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通过 Raman 代谢标记对细胞外囊泡进行体外分子成像。

Molecular imaging of extracellular vesicles in vitro via Raman metabolic labelling.

机构信息

Department of Materials, Imperial College London, London SW7 2AZ, UK.

GSK Medicines Research Centre, Gunnels Wood Road, Stevenage, Hertfordshire SG1 2NY, UK.

出版信息

J Mater Chem B. 2020 May 27;8(20):4447-4459. doi: 10.1039/d0tb00620c.

Abstract

Extracellular vesicles (EVs) are biologically-derived nanovectors important for intercellular communication and trafficking. As such, EVs show great promise as disease biomarkers and therapeutic drug delivery vehicles. However, despite the rapidly growing interest in EVs, understanding of the biological mechanisms that govern their biogenesis, secretion, and uptake remains poor. Advances in this field have been hampered by both the complex biological origins of EVs, which make them difficult to isolate and identify, and a lack of suitable imaging techniques to properly study their diverse biological roles. Here, we present a new strategy for simultaneous quantitative in vitro imaging and molecular characterisation of EVs in 2D and 3D based on Raman spectroscopy and metabolic labelling. Deuterium, in the form of deuterium oxide (D2O), deuterated choline chloride (d-Chol), or deuterated d-glucose (d-Gluc), is metabolically incorporated into EVs through the growth of parent cells on medium containing one of these compounds. Isolated EVs are thus labelled with deuterium, which acts as a bio-orthogonal Raman-active tag for direct Raman identification of EVs when introduced to unlabelled cell cultures. Metabolic deuterium incorporation demonstrates no apparent adverse effects on EV secretion, marker expression, morphology, or global composition, indicating its capacity for minimally obstructive EV labelling. As such, our metabolic labelling strategy could provide integral insights into EV biocomposition and trafficking. This approach has the potential to enable a deeper understanding of many of the biological mechanisms underpinning EVs, with profound implications for the design of EVs as therapeutic delivery vectors and applications as disease biomarkers.

摘要

细胞外囊泡(EVs)是一种重要的生物衍生纳米载体,在细胞间通讯和物质转运中发挥着重要作用。因此,EVs 作为疾病生物标志物和治疗性药物递送载体具有很大的应用潜力。然而,尽管人们对 EVs 的兴趣迅速增长,但对控制其生物发生、分泌和摄取的生物学机制的理解仍然很差。这一领域的进展受到 EVs 复杂的生物学起源的阻碍,这使得它们难以分离和鉴定,并且缺乏合适的成像技术来正确研究它们多样化的生物学作用。在这里,我们提出了一种基于拉曼光谱和代谢标记的新策略,用于在 2D 和 3D 中同时对 EVs 进行定量体外成像和分子特征分析。氘(以重水(D2O)、氘代氯化胆碱(d-Chol)或氘代 d-葡萄糖(d-Gluc)的形式)通过在含有这些化合物之一的培养基中生长亲代细胞而代谢掺入到 EVs 中。因此,分离的 EVs 被标记上氘,当引入未标记的细胞培养物时,氘可作为生物正交的拉曼活性标记物,用于直接拉曼识别 EVs。代谢氘掺入表明对 EV 分泌、标记物表达、形态或整体组成没有明显的不良影响,表明其对 EV 标记具有最小的阻塞能力。因此,我们的代谢标记策略可以为 EV 生物组成和运输提供整体见解。这种方法有可能深入了解支持 EV 的许多生物学机制,对 EV 作为治疗性药物传递载体的设计和作为疾病生物标志物的应用具有深远的影响。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d6e5/7610785/370c502b35e2/EMS103713-f001.jpg

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