左旋咪唑满足CTLL-2细胞对巯基的需求,介导对有丝分裂原刺激的增强增殖反应,但不增加白细胞介素-2的产生。

N I Obiri, S L Dupere, S B Pruett, A Lackey, D Emma, T E O'Connor
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引用次数: 0

摘要

我们检测了左旋咪唑(LMS)对OKT3-、植物血凝素-和豆豆素- a刺激淋巴细胞增殖反应和白细胞介素-2 (IL-2)浓度的影响。虽然在LMS刺激下淋巴细胞增殖反应增强,但在刺激和未刺激的培养中观察到相似水平的IL-2。通过对培养的il -2依赖性CTLL-2细胞生长的影响,进一步表征LMS对增殖反应增强作用的机制。由于该细胞系已被证明需要2-巯基乙醇(2-ME)才能在重组IL-2中正常生长,因此将LMS对其生长的几个参数的影响与2-ME进行了比较。与2-ME不同,LMS没有增强35s -胱氨酸的摄取。这两种化合物都增加了细胞培养中的硫醇浓度,但(氧化)2-ME诱导了更大的增加。一般来说,LMS对CTLL-2生长的影响与已知结构无关的具有抗氧化特性的化合物非常相似,并且通过用LMS取代2-ME来满足该细胞系在重组IL-2中生长所证明的硫醇需求。当采用受体-配体结合实验检测LMS对CTLL-2细胞中IL-2受体(IL-2R)表达的影响时,低水平(10-80 pM)的125IL-2被观察到IL-2R表达水平适度增加。具有生物活性的高亲和力IL-2R复合物被认为优先结合在低水平的125IL-2上,这表明LMS的这种作用具有功能相关性。这些观察结果有助于降低过继免疫治疗中体外淋巴细胞扩增的成本和持续时间,也可用于改善免疫功能受损患者对免疫治疗的反应。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Levamisole meets sulfhydryl requirements of CTLL-2 cells and mediates enhanced proliferative response to mitogen stimulation without increasing interleukin-2 production.

We examined the effect of levamisole (LMS) on the proliferative response and interleukin-2 (IL-2) concentration in OKT3-, phytohemagglutinin-, and concanavalin-A-stimulated lymphocyte cultures. Although proliferative response was enhanced in lymphocyte cultures stimulated in the presence of LMS, similar levels of IL-2 were observed in stimulated and unstimulated cultures. The mechanism of the enhancement effect of LMS on proliferative response was further characterized by studying its effects on the growth of IL-2-dependent CTLL-2 cells in culture. Since this cell line has been shown to require 2-mercaptoethanol (2-ME) for normal growth in recombinant IL-2, the effect of LMS on several parameters of its growth was compared with that of 2-ME. Unlike 2-ME, LMS did not enhance 35S-cystine uptake. Both compounds increased thiol concentration in the cell culture, but (oxidized) 2-ME induced a greater increase. Generally, the effects of LMS on CTLL-2 growth were quite similar to those of structurally unrelated compounds known to have antioxidant properties, and the demonstrated thiol requirement of this cell line for growth in recombinant IL-2 was met by substituting LMS for 2-ME. When the effect of LMS on IL-2 receptor (IL-2R) expression in CTLL-2 cells was examined by a receptor-ligand binding assay involving low levels (10-80 pM) of 125IL-2, a modest increase in the level of IL-2R expression was observed. The biologically active high-affinity IL-2R complex is believed to be preferentially bound at the low levels of 125IL-2 used here, suggesting a functional relevance for this effect of LMS. These observations should be useful in minimizing the cost and duration of in vitro expansion of lymphocytes for use in adoptive immunotherapy and should be applicable in improving the response of immunologically impaired patients to immunotherapy.

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