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人外周血中活化的T细胞:用反向溶血空斑试验进行定量分析。

Activated T cells in human peripheral blood: quantitation with a reverse hemolytic plaque assay.

作者信息

Cohen P L, Litvin D A, Winfield J B

出版信息

J Immunol. 1981 Nov;127(5):1777-81.

PMID:7028863
Abstract

Rabbit antiserum to culture supernatant of concanavalin A-stimulated peripheral blood mononuclear cells was used in a reverse hemolytic plaque assay to detect activated T lymphocytes in human peripheral blood. The number of plaque-forming cells in fresh, unstimulated lymphocyte preparations was approximately 400/10(6) cells, and increased 7- to 14-fold after stimulation with a variety of mitogens and antigens. The kinetics of the increase paralleled 3H-thymidine incorporation, with a maximum on day 3 of culture. Plaques were eliminated by treatment of cells with anti-Leu-I + complement or by depletion of E-rosettes. The activated T cells were not restricted to a given inducer, suppressor, or Ia+ T cell subset, however. Both mitogen-stimulated culture supernatants and mitogen-activated lymphocytes, but not resting lymphocytes, were effective in absorbing the capacity of the rabbit antiserum to develop plaques. This suggested that the predominant specificity of this antiserum was directed toward surface membrane determinant(s) of T cells actively shed into the medium. This process was shown to require ongoing protein synthesis, and, in mitogen-stimulated lymphocyte preparations, DNA synthesis as well. This approach has enabled detection of a surprisingly large number of endogenously activated T cells in normal human blood, and should be useful for the analysis of immunoregulatory events at the single-cell level.

摘要

用针对伴刀豆球蛋白A刺激的外周血单核细胞培养上清液的兔抗血清,通过反向溶血空斑试验检测人外周血中的活化T淋巴细胞。新鲜的、未受刺激的淋巴细胞制剂中的空斑形成细胞数量约为400/10⁶细胞,在用多种丝裂原和抗原刺激后增加了7至14倍。增加的动力学与³H-胸腺嘧啶核苷掺入平行,在培养第3天达到最大值。通过用抗Leu-I +补体处理细胞或通过去除E花环来消除空斑。然而,活化的T细胞并不局限于特定的诱导型、抑制型或Ia⁺ T细胞亚群。丝裂原刺激的培养上清液和丝裂原活化的淋巴细胞,但静止淋巴细胞无效,均能有效吸收兔抗血清形成空斑的能力。这表明该抗血清的主要特异性针对主动释放到培养基中的T细胞表面膜决定簇。该过程显示需要持续的蛋白质合成,并且在丝裂原刺激的淋巴细胞制剂中也需要DNA合成。这种方法能够检测正常人血液中数量惊人的内源性活化T细胞,并且应该有助于在单细胞水平分析免疫调节事件。

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