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CHEMOKINE RECEPTOR 7 (CCR7)-EXPRESSION AND IFNγ PRODUCTION DEFINE VACCINE-SPECIFIC CANINE T CELL SUBSETS

机译:趋化因子受体7(CCR7)-表达和IFNγ产生确定的疫苗特异性犬T细胞亚群

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摘要

Canines suffer from and serve as strong translational animals models for many immunological disorders and infectious diseases. Routine vaccination has been a mainstay of protecting dogs through the stimulation of robust antibody responses and expansion of memory T cell populations. Commercially available reagents and described techniques are limited for identifying and characterizing canine T cell subsets and evaluating T cell-specific effector function. To define reagents for delineating naïve versus activated T cells and identify antigen-specific T cells, we tested anti-human and anti-bovine T-cell specific cell surface marker reagents for cross-reactivity with canine peripheral blood mononuclear cells (PBMCs. Both CD4+ and CD8+ T cells from healthy canine donors showed reactivity to CCL19-Ig, a CCR7 ligand, and coexpression with CD62L. An in vitro stimulation with concanavalin A validated downregulation of CCR7 and CD62L expression on stimulated healthy control PBMCs, consistent with an activated T cell phenotype. Anti-IFNγ antibodies identified antigen-specific IFNγ-producing CD4+ and CD8+ T cells upon in vitro vaccine antigen PBMC stimulation. PBMC isolation within 24 hours of sample collection allowed for efficient cell recovery and accurate T cell effector function characterization. These data provide a reagent and techniques platform via flow cytometry for identifying canine T cell subsets and characterizing circulating antigen-specific canine T cells for potential use in diagnostic and field settings.
机译:犬患有许多免疫性疾病和传染病,并成为其强有力的转化动物模型。常规疫苗接种一直是通过刺激强大的抗体应答和扩大记忆T细胞种群来保护狗的主要手段。市售试剂和描述的技术仅限于鉴定和表征犬T细胞亚群和评估T细胞特异性效应子功能。为了定义用于区分幼稚和活化T细胞的试剂并鉴定抗原特异性T细胞,我们测试了抗人和抗牛T细胞特异性细胞表面标志物试剂与犬外周血单个核细胞(PBMC)的交叉反应性。来自健康犬供体的 + 和CD8 + T细胞显示出与CCR7配体CCL19-Ig的反应性,并与CD62L共表达。伴刀豆球蛋白A的体外刺激证实了其下调CCR7和CD62L在刺激的健康对照PBMCs上的表达与活化的T细胞表型一致,抗IFNγ抗体鉴定了产生抗原特异性IFNγ的CD4 + 和CD8 + T细胞体外疫苗抗原PBMC刺激后,在样品采集后24小时内分离PBMC可实现有效的细胞回收和准确的T细胞效应子功能表征,这些数据提供了通过流式细胞术鉴定犬T细胞来源的试剂和技术平台并鉴定循环中的抗原特异性犬T细胞,以用于诊断和现场环境。

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