Clayton A, Court J, Navabi H, Adams M, Mason M D, Hobot J A, Newman G R, Jasani B
Section of Clinical Oncology, University of Wales College of Medicine, Velindre Hospital, Whitchurch, Cardiff CF14 2TL, UK.
J Immunol Methods. 2001 Jan 1;247(1-2):163-74. doi: 10.1016/s0022-1759(00)00321-5.
We present a simple yet powerful method for the isolation and analysis of exosomes released by antigen-presenting cells (APC). Exosomes are small vesicles (40-90 nm) released by APC, and may have an immuno-regulatory function in vivo. Such exosomes originate from MHC class II peptide loading compartments and, as such, express high levels of MHC Class II. We have utilised magnetic beads, coated with monoclonal antibodies specific for HLA DP, DQ, DR for the specific isolation of exosomes from cell-free supernatants. Beads coated with exosomes are subsequently stained with conjugated antibodies, and analysed by flow cytometry. Characterisation of exosomes by this method demonstrated that exosomes derived from B-lymphocytes express abundant MHC Class I and II molecules. Other immunologically important molecules detected included the co-stimulatory molecules B7.1 (CD80) and B7.2 (CD86). The adhesion molecule ICAM-1 (CD54) was also detected. These exosomes also expressed the B cell marker CD20, and the complement inhibitory protein CD59. The expression of CD63, a lysosomal marker, was variable, and there was no detectable expression of transferrin receptor (CD71). Monocyte derived dendritic cells (cultured for 7 days in GM-CSF/IL-4), demonstrated an immature phenotype, and secreted exosomes with a similar phenotype, with abundant MHC molecules. The expression of CD63 was consistently strong, and the MHC Class I-like molecule CD1a was also present, suggesting a possible function in the presentation of lipid antigens. Again CD59 was expressed suggesting a possible role for APC exosomes in complement regulation. There was no detectable CD71, CD40, CD14, CD20 or CD83. Modification of the extraction protocol allowed a comparative analysis of exosome secretion under various conditions. Treatment of cells with calcium ionophore, or phorbol ester resulted in apparent increases in exosome release, while the phosphatidyl inositol 3-kinase inhibitor, wortmannin, reduced exosome secretion. The immuno-magnetic isolation and analysis of exosomes is a versatile and rapid tool for the analysis of APC exosomes, and may prove a valuable tool for the study of exosome biology.
我们提出了一种简单却强大的方法,用于分离和分析抗原呈递细胞(APC)释放的外泌体。外泌体是APC释放的小囊泡(40 - 90纳米),在体内可能具有免疫调节功能。此类外泌体起源于MHC II类肽装载区室,因此表达高水平的MHC II类分子。我们利用包被有针对HLA DP、DQ、DR的单克隆抗体的磁珠,从无细胞上清液中特异性分离外泌体。包被有外泌体的磁珠随后用偶联抗体染色,并通过流式细胞术进行分析。用这种方法对外泌体进行表征表明,源自B淋巴细胞的外泌体表达丰富的MHC I类和II类分子。检测到的其他免疫重要分子包括共刺激分子B7.1(CD80)和B7.2(CD86)。还检测到黏附分子ICAM - 1(CD54)。这些外泌体还表达B细胞标志物CD20和补体抑制蛋白CD59。溶酶体标志物CD63的表达存在差异,未检测到转铁蛋白受体(CD71)的表达。单核细胞衍生的树突状细胞(在GM - CSF/IL - 4中培养7天)表现出未成熟表型,并分泌具有类似表型且含有丰富MHC分子的外泌体。CD63的表达始终很强,且MHC I类样分子CD1a也存在,这表明其在脂质抗原呈递中可能具有功能。同样检测到CD59的表达,这表明APC外泌体在补体调节中可能发挥作用。未检测到CD71、CD40、CD14、CD20或CD83。提取方案的修改允许对不同条件下外泌体的分泌进行比较分析。用钙离子载体或佛波酯处理细胞导致外泌体释放明显增加,而磷脂酰肌醇3 -激酶抑制剂渥曼青霉素则减少外泌体分泌。外泌体的免疫磁珠分离和分析是一种用于分析APC外泌体的通用且快速的工具,可能成为外泌体生物学研究的有价值工具。
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