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从人外周血单个核细胞体外生成抗原特异性溶血空斑形成细胞。

In vitro generation of antigen-specific hemolytic plaque-forming cells from human peripheral blood mononuclear cells.

作者信息

Misiti J, Waldmann T A

出版信息

J Exp Med. 1981 Oct 1;154(4):1069-84. doi: 10.1084/jem.154.4.1069.

Abstract

We have described a culture and assay system for the sensitization of human peripheral blood mononuclear cells with a T cell-dependent antigen, sheep erythrocytes, in the absence of nonspecific stimulatory agents and with the subsequent generation of macroscopic hemolytic plaques. We have shown that the antibody produced by the plaque-forming cells generated in this culture system is specific for the sensitizing antigen, and that the plaques created are not false plaques because their formation is inhibited by cycloheximide. The success of this system can be attributed to several critical factors including large numbers of peripheral blood mononuclear cells (5 x 10(6) culture), a prolonged period of incubation (10-11 d), continuous rocking during the entire period of incubation, culturing in large (35-mm) flat-bottomed culture dishes in the presence of human plasma, and the appropriate antigen concentration (5 x 10(6) sheep erythrocytes/culture). Furthermore, the generation of macroscopic hemolytic plaques requires plaquing sensitized peripheral blood mononuclear cells in target cell monolayers fixed in an agarose matrix with an incubation period of 2-3 h. We have further shown that the antigen-specific response measured by this system is dependent on adherent cells and T lymphocytes. At least one population of the helper T cells is sensitive to 2,000 rad irradiation. This system is simple, sensitive, and should serve as an effective tool for the analysis of cellular interactions involved in the generation of human antigen-specific plaque-forming cells, the genetic control the human immune response, and the pathophysiology of altered immunoregulation in disease.

摘要

我们描述了一种培养和检测系统,用于在不存在非特异性刺激剂的情况下,用T细胞依赖性抗原绵羊红细胞对人外周血单个核细胞进行致敏,并随后产生肉眼可见的溶血空斑。我们已经表明,在该培养系统中产生的空斑形成细胞所产生的抗体对致敏抗原具有特异性,并且所形成的空斑不是假空斑,因为其形成受到环己酰亚胺的抑制。该系统的成功可归因于几个关键因素,包括大量的外周血单个核细胞(5×10⁶个/培养物)、延长的孵育期(10 - 11天)、整个孵育期间持续摇晃、在人血浆存在下于大的(35毫米)平底培养皿中培养以及适当的抗原浓度(5×10⁶个绵羊红细胞/培养物)。此外,产生肉眼可见的溶血空斑需要将致敏的外周血单个核细胞铺在固定于琼脂糖基质中的靶细胞单层上,并孵育2 - 3小时。我们还进一步表明,通过该系统测量的抗原特异性反应依赖于贴壁细胞和T淋巴细胞。至少一群辅助性T细胞对2000拉德辐射敏感。该系统简单、灵敏,应可作为一种有效工具,用于分析参与人抗原特异性空斑形成细胞产生、人类免疫反应的遗传控制以及疾病中免疫调节改变的病理生理学的细胞间相互作用。

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