[Cytokine measurement using a multiplex technique with spectral flow cytometry: application in the study of the immunobiology of ascariasis].

Ana Lozano, Carolina Sánchez-Marrugo, Kevin Llinás-Caballero, Carlos Barrios, Nathalie Acevedo, Josefina Zakzuk, Luis Caraballo
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Abstract

Objective: To quantify the production of Th1/Th2/Th17 cytokines induced by Ascaris lumbricoides antigens in peripheral blood mononuclear cells (PBMCs) using a multiplex technique.

Methods: PBMCs were cultured from individuals with mild A. lumbricoides infection (n = 20) and uninfected individuals (n = 21) and stimulated with A. lumbricoides extract (ExtAscaris), a mix of anti-CD2/CD3/CD28 (CDmix) as a positive control, and only medium (negative control). Cytokines in the supernatants were measured using the BD™ Cytometric Bead Array Human Th1/Th2/Th17 kit, to identify IFN-γ, TNF, IL-10, IL-6, IL-4, IL-2, and IL-17A. Readings were taken on a spectral cytometer (Northern Lights, Cytek, USA), and analysis was performed using R software with packages "tidyverse," "beadplexr," "flowCore," and "arsenal." Cytokine concentrations were calculated using a 5-parameter logistic curve. The t-test was used to compare cases and controls, and statistical significance was set at p < 0.05. The study was approved by the Ethics Committee of the University of Cartagena and the participants provided informed consent. This study was financially supported by the Colombian Sistema General de Regalías under the BPIN2020000100405 - BPIN2020000100364.

Results: Efficient fluorescence intensity extraction for each cytokine was achieved using detection channel R8 and the "mclust" clustering model (Figure 1). No significant differences were found in the levels of the seven cytokines between cases and controls (Figure 2). Although the IFN-γ response to ExtAscaris was higher in cases than in controls (252.5 ng/mL vs. 173.1 ng/mL), the difference was not significant. IL-17A (detection limit: 18.9 pg/mL) was more detectable in cases than controls (5 cases, 23% vs. 2 controls, 9.5%). IL-4 was only detected in the supernatants from CDmix-stimulated cultures but not with the Ascaris extract (Figure 2).

Conclusions: The multiplex technique using spectral flow cytometry combined with open-source software analysis proved applicable for quantifying cytokines induced by A. lumbricoides antigens in PBMCs. However, a more sensitive method is needed to evaluate IL-4 response in the context of ascariasis. The results did not reveal significant differences in cytokine production between cases and controls for the evaluated stimuli.

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[使用光谱流式细胞仪的多重技术测量细胞因子:在蛔虫病免疫生物学研究中的应用]。
目的采用多重技术定量检测外周血单核细胞(PBMCs)中由蛔虫抗原诱导产生的 Th1/Th2/Th17 细胞因子:方法:培养轻度蛔虫感染者(n = 20)和未感染者(n = 21)的外周血单核细胞,用蛔虫提取物(ExtAscaris)、作为阳性对照的抗 CD2/CD3/CD28 混合液(CDmix)和仅用培养基(阴性对照)进行刺激。使用 BD™ Cytometric Bead Array Human Th1/Th2/Th17 试剂盒检测上清液中的细胞因子,以确定 IFN-γ、TNF、IL-10、IL-6、IL-4、IL-2 和 IL-17A。在光谱细胞计数器(Northern Lights,美国赛泰克公司)上读取数据,并使用 R 软件包 "tidyverse"、"beadplexr"、"flowCore "和 "arsenal "进行分析。细胞因子浓度用 5 参数逻辑曲线计算。病例与对照组的比较采用t检验,统计学意义以p < 0.05为标准。该研究获得了卡塔赫纳大学伦理委员会的批准,参与者也提供了知情同意书。本研究得到了哥伦比亚政府总系统(BPIN2020000100405 - BPIN2020000100364)的资助:使用检测通道 R8 和 "mclust "聚类模型(图 1)对每种细胞因子进行了高效的荧光强度提取。病例与对照组之间的七种细胞因子水平无明显差异(图 2)。虽然病例对 ExtAscaris 的 IFN-γ 反应高于对照组(252.5 纳克/毫升对 173.1 纳克/毫升),但差异并不显著。病例比对照组更容易检测到 IL-17A(检测限:18.9 pg/mL)(5 例病例,23% 对 2 例对照组,9.5%)。IL-4只在CDmix刺激培养物的上清液中检测到,而在蛔虫提取物中检测不到(图2):使用光谱流式细胞仪结合开源软件分析的多重技术证明适用于定量检测 PBMCs 中蛔虫抗原诱导的细胞因子。不过,还需要一种更灵敏的方法来评估蛔虫病中的 IL-4 反应。结果显示,病例与对照组在所评估的刺激因素下产生的细胞因子没有明显差异。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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