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平衡产量、纯度和实用性:改良的差速超速离心法从人血清中高效分离小细胞外囊泡的方案。

Balancing yield, purity and practicality: a modified differential ultracentrifugation protocol for efficient isolation of small extracellular vesicles from human serum.

机构信息

a Division of Epidemiology, Department of Environmental Health , University of Cincinnati College of Medicine , Cincinnati , OH , USA.

b Cincinnati Cancer Center , Cincinnati , OH , USA.

出版信息

RNA Biol. 2019 Jan;16(1):5-12. doi: 10.1080/15476286.2018.1564465. Epub 2019 Jan 13.

Abstract

Ultracentrifugation remains the gold standard for isolation of small extracellular vesicles (sEV), particularly for cancer applications. The objective of this study was to determine if a widely used ultracentrifugation protocol for isolation of serum sEV could be modified to reduce the number of ultracentrifugation cycles and increase efficiency, while maintaining equal or better sample purity and yield. Serum was obtained from two healthy subjects. sEVs were isolated from 1 mL aliquots using three different ultracentrifugation protocols. Co-isolation of RNA carrier protein was assessed by performing Western blots for ApoA-I, ApoB, and Ago2. Small RNA-sequencing was performed on the sEV isolates, and differential detection of small ncRNA was compared across isolation protocols. Reduction from three- to two-ultracentrifuge cycles with no sucrose cushion resulted in a much higher sEV yield but also had the highest levels of lipoprotein and Ago2 contamination. However, the two-ultracentrifugation cycle protocol that incorporated a 30% sucrose cushion into the first cycle resulted in slightly higher sEV yields with lower levels of protein contamination compared to the lengthier three-ultracentrifugation cycle approach, therefore presenting a more efficient alternative approach for isolation of serum sEVs. It was also notable that there were some differences in sEV ncRNA cargo according to protocol, although it was less than expected given the differences in co-isolated RNA carrier proteins. Our results suggest that use of the modified serum sEV isolation protocol with two ultracentrifugation cycles and incorporating a 30% sucrose cushion offers a more efficient approach in terms of efficiency and purity.

摘要

超速离心仍然是分离小细胞外囊泡 (sEV) 的金标准,特别是对于癌症应用。本研究的目的是确定是否可以修改广泛用于分离血清 sEV 的超速离心方案,以减少超速离心循环的次数并提高效率,同时保持相等或更好的样品纯度和产量。从两名健康受试者中获得血清。使用三种不同的超速离心方案从 1 mL 等分试样中分离 sEV。通过进行 ApoA-I、ApoB 和 Ago2 的 Western blot 评估 RNA 载体蛋白的共分离。对 sEV 分离物进行小 RNA 测序,并比较分离方案之间小 ncRNA 的差异检测。从三个超速离心循环减少到两个超速离心循环而不使用蔗糖垫导致 sEV 产量大大增加,但脂蛋白和 Ago2 的污染水平也最高。然而,在第一个循环中加入 30%蔗糖垫的两超速离心循环方案与更长的三个超速离心循环方法相比,sEV 产量略高,蛋白污染水平较低,因此为分离血清 sEV 提供了更有效的替代方法。值得注意的是,根据方案,sEV ncRNA 货物也存在一些差异,尽管与共分离的 RNA 载体蛋白的差异相比,差异较小。我们的结果表明,使用改良的血清 sEV 分离方案,两个超速离心循环并加入 30%蔗糖垫,在效率和纯度方面提供了更有效的方法。

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