素γ (IFN-γ)水平显著升高，但IL-17水平无显著升高。为了确定ATCV-1 SOD1或SOD1- g93a在小鼠巨噬细胞中的表达是否会提高炎症因子的表达，我们用编码ATCV-1 SOD1、野生型人SOD1、SOD1- g93a或空载体的质粒转染了RAW264.7小鼠巨噬细胞细胞系。稳定表达wtSOD1或G93A-SOD1的RAW264.7细胞被poly I:C和干扰素- γ单独或联合刺激，诱导炎症因子，如IL-6和一氧化氮（NO），抗炎因子，如IL-10，或激活干扰素刺激反应元件（ISRE）启动子。刺激后，表达SOD1- g93a的RAW264.7细胞中IL-6和NO的产生明显高于表达SOD1- g93a的细胞，但IL-10和ISRE启动子活性不明显。此外，与SOD1表达的RAW264.7细胞相比，表达SOD1- g93a的细胞在ATCV-1糖蛋白的作用下产生更高水平的IL-6和NO。最后，将编码ATCV-1 SOD1的质粒转染RAW264.7细胞，显著增加炎症因子在poly I:C和IFN-γ反应中的表达，主要以干扰素调节因子3 （IRF3）依赖的方式表达。这些数据清楚地表明，巨噬细胞中G93A-SOD1或ATCV-1 SOD1的表达在模拟病毒感染、病毒成分或T细胞因子刺激后显著升高炎症因子的表达，从而提示巨噬细胞中非典型SOD1参与ALS-MND的一种机制。

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Expression of human superoxide dismutase (SOD) 1 G93A and chlorovirus ATCV-1 SOD increases the response of macrophages to inflammatory stimulants, including ATCV-1 major capsid protein glycans

One cause of familial Amyotrophic Lateral Sclerosis (ALS) is a mutation in Super Oxide Dismutase 1 (SOD1) whereby amino acid 93 is alanine instead of glycine (SOD1-G93A). Transgenic mice expressing human SOD1-G93A pathogenic variant develop motor neuron disease (MND), similar to ALS. Humans with ALS and SOD1-G93A mice have elevated production of inflammatory cytokines, such as IL-6, which may promote MND. We previously showed that infection with the Chlorovirus Acanthocystis turfacea chlorella virus 1 (ATCV-1), which encodes a SOD1, accelerates onset of MND in these mice and induces macrophages to produce high levels of IL-6. We confirm here that ALS patients compared with healthy controls have significantly elevated levels of plasma IL-6 and Interferon-gamma (IFN-γ), but not IL-17. To determine if expression of ATCV-1 SOD1 or SOD1-G93A in mouse macrophages elevates expression of inflammatory cytokines, we transfected the RAW264.7 mouse macrophage cell line with plasmids encoding ATCV-1 SOD1, wild-type human SOD1, SOD1-G93A, or an empty vector. RAW264.7 cells stably expressing wtSOD1 or G93A-SOD1 were stimulated with poly I:C and Interferon-gamma, alone, or in combination to induce inflammatory factors, such as IL-6 and Nitric Oxide (NO), anti-inflammatory factors, such as IL-10, or activation of Interferon Stimulated Response Elements (ISRE) promoters. After stimulation, production of IL-6 and NO, but not IL-10 or ISRE promoter activity was significantly higher in RAW264.7 cells expressing SOD1-G93A compared with wt SOD1. Moreover, RAW264.7 cells expressing SOD1-G93A compared with wt SOD1 produced higher levels of IL-6 and NO in response to ATCV-1 glycoproteins. Finally, transfection of plasmid encoding ATCV-1 SOD1 into RAW264.7 cells significantly increased expression of inflammatory factors in responses to poly I:C and IFN-γ, primarily in an Interferon regulatory factor 3 (IRF3) dependent fashion. These data clearly show that expression of G93A-SOD1 or ATCV-1 SOD1 in macrophages significantly elevates expression of inflammatory factors following stimulations that mimic virus infection, viral components, or T cell cytokines, thereby suggesting one mechanism by which atypical SOD1 in macrophages can contribute to ALS-MND.

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来源期刊

Immunobiology 医学-免疫学

CiteScore

5.00

自引率

3.60%

发文量

108

审稿时长

55 days

期刊介绍： Immunobiology is a peer-reviewed journal that publishes highly innovative research approaches for a wide range of immunological subjects, including • Innate Immunity, • Adaptive Immunity, • Complement Biology, • Macrophage and Dendritic Cell Biology, • Parasite Immunology, • Tumour Immunology, • Clinical Immunology, • Immunogenetics, • Immunotherapy and • Immunopathology of infectious, allergic and autoimmune disease.