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人雪旺细胞衍生细胞外囊泡的分离、生物活性评估及组学表征

Human Schwann Cell-Derived Extracellular Vesicle Isolation, Bioactivity Assessment, and Omics Characterization.

作者信息

Khan Aisha, Oliveira Julia, Lee Yee-Shuan, Guest James D, Silvera Risset, Pressman Yelena, Pearse Damien D, Nettina Adriana E, Goldschmidt-Clermont Pascal J, Al-Ali Hassan, Williams Indigo, Levi Allan D, Dietrich W Dalton

机构信息

Interdisciplinary Stem Cell Institute, Miller School of Medicine, University of Miami, Miami, FL, USA.

The Miami Project to Cure Paralysis, Miller School of Medicine, University of Miami, Miami, FL, USA.

出版信息

Int J Nanomedicine. 2025 Apr 4;20:4123-4144. doi: 10.2147/IJN.S500159. eCollection 2025.

Abstract

PURPOSE

Schwann cell-derived extracellular vesicles (SCEVs) have demonstrated favorable effects in spinal cord, peripheral nerve, and brain injuries. Herein, a scalable, standardized, and efficient isolation methodology of SCEVs obtaining a high yield with a consistent composition as measured by proteomic, lipidomic, and miRNA analysis of their content is described for future clinical use.

METHODS

Human Schwann cells were obtained ethically from nine donors and cultured in a defined growth medium optimized for proliferation. At confluency, the culture was replenished with an isolation medium for 48 hours, then collected and centrifuged sequentially at low and ultra-high speeds to collect purified EVs. The EVs were characterized with mass spectrometry to identify and quantify proteins, lipidomic analysis to assess lipid composition, and next-generation sequencing to confirm miRNA profiles. Each batch of EVs was assessed to ensure their therapeutic potential in promoting neurite outgrowth and cell survival.

RESULTS

High yields of SCEVs were consistently obtained with similar comprehensive molecular profiles across samples, indicating the reproducibility and reliability of the isolation method. Bioactivity to increase neurite process growth was confirmed in vitro. The predominance of triacylglycerol and phosphatidylcholine suggested its role in cellular membrane dynamics essential for axon regeneration and inflammation mitigation. Of the 2517 identified proteins, 136 were closely related to nervous system repair and regeneration. A total of 732 miRNAs were cataloged, with the top 30 miRNAs potentially contributing to axon growth, neuroprotection, myelination, angiogenesis, the attenuation of neuroinflammation, and key signaling pathways such as VEGFA-VEGFR2 and PI3K-Akt signaling, which are crucial for nervous system repair.

CONCLUSION

The study establishes a robust framework for SCEV isolation and their comprehensive characterization, which is consistent with their therapeutic potential in neurological applications. This work provides a valuable proteomic, lipidomic, and miRNA dataset to inform future advancements in applying SCEV to the experimental treatment of neurological injuries and diseases.

摘要

目的

雪旺细胞衍生的细胞外囊泡(SCEV)已在脊髓、周围神经和脑损伤中显示出良好效果。本文描述了一种可扩展、标准化且高效的SCEV分离方法,该方法能够获得高产率,且通过对其内容物进行蛋白质组学、脂质组学和miRNA分析,可得到成分一致的SCEV,以供未来临床使用。

方法

从九名供体处伦理获取人雪旺细胞,并在优化用于增殖的限定生长培养基中培养。细胞汇合后,用分离培养基补充培养48小时,然后收集并依次进行低速和超高速离心以收集纯化的细胞外囊泡(EV)。通过质谱对EV进行表征以鉴定和定量蛋白质,进行脂质组分析以评估脂质组成,并通过下一代测序确认miRNA谱。对每一批EV进行评估,以确保其在促进神经突生长和细胞存活方面的治疗潜力。

结果

始终能获得高产率的SCEV,且各样本间具有相似的综合分子谱,表明该分离方法具有可重复性和可靠性。体外证实了其增加神经突生长的生物活性。三酰甘油和磷脂酰胆碱的优势表明其在轴突再生和减轻炎症所必需的细胞膜动力学中的作用。在鉴定出的2517种蛋白质中,有136种与神经系统修复和再生密切相关。共编目了732种miRNA,其中排名前30的miRNA可能有助于轴突生长、神经保护、髓鞘形成、血管生成、神经炎症减轻以及VEGFA-VEGFR2和PI3K-Akt信号传导等关键信号通路,这些信号通路对神经系统修复至关重要。

结论

该研究建立了一个强大的SCEV分离及其全面表征的框架,这与其在神经学应用中的治疗潜力一致。这项工作提供了有价值的蛋白质组学、脂质组学和miRNA数据集,为未来将SCEV应用于神经损伤和疾病的实验性治疗的进展提供参考。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/20c8/11977562/23e633b32878/IJN-20-4123-g0001.jpg

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