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人单核细胞和树突状细胞作为T细胞复制辅助细胞的相对效能。

Relative efficacy of human monocytes and dendritic cells as accessory cells for T cell replication.

作者信息

Van Voorhis W C, Valinsky J, Hoffman E, Luban J, Hair L S, Steinman R M

出版信息

J Exp Med. 1983 Jul 1;158(1):174-91. doi: 10.1084/jem.158.1.174.

Abstract

Monocyte-specific monoclonal antibodies (7) were used to compare the efficacy of monocytes and dendritic cells as accessory or stimulator cells for human T cell replication. Both unfractionated and plastic-adherent mononuclear cells were first treated with a cytolytic antimonocyte antibody that kills greater than 95% of monocytes but not dendritic cells. When tested as stimulators of the mixed leukocyte reaction (MLR) and of oxidative mitogenesis (the proliferation of T cells modified with sodium periodate), the monocyte-depleted cells had normal or enhanced stimulatory capacity. Monocyte-depleted mononuclear cells also proliferated normally to soluble antigens (Candida albicans, tetanus toxoid), even under limiting conditions of cell dose, antigen dose, and culture time. Adherent blood mononuclear cells were next separated into monocyte-enriched and -depleted components using fluoresceinated antimonocyte antibody and the cell sorter. The depleted fraction (less than 2% monocytes by esterase staining and by cytology) contained the dendritic cells and exhibited at least 75% of the accessory activity. The monocyte-rich fraction (approximately 97% esterase positive) stimulated the MLR and oxidative mitogenesis weakly, and was comparable in potency to nonadherent cells. Cell-specific antibodies and complement were also used to prepare dendritic cells that were thoroughly depleted of monocytes and lymphocytes. The dendritic cells (70-80% pure) were potent stimulators of the allogeneic MLR, syngeneic MLR, and tetanus toxoid response, being active at stimulator to responder ratios of 1:100 or less. Taken together with previous studies (1, 2), these experiments indicate that the dendritic cell is the major stimulator of T cell replication in man. The contribution of class II products of the major histocompatibility complex (7) was then evaluated with a new monoclonal, 9.3F10. Accessory function was dramatically inhibited if cells bearing class II antigens were killed with 9.3F10 and complement, or if class II molecules were blocked by the addition of 9.3F10 Fab to the culture medium. The expression of 9.3F10 class II products was therefore studied on purified monocytes and dendritic cells. Most if not all cells in both populations reacted with 9.3F10, and each population exhibited approximately 150,000 125I-Fab 9.3F10 binding sites per cell. Since Ia+ dendritic cells are active accessory cells, but Ia+ monocytes are not, class II products are necessary but not sufficient for the stimulation of T cell proliferation in man.

摘要

使用单核细胞特异性单克隆抗体(7种)比较单核细胞和树突状细胞作为人T细胞增殖的辅助细胞或刺激细胞的功效。未分离的和贴壁单核细胞首先用溶细胞抗单核细胞抗体处理,该抗体可杀死超过95%的单核细胞,但不杀死树突状细胞。当作为混合淋巴细胞反应(MLR)和氧化有丝分裂(经高碘酸钠修饰的T细胞增殖)的刺激剂进行测试时,单核细胞耗竭的细胞具有正常或增强的刺激能力。单核细胞耗竭的单核细胞即使在细胞剂量、抗原剂量和培养时间的限制条件下,对可溶性抗原(白色念珠菌、破伤风类毒素)也能正常增殖。接下来,使用荧光素化抗单核细胞抗体和细胞分选仪将贴壁血单核细胞分离为富含单核细胞和单核细胞耗竭的组分。耗竭组分(通过酯酶染色和细胞学检查单核细胞少于2%)含有树突状细胞,并表现出至少75%的辅助活性。富含单核细胞的组分(约97%酯酶阳性)对MLR和氧化有丝分裂的刺激作用较弱,其效力与非贴壁细胞相当。还使用细胞特异性抗体和补体制备完全不含单核细胞和淋巴细胞的树突状细胞。这些树突状细胞(纯度为70 - 80%)是同种异体MLR、同基因MLR和破伤风类毒素反应的有效刺激剂,在刺激剂与反应剂比例为1:100或更低时仍具有活性。与先前的研究(1, 2)一起,这些实验表明树突状细胞是人类T细胞增殖的主要刺激剂。然后用一种新的单克隆抗体9.3F10评估主要组织相容性复合体(7种)II类产物的作用。如果用9.3F10和补体杀死携带II类抗原的细胞,或者通过向培养基中添加9.3F10 Fab来阻断II类分子,则辅助功能会受到显著抑制。因此,研究了纯化的单核细胞和树突状细胞上9.3F10 II类产物的表达。两个群体中的大多数(如果不是全部)细胞都与9.3F10反应,每个群体的细胞均表现出约150,000个125I - Fab 9.3F10结合位点。由于Ia +树突状细胞是活跃的辅助细胞,而Ia +单核细胞不是,因此II类产物对于人类T细胞增殖的刺激是必要的,但不是充分的。

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