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Isolation of urinary extracellular vesicles from Tamm-Horsfall protein-depleted urine and their application in the development of a lectin-exosome-binding assay

机译:Tamm-Horsfall蛋白贫化尿液中尿液细胞外囊泡的分离及其在凝集素-外泌体结合测定中的应用

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Urine is a readily available source of relatively large quantities of extracellular vesicles (EVs). However, the isolation of urinary EVs (uEVs) is complicated by the presence of Tamm-Horsfall protein (THP), which polymerizes and co-precipitates as a contaminant. This may make glycan analysis of uEVs difficult since THP is heavily glycosylated. To facilitate glycosylation analysis and address the need for elimination of non-uEV glycans, we present a modification of the uEV isolation procedure and use the isolated uEVs in the development of a lectin-exosome binding assay. Salt precipitation was employed to remove THP under conditions originally described for its separation from urine, followed by differential centrifugation. The quality of the isolated uEVs was examined by electron microscopy, SDS-PAGE, and immunoblotting. The uEVs were subsequently immobilized on solid phase and probed with labeled plant lectins using the lectin-exosome binding assay. Our results indicate that the isolated uEVs had preserved structural integrity and reacted with labeled plant lectins in a selective, carbohydrate-dependent manner. The basic lectin binding pattern of uEVs obtained by our method can be used as a reference for assessing the composition of their surface glycans in different physiological and pathological conditions.
机译:尿是相对大量的细胞外囊泡(EV)的容易获得的来源。但是,Tamm-Horsfall蛋白(THP)的存在使尿液电动汽车(uEV)的分离变得复杂,该蛋白质会聚合并作为污染物共沉淀。由于THP被高度糖基化,这可能使uEV的聚糖分析变得困难。为了促进糖基化分析和解决消除非uEV聚糖的需求,我们提出了uEV分离程序的改进,并将分离的uEV用于凝集素-外泌体结合测定的开发。在最初描述的与尿液分离的条件下,采用盐沉淀法去除THP,然后进行离心分离。通过电子显微镜,SDS-PAGE和免疫印迹检查分离出的uEV的质量。随后将uEV固定在固相上,并使用凝集素-外泌体结合测定法用标记的植物凝集素进行探测。我们的结果表明,分离出的uEV保留了结构完整性,并以选择性,碳水化合物依赖性的方式与标记的植物凝集素反应。通过我们的方法获得的uEV的基本凝集素结合模式可作为评估其在不同生理和病理条件下表面聚糖组成的参考。

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