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Short-term lipopolysaccharide stimulation induces differentiation of murine bone marrow-derived dendritic cells into a tolerogenic phenotype.

机译:短期脂多糖刺激诱导小鼠骨髓来源的树突状细胞分化为耐受性表型。

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Dendritic cells (DCs) are professional, antigen-presenting cells, which induce and regulate T cell reactivity. DCs are crucial in innate and adaptive immune responses, and are also involved in central and peripheral tolerance induction. Tolerance can be mediated by immature and semi-mature DCs expressing low levels of co-stimulator and major histocompatibility complex (MHC) molecules. The aim of this study was to investigate the ability of short-term lipopolysaccharide (LPS) stimulation to modulate the stage of differentiation of bone marrow-derived DCs. For this purpose, DCs obtained from DBA1/lacJ mice were stimulated for four (4hLPS/DCs) or 24 (24hLPS/DCs) hours with LPS, using DCs without stimulation (0hLPS/DCs) as a control. Flow cytometry analysis of 4hLPS/DCs showed intermediate CD40 and MHC class II expression, lower than that of 24hLPS/DCs (fully mature), and greater than that of 0hLPS/DCs (immature). A functional assay showed that 4hLPS/DCs displayed increased endocytotic ability compared to 24hLPS/DCs, indicating a semi-mature state. 4hLPS/DCs were greater producers of IL-10 protein and TGFbeta1 mRNA than 24hLPS/DCs and immature DCs, displaying a cytokine production pattern that is characteristic of tolerogenic DCs. An assay for antigen-presenting capacity demonstrated that 4hLPS/DCs induced secretion of IL-2 from an OTH4 T cell hybridoma, indicating a functional presenting activity. Finally, the tolerogenic phenotype of 4hLPS/DCs was demonstrated by their ability to interfere with the progression of bovine type II collagen (bII)-induced arthritis (CIA) when they were loaded with bCII antigen and injected into mice with established CIA. We conclude that the stimulation of murine bone marrow-derived DCs with LPS for four hours generates semi-mature DCs with tolerogenic capability.
机译:树突状细胞(DC)是专业的抗原呈递细胞,可诱导和调节T细胞反应性。 DC在先天性和适应性免疫应答中至关重要,并且还参与中枢和外周耐受诱导。可以通过表达低水平的共刺激物和主要组织相容性复合物(MHC)分子的未成熟和半成熟DC介导耐受性。这项研究的目的是研究短期脂多糖(LPS)刺激调节骨髓来源DC分化阶段的能力。为此,使用不刺激的DC(0hLPS / DC)作为对照,使用LPS刺激从DBA1 / lacJ小鼠获得的DC四个小时(4hLPS / DC)或24(24hLPS / DCs)小时。 4hLPS / DC的流式细胞仪分析显示中等的CD40和MHC II类表达,低于24hLPS / DC(完全成熟)的表达,大于0hLPS / DC(未成熟)的表达。功能分析表明,与24hLPS / DC相比,4hLPS / DC显示出增加的内吞能力,表明其为半成熟状态。 4hLPS / DCs比24hLPS / DCs和未成熟DCs产生的IL-10蛋白和TGFbeta1 mRNA更大,显示出具有致耐受性DCs特征的细胞因子产生模式。抗原呈递能力的测定表明4hLPS / DCs诱导了OTH4 T细胞杂交瘤中IL-2的分泌,表明其具有功能性呈递活性。最后,当4hLPS / DC加载bCII抗原并注射入已建立CIA的小鼠中时,它们具有干扰牛II型胶原(bII)诱导的关节炎(CIA)进展的能力,从而证明了4hLPS / DC的耐受性表型。我们得出的结论是,用LPS刺激鼠类骨髓DC持续4小时会产生具有耐受力的半成熟DC。

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