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Isolation and Characterization of RNA-Containing Exosomes

机译:含RNA的外泌体的分离与鉴定

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摘要

The field of exosome research is rapidly expanding, with a dramatic increase in publications in recent years. These small vesicles (30-100 nm) of endocytic origin were first proposed to function as a way for reticulocytes to eradicate the transferrin receptor while maturing into erythrocytes1, and were later named exosomes. Exosomes are formed by inward budding of late endosomes, producing multivesicular bodies (MVBs), and are released into the environment by fusion of the MVBs with the plasma membrane2. Since the first discovery of exosomes, a wide range of cells have been shown to release these vesicles. Exosomes have also been detected in several biological fluids, including plasma, nasal lavage fluid, saliva and breast milk3-6. Furthermore, it has been demonstrated that the content and function of exosomes depends on the originating cell and the conditions under which they are produced. A variety of functions have been demonstrated for exosomes, such as induction of tolerance against allergen7,8, eradication of established tumors in mice9, inhibition and activation of natural killer cells10-12, promotion of differentiation into T regulatory cells13, stimulation of T cell proliferation14 and induction of T cell apoptosis15. Year 2007 we demonstrated that exosomes released from mast cells contain messenger RNA (mRNA) and microRNA (miRNA), and that the RNA can be shuttled from one cell to another via exosomes. In the recipient cells, the mRNA shuttled by exosomes was shown to be translated into protein, suggesting a regulatory function of the transferred RNA16. Further, we have also shown that exosomes derived from cells grown under oxidative stress can induce tolerance against further stress in recipient cells and thus suggest a biological function of the exosomal shuttle RNA17. Cell culture media and biological fluids contain a mixture of vesicles and shed fragments. A high quality isolation method for exosomes, followed by characterization and identification of the exosomes and their content, is therefore crucial to distinguish exosomes from other vesicles and particles. Here, we present a method for the isolation of exosomes from both cell culture medium and body fluids. This isolation method is based on repeated centrifugation and filtration steps, followed by a final ultracentrifugation step in which the exosomes are pelleted. Important methods to identify the exosomes and characterize the exosomal morphology and protein content are highlighted, including electron microscopy, flow cytometry and Western blot. The purification of the total exosomal RNA is based on spin column chromatography and the exosomal RNA yield and size distribution is analyzed using a Bioanalyzer.
机译:外来体研究领域正在迅速扩展,近年来出版物急剧增加。这些内吞起源的小囊泡(30-100 nm)首先被提出来作为网织细胞根除转铁蛋白受体同时成熟为红细胞 1 的一种方式,后来被称为外泌体。外来体是由晚期内体向内萌芽形成,产生多囊泡体(MVB),并通过MVB与质膜 2 融合而释放到环境中。自从首次发现外来体以来,已显示出广泛的细胞可释放这些囊泡。还已经在几种生物体液中检测到外来体,包括血浆,鼻灌洗液,唾液和母乳 3-6 。此外,已证明外泌体的含量和功能取决于原始细胞及其产生的条件。已证明外泌体具有多种功能,例如诱导对变应原 7,8 的耐受性,根除小鼠 9 中已建立的肿瘤,抑制和激活自然杀伤细胞 10-12 ,促进向T调节细胞的分化 13 ,刺激T细胞增殖 14 并诱导T细胞凋亡 15 。 2007年,我们证明了肥大细胞释放的外泌体包含信使RNA(mRNA)和微小RNA(miRNA),并且RNA可以通过外泌体从一种细胞转运到另一种细胞。在受体细胞中,外来体穿梭的mRNA被显示为翻译成蛋白质,表明转移的RNA 16 具有调节功能。此外,我们还表明,在氧化应激条件下生长的细胞衍生的外泌体可以诱导对受体细胞进一步胁迫的耐受性,因此表明外泌体穿梭RNA 17 的生物学功能。细胞培养基和生物体液包含囊泡和脱落的碎片的混合物。因此,一种高质量的外泌体分离方法,然后表征和鉴定外泌体及其含量,对于区分外泌体与其他囊泡和颗粒至关重要。在这里,我们提出了一种从细胞培养基和体液中分离外泌体的方法。该分离方法基于重复的离心和过滤步骤,然后是最终的超离心步骤,其中将外泌体制成颗粒。重点介绍了鉴定外泌体并表征外泌体形态和蛋白质含量的重要方法,包括电子显微镜,流式细胞仪和蛋白质印迹。总外泌体RNA的纯化基于旋转柱色谱,并使用生物分析仪分析外泌体RNA的产量和大小分布。

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