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Influence of nasal polyp tissue on the differentiation and activation of T lymphocytes in a co-culture system

机译:鼻息肉组织对共培养系统中T淋巴细胞分化和活化的影响

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摘要

Abstract: T cell subpopulations in nasal polyps differ from peripheral lymphocytes in patients with chronic rhinosinusitis with nasal polyps (CRSwNP). However, little is known about the modulatory influence of the inflamed nasal polyp epithelial cells on the phenotype of the T cells. The aim of the present study was to assess this interaction. Tissue and blood samples were collected from 16 patients undergoing paranasal sinus surgery. Polypoid tissue was cultured under air-liquid interface conditions. Subsequently, cluster of differentiation (CD)3/CD28 activated peripheral lymphocytes from the same patients were added. After 3 days lymphocytes were separated from co-culture and analyzed by multicolor flow cytometry. Additionally, cytokine expression of the polyp tissue was measured using a human T helper cell (TH)1/TH2/TH17 antibody array. Viability staining of CD3+ lymphocytes detected fewer apoptotic cells under co-culture conditions compared with in mono-culture. There was a significantly higher frequency of CD4+ and CD8+ T cells in the co-culture system than in PBMC culture alone. Human leukocyte antigen (HLA)-DR isotype was significantly downregulated on co-cultured CD3+ lymphocytes and CD3+CD4+ T cells compared with the mono-cultured counterparts. Conventional Forkhead box P3- memory CD4+ T cells and activated regulatory T cells increased in frequency, and resting regulatory T cells decreased in the co-culture. Cytokine analysis identified expression of interleukin (IL)-6, IL-6 receptor, granulocyte-macrophage colony-stimulating factor, transforming growth factor-β and macrophage inflammatory protein-3 in the polyp tissue. In summary, the present study performed a comparison between peripheral lymphocytes cultured with and without nasal polyp tissue cells was performed. The downregulation of HLA and the differentiation of Treg and Tconv by nasal polypoid tissue on PBMCs was demonstrated. Interestingly, the in vivo downregulation of HLA-DR on CD3+ lymphocytes, as reported previously, was confirmed in vitro. The inhibitory effect of polypoid tissue on the activation of lymphocytes is a possible pathogenic mechanism underlying CRSwNP.
机译:摘要:慢性鼻窦炎伴鼻息肉(CRSwNP)患者的鼻息肉中的T细胞亚群不同于外周淋巴细胞。然而,关于鼻息肉上皮发炎细胞对T细胞表型的调节作用了解甚少。本研究的目的是评估这种相互作用。收集了16名接受鼻旁窦手术的患者的组织和血液样本。在气液界面条件下培养息肉样组织。随后,添加了来自同一患者的分化簇(CD)3 / CD28激活的外周淋巴细胞。 3天后,从共培养物中分离淋巴细胞,并通过多色流式细胞术进行分析。另外,使用人类T辅助细胞(TH)1 / TH2 / TH17抗体阵列测量息肉组织的细胞因子表达。与单培养相比,共培养条件下CD3 + 淋巴细胞的活力染色检测到较少的凋亡细胞。共培养系统中CD4 + 和CD8 + T细胞的频率明显高于单独的PBMC培养。与CD3 + 淋巴细胞和CD3 + CD4 + T细胞共培养相比,人白细胞抗原(HLA)-DR同种型显着下调。单一文化的同行。常规叉头盒P3 -记忆CD4 + T细胞和活化的调节性T细胞的频率增加,而静息的调节性T细胞在共培养物中减少。细胞因子分析确定了息肉组织中白介素(IL)-6,IL-6受体,粒细胞-巨噬细胞集落刺激因子,转化生长因子-β和巨噬细胞炎性蛋白3的表达。总而言之,本研究进行了在有和没有鼻息肉组织细胞培养的外周淋巴细胞之间的比较。证实了鼻息肉样组织在PBMCs上HLA的下调以及Treg和Tconv的分化。有趣的是,如先前报道的,在体外证实了HLA-DR在CD3 + 淋巴细胞上的体内下调。息肉样组织对淋巴细胞活化的抑制作用是CRSwNP潜在的致病机制。

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