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采用结合亲和洗脱和大小排阻色谱法可实现细胞外囊泡的可重现和可扩展的纯化。

Reproducible and scalable purification of extracellular vesicles using combined bind-elute and size exclusion chromatography.

机构信息

Department of Laboratory Medicine, Karolinska Institutet, Stockholm, Sweden.

Department of Physiology, Anatomy and Genetics, University of Oxford, Oxford, United Kingdom.

出版信息

Sci Rep. 2017 Sep 14;7(1):11561. doi: 10.1038/s41598-017-10646-x.

Abstract

Extracellular vesicles (EVs) play a pivotal role in cell-to-cell communication and have been shown to take part in several physiological and pathological processes. EVs have traditionally been purified by ultracentrifugation (UC), however UC has limitations, including resulting in, operator-dependant yields, EV aggregation and altered EV morphology, and moreover is time consuming. Here we show that commercially available bind-elute size exclusion chromatography (BE-SEC) columns purify EVs with high yield (recovery ~ 80%) in a time-efficient manner compared to current methodologies. This technique is reproducible and scalable, and surface marker analysis by bead-based flow cytometry revealed highly similar expression signatures compared with UC-purified samples. Furthermore, uptake of eGFP labelled EVs in recipient cells was comparable between BE-SEC and UC samples. Hence, the BE-SEC based EV purification method represents an important methodological advance likely to facilitate robust and reproducible studies of EV biology and therapeutic application.

摘要

细胞外囊泡 (EVs) 在细胞间通讯中发挥着关键作用,并被证明参与了几种生理和病理过程。EVs 传统上通过超速离心 (UC) 进行纯化,但 UC 有其局限性,包括产生依赖于操作人员的产量、EV 聚集和改变 EV 形态,而且耗时。在这里,我们展示了市售的结合洗脱大小排阻色谱 (BE-SEC) 柱可以高效地纯化 EV,与当前方法相比,回收率约为 80%。该技术具有可重复性和可扩展性,通过基于珠子的流式细胞术进行表面标志物分析,与 UC 纯化的样品相比,显示出高度相似的表达特征。此外,在受体细胞中摄取 eGFP 标记的 EV 在 BE-SEC 和 UC 样品之间是可比的。因此,基于 BE-SEC 的 EV 纯化方法是一个重要的方法学进展,可能会促进 EV 生物学和治疗应用的稳健和可重复的研究。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8d63/5599601/d70a4260ad56/41598_2017_10646_Fig1_HTML.jpg

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