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评估基于流式细胞术的临床自然杀伤细胞活性检测方法。

Evaluation of a flow cytometry-based assay for natural killer cell activity in clinical settings.

机构信息

Department of Psychiatry & Behavioral Sciences, University of Miami Miller School of Medicine, Miami, FL 33136, USA.

出版信息

Scand J Immunol. 2012 Apr;75(4):455-62. doi: 10.1111/j.1365-3083.2011.02667.x.

Abstract

Natural killer (NK) cells are not only important in first line defence against viral and bacterial infections, but also in immune surveillance of malignant cells and thus NK cell cytotoxicity is primary indicator of immune function. Although chromium release assay is recognized as 'gold standard' for measuring NK cell activity, it has disadvantages like use of radioactive compounds, poor loading and high spontaneous release. It is difficult to perform this assay in clinical laboratory because of difficulties with disposal of radioactive waste and standardization problems. We describe a flow cytometry-based assay for the measurement of NK cell activity by incorporating fluorescent dye, DiO, into membranes of target cells. NK cell activity was measured at baseline, 1 and 4 weeks follow-up in 20 normal healthy individuals on a dietary supplement immunomodulator to enhance NK cell function. Mean baseline NK cell activity percentage (21.5; SD = 9.3) increased significantly to a maximum level at 1 week (31.3%; SD = 7.9; P = 0.007) and then returned to baseline level at 4 weeks (21.5; SD = 8.3). An important feature of flow cytometry-based assays is its ability to discriminate effector cells from target cells, and potential for explaining molecular interactions underlying target cell lysis. Under clinical settings, this assay will be of interest for frequently monitoring immunological status of patients on treatment for various diseases that affect their immune status. The assay is easy to perform without using radioactive material and thus could become a tool for monitoring pathogenesis and immune reconstitution.

摘要

自然杀伤 (NK) 细胞不仅在抵御病毒和细菌感染的第一线防御中很重要,而且在恶性细胞的免疫监视中也很重要,因此 NK 细胞的细胞毒性是免疫功能的主要指标。虽然铬释放试验被认为是测量 NK 细胞活性的“金标准”,但它也有一些缺点,如使用放射性化合物、负载不良和自发释放率高。由于放射性废物处理和标准化问题的困难,在临床实验室中很难进行这项检测。我们描述了一种基于流式细胞术的方法,通过将荧光染料 DiO 掺入靶细胞的膜中来测量 NK 细胞的活性。我们在 20 名正常健康个体的饮食补充免疫调节剂上测量了基线、1 周和 4 周时的 NK 细胞活性。NK 细胞活性的基线平均百分比(21.5;SD=9.3)在 1 周时显著增加到最高水平(31.3;SD=7.9;P=0.007),然后在 4 周时恢复到基线水平(21.5;SD=8.3)。流式细胞术检测的一个重要特点是能够区分效应细胞和靶细胞,并且能够解释导致靶细胞裂解的分子相互作用。在临床环境中,这种检测方法将对经常监测各种影响其免疫状态的疾病患者的免疫状态感兴趣。该检测方法易于操作,无需使用放射性物质,因此可能成为监测发病机制和免疫重建的工具。

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