Fang Shu-Bin, Zhang Hong-Yu, Wang Cong, He Bi-Xin, Liu Xiao-Qing, Meng Xiang-Ci, Peng Ya-Qi, Xu Zhi-Bin, Fan Xing-Liang, Wu Zhang-Jin, Chen Dong, Zheng Lei, Zheng Song Guo, Fu Qing-Ling
Otorhinolaryngology Hospital, The First Affiliated Hospital, Sun Yat-sen University, Guangzhou, China.
Department of Laboratory Medicine, Nanfang Hospital, Southern Medical University, Guangzhou, China.
J Extracell Vesicles. 2020 Feb 10;9(1):1723260. doi: 10.1080/20013078.2020.1723260. eCollection 2020.
Group 2 innate lymphoid cells (ILC2s) are recently reported to play a more critical role in allergic diseases. We previously identified that mesenchymal stromal cells (MSCs) elicited therapeutic effects on allergic airway inflammation. Small extracellular vesicles (sEV) derived from MSCs possess striking advantages including low immunogenicity and high biosafety, and is extremely promising cell-free therapeutic agents. However, the effects of MSC-sEV on ILC2s are still unclear. Additionally, scalable isolation protocols are required for the mass production of homogenous MSC-sEV especially in clinical application. We previously reported that induced pluripotent stem cells-derived MSCs were the ideal cellular source for the large preparation of MSC-sEV. Here we developed a standardized scalable protocol of anion-exchange chromatography for isolation of MSC-sEV, and investigated the effects of MSC-sEV on ILC2 function from patients with allergic rhinitis and in a mouse ILC2-dominant asthma model. The characterization of MSC-sEV was successfully demonstrated in terms of size, morphology and specific markers. Using flow cytometry and human Cytokine Antibody Array, MSC-sEV but not fibroblasts-sEV (Fb-sEV) were found to significantly inhibit the function of human ILC2s. Similarly, systemic administration of MSC-sEV but not Fb-sEV exhibited an inhibition of ILC2 levels, inflammatory cell infiltration and mucus production in the lung, a reduction in levels of T helper 2 cytokines, and alleviation of airway hyperresponsiveness in a mouse model of asthma. Using RNA sequencing, miR-146a-5p was selected as the candidate to mediate the above effects of MSC-sEV. We next revealed the uptake of ILC2s to MSC-sEV, and that transfer of miR-146a-5p in MSC-sEV to ILC2s in part contributed to the effects of MSC-sEV on ILC2s and in a mouse model. In conclusion, we demonstrated that MSC-sEV were able to prevent ILC2-dominant allergic airway inflammation at least partially through miR-146a-5p, suggesting that MSC-sEV could be a novel cell-free strategy for the treatment of allergic diseases.
最近有报道称,第2组固有淋巴细胞(ILC2s)在过敏性疾病中发挥着更关键的作用。我们之前发现间充质基质细胞(MSCs)对过敏性气道炎症具有治疗作用。源自MSCs的小细胞外囊泡(sEV)具有显著优势,包括低免疫原性和高生物安全性,是极具前景的无细胞治疗剂。然而,MSC-sEV对ILC2s的影响仍不清楚。此外,大规模生产同质MSC-sEV需要可扩展的分离方案,尤其是在临床应用中。我们之前报道过,诱导多能干细胞来源的MSCs是大规模制备MSC-sEV的理想细胞来源。在此,我们开发了一种用于分离MSC-sEV的阴离子交换色谱标准化可扩展方案,并研究了MSC-sEV对过敏性鼻炎患者的ILC2功能以及在小鼠ILC2主导的哮喘模型中的影响。成功从大小、形态和特定标志物方面对MSC-sEV进行了表征。使用流式细胞术和人细胞因子抗体阵列,发现MSC-sEV而非成纤维细胞来源的小细胞外囊泡(Fb-sEV)能显著抑制人ILC2s的功能。同样,在哮喘小鼠模型中,全身给予MSC-sEV而非Fb-sEV可抑制肺部ILC2水平、炎症细胞浸润和黏液分泌,降低辅助性T细胞2细胞因子水平,并减轻气道高反应性。通过RNA测序,选择miR-146a-5p作为介导MSC-sEV上述作用的候选分子。接下来我们揭示了ILC2s对MSC-sEV的摄取,并且MSC-sEV中的miR-146a-5p转移至ILC2s在一定程度上促成了MSC-sEV对ILC2s的作用以及在小鼠模型中的作用。总之,我们证明了MSC-sEV至少部分能够通过miR-146a-5p预防ILC2主导的过敏性气道炎症,这表明MSC-sEV可能是一种治疗过敏性疾病的新型无细胞策略。
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