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Influence of Specimen Age and Use of Different Negative Controls in Determination of Intracytoplasmic Levels of Cytokines after Whole-Blood Culture Assay

机译:全血培养后标本年龄和使用不同阴性对照对细胞因子胞浆内水平测定的影响

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摘要

Intracytoplasmic detection of cytokines by flow cytometry has become a powerful tool in the characterization of cytokine-producing cells. However, it is not known to what extent specimen age and the use of various negative controls may influence the amount of cytokine-positive cells. We therefore compared different times of storage and the use of several negative controls in the determination of intracytoplasmic levels of cytokines. There was a substantial decline of interleukin-2- and gamma interferon-positive lymphocytes after 20 h and especially after 48 h of storage. The precision of intracytoplasmic interleukin-6 determination decreases after long-term storage compared to 2 h of storage, whereas the amount of interleukin-8-positive monocytes remained rather stable. Therefore, we recommend performing the analysis as fast as possible after the blood sample is drawn. Under consideration of isotype-matched antibodies and nonstimulated cells as negative controls instead of the purified antibody-blocking control, strikingly higher amounts of interleukin-2-, gamma interferon, interleukin-6-, and interleukin-8-positive cells were found. For a meaningful interpretation of data these differences have to be kept in mind. Further studies should evaluate the exact specificity of these controls.
机译:通过流式细胞术对细胞因子进行胞质内检测已成为表征细胞因子产生细胞的有力工具。但是,尚不清楚样品的年龄和使用各种阴性对照在多大程度上会影响细胞因子阳性细胞的数量。因此,我们比较了不同的储存时间和使用几种阴性对照来确定细胞因子的胞浆内水平。 20小时后,特别是在48小时后,白介素2和γ干扰素阳性淋巴细胞明显减少。长期保存后,与保存2 h相比,胞浆中白细胞介素6的测定精度降低,而白细胞介素8阳性单核细胞的数量则保持稳定。因此,我们建议在抽取血液样本后尽快执行分析。在考虑同种型匹配的抗体和未刺激的细胞作为阴性对照而不是纯化的抗体阻断对照的情况下,发现白细胞介素-2,γ干扰素,白介素-6和白介素8阳性细胞的数量明显更高。为了对数据进行有意义的解释,必须牢记这些差异。进一步的研究应评估这些对照的确切特异性。

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