人单核细胞体外抑制淋巴因子激活的杀伤细胞扩增。

Molecular biotherapy Pub Date : 1991-03-01
P L Triozzi, W A Aldrich, J J Rinehart
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引用次数: 0

摘要

从人外周血单核细胞(PBMC)中消耗单核细胞增强了淋巴因子激活杀伤细胞(LAK)的体外活化。为了确定单核细胞是否也改变了lac细胞的扩增,我们评估了两种从PBMC中消耗单核细胞的方法:尼龙羊毛粘附(NWA)和苯丙氨酸甲酯(PME)处理。两种消耗单核细胞的方法都增强了白细胞介素-2 (IL-2)驱动的细胞增殖;然而,NWA耗尽后LAK的扩张明显大于PME。NWA和PME耗竭后LAK细胞毒性相当。单核细胞耗损程度(通过评估形态和Leu- m3 (CD14)阳性细胞的数量来确定)以及Leu 19 (CD56)、OKT-3 (CD3)、Leu (CD8)和Leu 3a (CD4)阳性细胞的增殖也相同。IL-2激活的细胞暴露于PME不改变其细胞毒性活性。然而,先用NWA,再用PME,或者先用PME,再用NWA治疗PBMC,会导致扩张减少。这种扩张的减少与PME单独治疗的PBMC相似。与单独使用NWA处理的细胞相比,将pme耗尽的细胞暴露于尼龙羊毛或从尼龙羊毛粘附的细胞中获得的上清液中进一步降低LAK的扩增。我们得出的结论是,即使在相对较低的细胞密度下,人单核细胞在IL-2驱动的PBMC培养中也能显著抑制lak细胞的扩增。此外,与PME治疗相比,NWA依从性对单核细胞的消耗更有效,这可能是由于后者治疗引起的细微细胞损伤。这些发现对IL-2在体外和体内产生的lak细胞具有重要意义。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Human monocytes inhibit lymphokine-activated killer cell expansion in vitro.

Depleting monocytes from human peripheral blood mononuclear cells (PBMC) enhances the in vitro activation of lymphokine-activated killer (LAK) cells. To determine if monocytes also altered LAK-cell expansion, we evaluated two methods of depleting monocytes from PBMC: nylon wool adherence (NWA) and phenylalanine methyl ester (PME) treatment. Both methods of depleting monocytes enhanced interleukin-2 (IL-2) driven, LAK-cell expansion; LAK expansion, however, was significantly greater after depletion with NWA than after PME. LAK cytotoxicity after NWA and PME depletion was equivalent. The degree of monocyte depletion, determined by evaluating morphology and the number of Leu-M3 (CD14) positive cells, and the proliferation of Leu 19 (CD56), OKT-3 (CD3), Leu2 (CD8), and Leu 3a (CD4) positive cells was also equivalent. Exposure of IL-2 activated cells to PME did not alter their cytotoxic activity. However, sequential treatment of PBMC with NWA, then PME, or with PME and then NWA, resulted in reduced expansion. This reduction in expansion was similar to PBMC treated with PME alone. Exposure of PME-depleted cells to nylon wool or to supernatants obtained from cells adherent to nylon wool further decreased LAK expansion relative to cells treated with NWA alone. We conclude that even at relatively low cell density, human monocytes markedly inhibit LAK-cell expansion in IL-2 driven PBMC cultures. Further, depletion of monocytes by NWA adherence is more effective than by treatment with PME, possibly due to subtle cellular damage induced by this latter treatment. These findings have implication for the in vitro and in vivo generation of LAK-cells by IL-2.

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