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经结膜下注射人脐带间充质干细胞通过调节 T 细胞应答缓解实验性变应性结膜炎。

Subconjunctival injection of human umbilical cord mesenchymal stem cells alleviates experimental allergic conjunctivitis via regulating T cell response.

机构信息

Department of Ophthalmology of Tongji Hospital, Laboratory of Clinical and Visual Sciences of Tongji Eye Institute, School of Medicine, Tongji University, 389 Xincun Road, Shanghai, 200065, China.

Department of Ophthalmology, Shanghai General Hospital (Shanghai First People's Hospital), Shanghai Jiao Tong University, Shanghai, 200080, China.

出版信息

Stem Cell Res Ther. 2023 Oct 2;14(1):281. doi: 10.1186/s13287-023-03484-4.

Abstract

BACKGROUND

T helper 2 (Th2) cells are thought to play critical roles in allergic conjunctivitis (AC). They release inflammatory cytokines to promote an allergic response in AC. Due to individual heterogeneity and long-term chronic management, current therapies do not always effectively control AC. Mesenchymal stem cells (MSCs) have been shown to be effective in treating allergy-related disorders, but it is unclear how exactly the Th2-mediated allergic response is attenuated. This study aims to elucidate the therapeutic effect and mechanism of the human umbilical cord MSCs (hUCMSCs) in a mouse model of experimental AC (EAC).

METHODS

A mouse EAC model was established by inoculating short ragweed (SRW) pollen. After the SRW pollen challenge, the mice received a single subconjunctival or tail vein injection of 2 × 10 hUCMSCs, or subconjunctival injection of hUCMSCs conditioned medium (hUCMSC-CM), and dexamethasone eye drops was used as positive control; subsequent scratching behavior and clinical symptoms were assessed. Immunostaining and flow cytometry were carried out to show allergic reactions and the activation of CD4 + T cell subsets in the conjunctiva and cervical lymph nodes (CLNs). Gene expression was determined by RNA-seq and further verified by qRT-PCR and Western blot. Co-culture assays were performed to explore the regulatory role of hUCMSCs in the differentiation of CD4 + naive T cells (Th0) into Th2 cells.

RESULTS

Subconjunctival administration of hUCMSCs resulted in fewer instances of scratching and lower inflammation scores in EAC mice compared to the tail vein delivery, hUCMSC-CM and control groups. Subconjunctival administration of hUCMSCs reduced the number of activated mast cells and infiltrated eosinophils in the conjunctiva, as well as decreased the number of Th2 cells in CLNs. After pretreatment with EAC mouse serum in vitro to mimic the in vivo milieu, hUCMSCs were able to inhibit the differentiation of Th0 into Th2 cells. Further evidence demonstrated that repression of Th2 cell differentiation by hUCMSCs is mediated by CRISPLD2 through downregulation of STAT6 phosphorylation. Additionally, hUMCSCs were able to promote the differentiation of Th0 cells into regulatory T cells in CLNs of EAC mice.

CONCLUSIONS

Subconjunctival injection of hUCMSCs suppressed the Th2-allergic response and alleviated clinical symptoms. This study provides not only a potential therapeutic target for the treatment of AC but also other T cell-mediated diseases.

摘要

背景

辅助性 T 细胞 2(Th2)细胞被认为在过敏性结膜炎(AC)中发挥关键作用。它们释放炎症细胞因子,以促进 AC 中的过敏反应。由于个体差异和长期慢性管理,目前的治疗方法并不总能有效控制 AC。间充质干细胞(MSCs)已被证明在治疗与过敏相关的疾病方面有效,但尚不清楚 Th2 介导的过敏反应是如何减弱的。本研究旨在阐明人脐带间充质干细胞(hUCMSCs)在实验性过敏性结膜炎(EAC)小鼠模型中的治疗效果和机制。

方法

通过接种豚草花粉建立小鼠 EAC 模型。在豚草花粉攻击后,小鼠接受单次结膜下或尾静脉注射 2×10 hUCMSCs,或结膜下注射 hUCMSCs 条件培养基(hUCMSC-CM),并使用地塞米松滴眼液作为阳性对照;随后评估抓挠行为和临床症状。免疫染色和流式细胞术用于显示结膜和颈部淋巴结(CLN)中的过敏反应和 CD4+T 细胞亚群的激活。通过 RNA-seq 确定基因表达,并通过 qRT-PCR 和 Western blot 进一步验证。共培养实验用于探索 hUCMSCs 在 CD4+幼稚 T 细胞(Th0)向 Th2 细胞分化中的调节作用。

结果

与尾静脉给药、hUCMSC-CM 和对照组相比,结膜下给予 hUCMSCs 可减少 EAC 小鼠的抓挠次数和炎症评分。结膜下给予 hUCMSCs 可减少激活的肥大细胞和浸润的嗜酸性粒细胞的数量,并减少 CLN 中的 Th2 细胞数量。体外用 EAC 小鼠血清预处理以模拟体内环境后,hUCMSCs 能够抑制 Th0 向 Th2 细胞的分化。进一步的证据表明,hUCMSCs 通过下调 STAT6 磷酸化抑制 Th2 细胞分化。此外,hUCMSCs 能够在 EAC 小鼠的 CLN 中促进 Th0 细胞向调节性 T 细胞的分化。

结论

结膜下注射 hUCMSCs 抑制了 Th2 过敏反应并缓解了临床症状。本研究不仅为 AC 等 T 细胞介导的疾病的治疗提供了一个潜在的治疗靶点,也为其他 T 细胞介导的疾病提供了一个潜在的治疗靶点。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5130/10546642/5414ea1d3796/13287_2023_3484_Fig1_HTML.jpg

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