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淋巴细胞调节分子的生化与生物学特性。V. 一株产生白细胞介素2的人白血病T细胞系的鉴定。

Biochemical and biological characterization of lymphocyte regulatory molecules. V. Identification of an interleukin 2-producing human leukemia T cell line.

作者信息

Gillis S, Watson J

出版信息

J Exp Med. 1980 Dec 1;152(6):1709-19. doi: 10.1084/jem.152.6.1709.

Abstract

To isolate a stable tumor cell line capable of producing human interleukin 2 (IL-2; formerly referred to as T cell growth factor), 16 human T and B leukemia cell lines were screened for constitutive and mitogen-stimulated IL-2 production. We found that the T cell leukemia line designated Jurkat-FHCRC produced > 200 U/ml of IL-2 activity after a 24-h stimulation with T cell mitogens. Peak mitogen-induced IL-2 activity was found in supernates harvested from 24-h Jurkat-FHCRC cell cultures stimulated with either 1% phytohemagglutinin or 20 microgram/ml concanavalin A. Addition of the fatty acid derivative phorbol myristate acetate to mitogen-stimulated cultures increased Jurkat-FHCRC IL-2 production to concentrations > 400 U/ml. IL-2 activity observed in such cases represented between 100--300 times that produced in conventional cultures of mitogen- or alloantigen-stimulated normal human peripheral blood or splenic lymphocytes. Jurkat-FHCRC-derived conditioned medium demonstrated equal capacity to promote the sustained in vitro proliferation of either murine or human activated T cell lines confirming the ability of Jurkat-FHCRC cells to produce human IL-2. These studies identify a new source of human IL-2 and establish a valuable reagent for the isolation and further molecular characterization of this immunoregulatory molecule.

摘要

为了分离出一种能够产生人白细胞介素2(IL-2;以前称为T细胞生长因子)的稳定肿瘤细胞系,对16种人T和B白血病细胞系进行了组成型和丝裂原刺激的IL-2产生情况筛查。我们发现,名为Jurkat-FHCRC的T细胞白血病细胞系在用T细胞丝裂原刺激24小时后产生的IL-2活性>200 U/ml。在用1%植物血凝素或20微克/毫升刀豆球蛋白A刺激24小时的Jurkat-FHCRC细胞培养物收获的上清液中发现了丝裂原诱导的IL-2活性峰值。向丝裂原刺激的培养物中添加脂肪酸衍生物佛波醇肉豆蔻酸酯可使Jurkat-FHCRC的IL-2产量增加到>400 U/ml的浓度。在这种情况下观察到的IL-2活性是丝裂原或同种异体抗原刺激的正常人外周血或脾淋巴细胞常规培养物中产生的活性的100 - 300倍。Jurkat-FHCRC来源的条件培养基显示出促进小鼠或人活化T细胞系体外持续增殖的同等能力,证实了Jurkat-FHCRC细胞产生人IL-2的能力。这些研究确定了人IL-2的一种新来源,并建立了一种有价值的试剂,用于分离和进一步对这种免疫调节分子进行分子表征。

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