白细胞介素-2 刺激和 TRPM3 治疗对肌痛性脑脊髓炎/慢性疲劳综合征患者中通道共定位与 NK 细胞功能的影响。
The effect of IL-2 stimulation and treatment of TRPM3 on channel co-localisation with PIP and NK cell function in myalgic encephalomyelitis/chronic fatigue syndrome patients.
机构信息
School of Medical Sciences, Griffith University, Gold Coast, Australia.
National Centre for Neuroimmunology and Emerging Diseases, Menzies Health Institute Queensland, Griffith University, Gold Coast, Australia.
出版信息
J Transl Med. 2021 Jul 15;19(1):306. doi: 10.1186/s12967-021-02974-4.
BACKGROUND
Myalgic Encephalomyelitis/Chronic Fatigue Syndrome (ME/CFS) is a serious multifactorial disorder. The origin remains ambiguous, however reduced natural killer (NK) cell cytotoxicity is a consistent immunological feature of ME/CFS. Impaired transient receptor potential melastatin 3 (TRPM3), a phosphatidylinositol dependent channel, and impaired calcium mobilisation have been implicated in ME/CFS pathology. This investigation aimed to examine the localisation of TRPM3 at the NK cell plasma membrane and co-localisation with phosphatidylinositol 4,5-bisphosphate (PIP). The effect of IL-2 priming and treatment using pregnenolone sulfate (PregS) and ononetin on TRPM3 co-localisation and NK cell cytotoxicity in ME/CFS patients and healthy controls (HC) was also investigated.
METHODS
NK cells were isolated from 15 ME/CFS patients and 15 age- and sex-matched HC. Immunofluorescent technique was used to determine co-localisation of TRPM3 with the NK cell membrane and with PIP of ME/CFS patients and HC. Flow cytometry was used to determine NK cell cytotoxicity. Following IL-2 stimulation and treatment with PregS and ononetin changes in co-localisation and NK cell cytotoxicity were measured.
RESULTS
Overnight treatment of NK cells with PregS and ononetin resulted in reduced co-localisation of TRPM3 with PIP and actin in HC. Co-localisation of TRPM3 with PIP in NK cells was significantly reduced in ME/CFS patients compared with HC following priming with IL-2. A significant increase in co-localisation of TRPM3 with PIP was reported following overnight treatment with ononetin within ME/CFS patients and between groups. Baseline NK cell cytotoxicity was significantly reduced in ME/CFS patients; however, no changes were observed following overnight incubation with IL-2, PregS and ononetin between HC and ME/CFS patients. IL-2 stimulation significantly enhanced NK cell cytotoxicity in HC and ME/CFS patients.
CONCLUSION
Significant changes in co-localisation suggest PIP-dependent TRPM3 function may be impaired in ME/CFS patients. Stimulation of NK cells with IL-2 significantly enhanced cytotoxic function in ME/CFS patients demonstrating normal function compared with HC. A crosstalk exists between IL-2 and TRPM3 intracellular signalling pathways which are dependent on Ca influx and PIP. While IL-2R responds to IL-2 binding in vitro, Ca dysregulation and impaired intracellular signalling pathways impede NK cell function in ME/CFS patients.
背景
肌痛性脑脊髓炎/慢性疲劳综合征(ME/CFS)是一种严重的多因素疾病。其起源仍不清楚,然而,自然杀伤(NK)细胞细胞毒性降低是 ME/CFS 的一致免疫学特征。瞬时受体电位 melastatin 3(TRPM3),一种依赖于磷脂酰肌醇的通道,以及钙动员受损,与 ME/CFS 病理学有关。本研究旨在检查 NK 细胞膜上 TRPM3 的定位及其与磷脂酰肌醇 4,5-二磷酸(PIP)的共定位。还研究了白细胞介素 2(IL-2)引发以及用孕烯醇酮硫酸盐(PregS)和 Ononetin 治疗对 ME/CFS 患者和健康对照(HC)中 TRPM3 共定位和 NK 细胞细胞毒性的影响。
方法
从 15 名 ME/CFS 患者和 15 名年龄和性别匹配的 HC 中分离 NK 细胞。免疫荧光技术用于确定 ME/CFS 患者和 HC 中 TRPM3 与 NK 细胞膜和 PIP 的共定位。使用流式细胞术测定 NK 细胞细胞毒性。在 IL-2 刺激和用 PregS 和 Ononetin 处理后,测量共定位和 NK 细胞细胞毒性的变化。
结果
HC 中,PregS 和 Ononetin overnight 处理会导致 TRPM3 与 PIP 和肌动蛋白的共定位减少。与 HC 相比,IL-2 引发后 ME/CFS 患者 NK 细胞中 TRPM3 与 PIP 的共定位明显减少。在 ME/CFS 患者中,Ononetin overnight 处理后,与 PIP 的共定位明显增加,且组间也有增加。ME/CFS 患者的 NK 细胞细胞毒性基础值明显降低,但 HC 和 ME/CFS 患者之间,经 overnight incubation with IL-2、PregS 和 Ononetin 处理后未见变化。IL-2 刺激可显著增强 HC 和 ME/CFS 患者的 NK 细胞细胞毒性。
结论
共定位的明显变化表明 ME/CFS 患者中 PIP 依赖性 TRPM3 功能可能受损。IL-2 刺激 NK 细胞可显著增强 ME/CFS 患者的细胞毒性功能,与 HC 相比,表现出正常功能。IL-2 和 TRPM3 细胞内信号通路之间存在串扰,这依赖于 Ca 流入和 PIP。虽然 IL-2R 对外界 IL-2 结合有反应,但 Ca 失调和细胞内信号通路受损会阻碍 ME/CFS 患者的 NK 细胞功能。
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