Interleukin-10 increases mannose receptor expression and endocytic activity in monocyte-derived dendritic cells.

D Longoni, L Piemonti, S Bernasconi, A Mantovani, P Allavena
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引用次数: 51

Abstract

Human monocyte-derived dendritic cells were differentiated in vitro for 7 days with granulocyte macrophage-colony stimulating factor and interleukin-13. These cultured dendritic cells are at an immature stage of differentiation and exhert high endocytic activity via surface mannose receptor and via fluid-phase macropinocytosis. We have investigated the modulation of endocytosis by interleukin-10 in these cells. When added during the last 24 h of the 7-day culture, interleukin-10 significantly stimulated the uptake of fluorescein-labelled dextran (39 +/- 16% increase, mean +/- SD of 6 experiments), a sugar binding to the mannose receptor. This effect was dose dependent and correlated with the length of exposure to interleukin-10, with a maximal effect (more than seven-fold increase) when the cytokine was added at the beginning of the culture (day 0). The interleukin-10-increased fluorescein-labelled-dextran endocytosis was mostly mediated via the mannose receptor, as unlabelled mannose and specific antimannose receptor monoclonal antibody inhibited most of the uptake. Moreover, interleukin-10-treated cells expressed increased levels (up to four-fold) of mannose receptor. Interleukin-10 also increased, although to a lesser extent, the fluid-phase endocytosis (macropinocytosis) of fluorescein-labelled albumin. Interleukin-10 had the opposite effect on the differentiation and functional activity of monocyte-derived dendritic cells; cells having a very low stimulatory capacity and reduced expression of MHC class II and CD1a after a 7-day exposure. Thus interleukin-10 had a strong immunosuppressive effect on the differentiation and functional activity of monocyte-derived dendritic cells and yet strongly stimulated endocytosis in these cells. We speculate that an increased endocytic activity would eventually result in a decreased availability of antigens in the external milieu, thus contributing to the immunosuppressive and tolerogenic activity of interleukin-10.

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白细胞介素-10增加甘露糖受体的表达和单核细胞来源的树突状细胞的内吞活性。
用粒细胞巨噬细胞集落刺激因子和白细胞介素-13体外分化人单核细胞来源的树突状细胞7天。这些培养的树突状细胞处于分化的未成熟阶段,并通过表面甘露糖受体和液相巨饮作用分泌出高的内吞活性。我们研究了白细胞介素-10对这些细胞内吞作用的调节。当在7天培养的最后24小时添加白介素-10时,白介素-10显著刺激了荧光素标记的葡聚糖的摄取(增加39 +/- 16%,6个实验的平均+/- SD),葡聚糖是一种与甘露糖受体结合的糖。这种效应是剂量依赖性的,与暴露于白介素-10的时间有关,在培养开始时(第0天)加入细胞因子时,效果最大(增加7倍以上)。白介素-10增加的荧光素标记的葡聚糖内吞作用主要通过甘露糖受体介导,因为未标记的甘露糖和特异性抗甘露糖受体单克隆抗体抑制了大部分摄取。此外,白细胞介素-10处理的细胞表达的甘露糖受体水平增加(高达四倍)。白细胞介素-10也增加了荧光素标记白蛋白的液相内吞作用(巨噬细胞作用),尽管程度较轻。白细胞介素-10对单核细胞来源的树突状细胞的分化和功能活性有相反的影响;暴露7天后,细胞具有非常低的刺激能力,MHC II类和CD1a的表达减少。因此,白细胞介素-10对单核细胞来源的树突状细胞的分化和功能活性有很强的免疫抑制作用,但强烈刺激这些细胞的内吞作用。我们推测,内吞活性的增加最终会导致抗原在外部环境中的可用性降低,从而促进白细胞介素-10的免疫抑制和耐受性活性。
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