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A simple and sensitive flow cytometric assay for the determination of the cytotoxic activity of human natural killer cells

机译:一种简单灵敏的流式细胞仪检测方法,用于测定人体自然杀伤细胞的细胞毒活性

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摘要

A new, simple and sensitive flow cytometric assay for the determination of the cytotoxic activity of human natural killer cells is described. The assay is based on the use of two fluorochromes. The target cell population is stained with one fluorochrome (octadecylamine-fluorescein isothiocyanate, F-18) prior to incubation with the effector cells. F-18 remains in the membrane of the target cells even when they are killed thereby permitting a clear separation between effector and target cells. Dead cells are determined by staining with a second fluorochrome (propidium iodide) after incubation of effector and target cells.udF-18 is not toxic and does not decrease the cytotoxic activity of human natural killer cells. It is also stable (exchange between labeled and non-labeled cells is negligible in a period of at least 4 h at 37°C) and it remains in the membrane of the killed cells. A clear distinction between unlabeled effector and labeled target cells is obtained, even after incubation of target and effector cells for 4 h at 37°C and using a high effector cell-target cell ratio (75:1). A good correlation with the 51Cr release assay was obtained.udA potential application of the flow cytometric cytotoxicity assay using whole blood instead of isolated lymphocytes is presented.udud
机译:描述了一种新的,简单而灵敏的流式细胞术测定法,用于测定人自然杀伤细胞的细胞毒活性。该测定基于两种荧光染料的使用。在与效应细胞孵育之前,将靶细胞群体用一种荧光染料(十八烷基胺-荧光素异硫氰酸酯,F-18)染色。即使被杀死,F-18仍保留在靶细胞的膜中,从而使效应子与靶细胞之间清晰分离。孵育效应细胞和靶细胞后,通过用第二种荧光染料(碘化丙啶)染色确定死细胞。 udF-18无毒,不会降低人类自然杀伤细胞的细胞毒活性。它也是稳定的(在37°C至少4小时内标记和未标记细胞之间的交换可以忽略不计),并且它保留在被杀死细胞的膜中。即使将目标细胞和效应细胞在37°C下孵育4小时并使用高效应细胞-靶细胞比例(75:1),也可以清楚地区分未标记的效应细胞和标记的靶细胞。获得了与51Cr释放测定的良好相关性。 ud提出了使用全血代替分离的淋巴细胞进行流式细胞术细胞毒性测定的潜在应用。 ud ud

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