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一种用于分离尿液外泌体的改良沉淀法。

A modified precipitation method to isolate urinary exosomes.

作者信息

Kanchi Ravi Rupesh, Khosroheidari Mahdieh, DiStefano Johanna K

机构信息

Diabetes, Cardiovascular and Metabolic Diseases Division, Translational Genomics Research Institute (TGen).

Diabetes, Cardiovascular and Metabolic Diseases Division, Translational Genomics Research Institute (TGen);

出版信息

J Vis Exp. 2015 Jan 16(95):51158. doi: 10.3791/51158.

Abstract

Identification of biomarkers that allow early detection of kidney diseases in urine and plasma has been an area of active interest for several years. Urinary exosome vesicles, 40-100 nm in size, are released into the urine under normal conditions by cells from all nephron segments and may contain protein, mRNA and microRNA representative of their cell type of origin. Under conditions of renal dysfunction or injury, exosomes may contain altered proportions of these components, which may serve as biomarkers for disease. There are currently several methods available for isolation of urinary exosomes, and we have previously conducted an experimental comparison of each of these approaches, including three based on ultracentrifugation, one using a nanomembrane ultrafiltration concentrator, one using a commercial precipitation reagent and one using a modification of the precipitation technique using ExoQuick reagent that we developed in our laboratory. We found the modified precipitation method produced the highest yield of exosome particles, miRNA, and mRNA, making this approach suitable for the isolation of exosomes for subsequent RNA profiling. We conclude that the modified exosome precipitation method offers a quick, scalable, and effective alternative for the isolation of exosomes from urine. In this report, we describe our modified precipitation technique using ExoQuick reagent for isolating exosomes from human urine.

摘要

多年来,寻找能够在尿液和血浆中早期检测肾脏疾病的生物标志物一直是一个备受关注的领域。尿外泌体囊泡大小为40 - 100纳米,在正常情况下由所有肾单位节段的细胞释放到尿液中,可能含有代表其起源细胞类型的蛋白质、mRNA和微小RNA。在肾功能不全或损伤的情况下,外泌体可能含有这些成分比例的改变,这可能作为疾病的生物标志物。目前有几种方法可用于分离尿外泌体,我们之前对每种方法都进行了实验比较,包括三种基于超速离心的方法、一种使用纳米膜超滤浓缩器的方法、一种使用商业沉淀试剂的方法以及一种使用我们实验室开发的ExoQuick试剂对沉淀技术进行改进的方法。我们发现改进后的沉淀方法产生的外泌体颗粒、miRNA和mRNA产量最高,使这种方法适用于分离外泌体以进行后续的RNA分析。我们得出结论,改进后的外泌体沉淀方法为从尿液中分离外泌体提供了一种快速、可扩展且有效的替代方法。在本报告中,我们描述了使用ExoQuick试剂从人尿液中分离外泌体的改进沉淀技术。

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