新鲜人血单核细胞与肿瘤靶点在单细胞水平上的相互作用:结合和形态特征。

K E Muse, H S Koren
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引用次数: 0

摘要

高纯度(97-99%)的人外周血单核细胞,通过edta可逆粘附程序分离,在快速51cr释放试验中表现出自发杀伤。使用单细胞偶联/右旋糖酐测定,我们定量地确定了单核细胞粘附到肿瘤靶细胞的选择要求。单核细胞对多种非贴壁肿瘤细胞系具有广泛的结合能力,而对非肿瘤靶细胞的结合水平最低。单核细胞与K562肿瘤细胞的结合是一个非常迅速的事件,在共沉淀后5分钟内达到饱和水平。低温和代谢抑制剂预处理降低了单核细胞与K562靶点的结合。用细胞骨骼破坏药物预处理单核细胞可显著降低结合。单核细胞在与K562细胞的结合中表现出特异性,Mg2+依赖,Ca2+独立的机制。结合后,需要Ca2+进行单核细胞介导的靶细胞裂解。利用透射电镜(TEM)和扫描电镜(SEM)技术对肿瘤细胞与单核细胞的结合进行了形态学研究。我们观察到,最初的结合是通过复杂的表面膜相互作用实现的,从相邻的效应靶细胞到稳定的偶联物,其特征是由大片紧密相邻的表面膜组成的接触区域。应用单细胞偶联/葡聚糖测定来评估单核细胞结合需求和单核细胞-靶细胞偶联过程的形态学特征,可能有助于阐明单核细胞介导的肿瘤细胞裂解的机制。
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Interactions between fresh human blood monocytes and tumor targets at the single cell level: binding and morphological characteristics.

Highly purified (97-99%), human peripheral blood monocytes, isolated by an EDTA-reversible adherence procedure, exhibit spontaneous killing in a rapid, 51Cr-release assay. Using the single cell conjugate/dextran assay, we have quantitatively determined select requirements for the adhesion of monocytes to neoplastic target cells. Monocytes expressed a broad binding capacity to a wide spectrum of nonadherent tumor cell lines, while binding at minimal levels to nontumor target cells. Binding of monocytes to K562 tumor cells is an extremely rapid event, reaching saturation levels within 5 min after cosedimentation. The binding of monocytes to K562 targets was reduced by low temperatures and pretreatment with metabolic inhibitors. Pretreatment of monocytes with cytoskeletal-disruptive drugs significantly reduced binding. Monocytes were shown to exhibit a specific, Mg2+-dependent, Ca2+-independent mechanism in their binding to K562 cells. Subsequent to binding, Ca2+ was required for monocyte-mediated target cell lysis to proceed. The binding of tumor cells by monocytes was studied morphologically using transmission (TEM) and scanning electron microscopic (SEM) techniques. It was observed that binding was achieved initially through complex, surface membrane interdigitations from apposing effector--target cells and progressed to stable conjugates, which were characterized by contact regions consisting of large expanses of closely apposed surface membranes. The application of the single cell conjugate/dextran assay to assess monocyte-binding requirements and the morphological characterization of the monocyte--target cell conjugation process may help in clarifying the mechanisms of monocyte-mediated tumor cell lysis.

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