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Comparison of separation methods for tissue‐derived extracellular vesicles in the liver heart and skeletal muscle

机译:肝心脏和骨骼肌组织衍生细胞外囊分离方法的比较

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摘要

Extracellular vesicles (EVs), which are nanosized vesicles released by cells as intracellular messengers, have high potential as biomarkers. EVs are usually collected from in vitro sources, such as cell culture media or biofluids, and not from tissues. Techniques enabling direct collection of EVs from tissues will extend the applications of EVs. We compared methods for separating EVs from solid liver, heart, and skeletal muscle. Compared with a precipitation method, an ultracentrifugation‐based method for collection of EVs from solid tissues yielded a higher proportion of EVs positive for EV‐related markers, with minimum levels of intracellular organelle‐related markers. Some tissue‐specific modifications, such as a sucrose cushion step, may improve the yield and purity of the collected EVs.
机译:细胞外囊泡(EVS),其作为细胞作为细胞内信使释放的纳米囊泡,具有高潜力作为生物标志物。 EVS通常从体外来源收集,例如细胞培养基或生物流体,而不是来自组织。能够从组织中直接收集EV的技术将扩展EVS的应用。我们比较了从固体肝,心脏和骨骼肌分离EV的方法。与沉淀法相比,来自固体组织的EV的超速离心的方法产生了较高的EV相关标记的EVS阳性比例,具有最小水平的细胞内细胞器相关标记。一些组织特异性修饰,例如蔗糖垫步骤,可以改善收集的EV的产率和纯度。

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