Center for Translational Immunology, University Medical Center Utrecht (UMC Utrecht), Utrecht, Netherlands.
Hubrecht Institute, Utrecht, Netherlands.
Front Immunol. 2023 Jan 4;13:1101999. doi: 10.3389/fimmu.2022.1101999. eCollection 2022.
Dendritic cells (DC) are crucial for initiating and shaping immune responses. So far, little is known about the functional specialization of human DC subsets in (local) inflammatory conditions. We profiled conventional (c)DC1, cDC2 and monocytes based on phenotype, transcriptome and function from a local inflammatory site, namely synovial fluid (SF) from patients suffering from a chronic inflammatory condition, Juvenile Idiopathic Arthritis (JIA) as well as patients with rheumatoid arthritis (RA).
Paired PB and SF samples from 32 JIA and 4 RA patients were collected for mononuclear cell isolation. Flow cytometry was done for definition of antigen presenting cell (APC) subsets. Cell sorting was done on the FACSAria II or III. RNA sequencing was done on SF APC subsets. Proliferation assays were done on co-cultures after CD3 magnetic activated cell sorting (MACS). APC Toll-like receptor (TLR) stimulation was done using Pam3CSK4, Poly(I:C), LPS, CpG-A and R848. Cytokine production was measured by Luminex.
cDC1, a relatively small DC subset in blood, are strongly enriched in SF, and showed a quiescent immune signature without a clear inflammatory profile, low expression of pathogen recognition receptors (PRRs), chemokine and cytokine receptors, and poor induction of T cell proliferation and cytokine production, but selective production of IFNλ upon polyinosinic:polycytidylic acid exposure. In stark contrast, cDC2 and monocytes from the same environment, showed a pro-inflammatory transcriptional profile, high levels of (spontaneous) pro-inflammatory cytokine production, and strong induction of T cell proliferation and cytokine production, including IL-17. Although the cDC2 and monocytes showed an overlapping transcriptional core profile, there were clear differences in the transcriptional landscape and functional features, indicating that these cell types retain their lineage identity in chronic inflammatory conditions.
Our findings suggest that at the site of inflammation, there is specific functional programming of human DCs, especially cDC2. In contrast, the enriched cDC1 remain relatively quiescent and seemingly unchanged under inflammatory conditions, pointing to a potentially more regulatory role.
树突状细胞 (DC) 对于启动和塑造免疫反应至关重要。到目前为止,人们对人类 DC 亚群在(局部)炎症条件下的功能特化知之甚少。我们基于表型、转录组和功能,从局部炎症部位(即患有慢性炎症性疾病的患者的滑液 (SF))对常规 (c)DC1、cDC2 和单核细胞进行了分析,即患有青少年特发性关节炎 (JIA) 的患者以及患有类风湿性关节炎 (RA) 的患者。
从 32 名 JIA 和 4 名 RA 患者中采集配对的 PB 和 SF 样本用于单核细胞分离。流式细胞术用于定义抗原呈递细胞 (APC) 亚群。细胞分选在 FACSAria II 或 III 上进行。对 SF APC 亚群进行 RNA 测序。在 CD3 磁激活细胞分选 (MACS) 后进行共培养的增殖测定。使用 Pam3CSK4、Poly(I:C)、LPS、CpG-A 和 R848 对 APC Toll 样受体 (TLR) 进行刺激。通过 Luminex 测量细胞因子产生。
cDC1 是血液中相对较小的 DC 亚群,在 SF 中强烈富集,表现出静止的免疫特征,没有明显的炎症特征,病原体识别受体 (PRR)、趋化因子和细胞因子受体表达水平低,诱导 T 细胞增殖和细胞因子产生能力差,但在暴露于聚肌苷酸:聚胞苷酸时选择性产生 IFNλ。相比之下,来自同一环境的 cDC2 和单核细胞表现出促炎转录谱,高水平的(自发)促炎细胞因子产生,以及强烈诱导 T 细胞增殖和细胞因子产生,包括 IL-17。尽管 cDC2 和单核细胞表现出重叠的转录核心谱,但在转录谱和功能特征上存在明显差异,这表明这些细胞类型在慢性炎症条件下保持其谱系身份。
我们的研究结果表明,在炎症部位,人类 DC 特别是 cDC2 具有特定的功能编程。相比之下,在炎症条件下,丰富的 cDC1 仍然相对静止,似乎没有变化,这表明其可能具有更具调节作用。
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