Jong Ambrose Y, Wu Chun-Hua, Li Jingbo, Sun Jianping, Fabbri Muller, Wayne Alan S, Seeger Robert C
Children's Center for Cancer and Blood Diseases and Division of Hematology, Oncology and Blood & Marrow Transplantation, Department of Pediatrics, The Saban Research Institute, Children's Hospital Los Angeles, USC-Norris Comprehensive Cancer Center, Keck School of Medicine, University of Southern California , Los Angeles , CA , USA.
J Extracell Vesicles. 2017 Feb 28;6(1):1294368. doi: 10.1080/20013078.2017.1294368. eCollection 2017.
Extracellular vesicles (EVs) have been the focus of great interest, as they appear to be involved in numerous important cellular processes. They deliver bioactive macromolecules such as proteins, lipids, and nucleic acids, allowing intercellular communication in multicellular organisms. EVs are secreted by all cell types, including immune cells such as natural killer cells (NK), and they may play important roles in the immune system. Currently, a large-scale procedure to obtain functional NK EVs is lacking, limiting their use clinically. In this report, we present a simple, robust, and cost-effective method to isolate a large quantity of NK EVs. After propagating and activating NK cells and then incubating them in exosome-free medium for 48 h, EVs were isolated using a polymer precipitation method. The isolated vesicles contain the tetraspanin CD63, an EV marker, and associated proteins (fibronectin), but are devoid of cytochrome C, a cytoplasmic marker. Nanoparticle tracking analysis showed a size distribution between 100 and 200 nm while transmission electron microscopy imaging displayed vesicles with an oval shape and comparable sizes, fulfilling the definition of EV. Importantly, isolated EV fractions were cytotoxic against cancer cells. Furthermore, our results demonstrate for the first time that isolated activated NK (aNK) cell EVs contain the cytotoxic proteins perforin, granulysin, and granzymes A and B, incorporated from the aNK cells. Activation of caspase -3, -7 and -9 was detected in cancer cells incubated with aNK EVs, and caspase inhibitors blocked aNK EV-induced cytotoxicity, suggesting that aNK EVs activate caspase pathways in target cells. The ability to isolate functional aNK EVs on a large scale may lead to new clinical applications. : NK: natural killer cells; activated NK (aNK) cells; EVs: extracellular vesicles; ALL: acute lymphoblastic leukaemia; aAPC: artificial antigen-presenting cell; TEM: transmission electron microscope; PBMC: peripheral blood mononuclear cells; FBS: foetal bovine serum.
细胞外囊泡(EVs)一直是人们极大关注的焦点,因为它们似乎参与了众多重要的细胞过程。它们传递生物活性大分子,如蛋白质、脂质和核酸,从而在多细胞生物中实现细胞间通讯。所有细胞类型都会分泌EVs,包括自然杀伤细胞(NK)等免疫细胞,并且它们可能在免疫系统中发挥重要作用。目前,缺乏一种大规模获取功能性NK EVs的方法,这限制了它们在临床上的应用。在本报告中,我们提出了一种简单、可靠且经济高效的方法来分离大量的NK EVs。在扩增和激活NK细胞后,将它们在无外泌体培养基中孵育48小时,然后使用聚合物沉淀法分离EVs。分离出的囊泡含有四跨膜蛋白CD63(一种EV标志物)和相关蛋白(纤连蛋白),但不含细胞质标志物细胞色素C。纳米颗粒跟踪分析显示大小分布在100至200纳米之间,而透射电子显微镜成像显示囊泡呈椭圆形且大小相当,符合EV的定义。重要的是,分离出的EV组分对癌细胞具有细胞毒性。此外,我们的结果首次证明,分离出的活化NK(aNK)细胞EVs含有从aNK细胞整合而来的细胞毒性蛋白穿孔素、颗粒溶素以及颗粒酶A和B。在用aNK EVs孵育的癌细胞中检测到了半胱天冬酶-3、-7和-9的激活,并且半胱天冬酶抑制剂阻断了aNK EV诱导的细胞毒性,这表明aNK EVs激活了靶细胞中的半胱天冬酶途径。大规模分离功能性aNK EVs的能力可能会带来新的临床应用。:NK:自然杀伤细胞;活化NK(aNK)细胞;EVs:细胞外囊泡;ALL:急性淋巴细胞白血病;aAPC:人工抗原呈递细胞;TEM:透射电子显微镜;PBMC:外周血单核细胞;FBS:胎牛血清
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