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单纯疱疹病毒抗体依赖性细胞毒性系统中黏附步骤的分析

Analysis of the adhesion step in the herpes simplex virus antibody-dependent cellular cytotoxicity system.

作者信息

Romano T J, Shore S L

出版信息

Infect Immun. 1979 Oct;26(1):163-72. doi: 10.1128/iai.26.1.163-172.1979.

Abstract

The lysis of herpes simplex virus-infected tissue culture cells by antibody-dependent cellular cytotoxicity (ADCC) requires a preliminary step in which effector cells adhere to the immunoglobulin G antibody-coated targets. To study the adhesion step, we made use of two observations: (i) some of the mononuclear cells in human blood form rosettes with antibody-coated target cells, and (ii) most ADCC effector cells can be removed by allowing mononuclear cells to adhere to monolayers of antibody-sensitized tissue culture cells. The effect of various experimental conditions on the adhesion step was assessed in ADCC cultures both at unit gravity and after centrifugation. At unit gravity both rosette formation and monolayer adhesion were partially reduced at 4 degrees C as compared to 37 degrees C. Both were also partially inhibited in glucose-free medium containing sodium azide and 2-deoxyglucose but were unaffected in glucose-free medium containing only one of these energy inhibitors. In contrast, after centrifugation neither reaction was inhibited at 4 degrees C or in glucose-free medium with sodium azide and 2-deoxyglucose. Cytochalasin B but not colchicine suppressed both reactions. Inhibition by cytochalasin B could not be reversed by centrifugation. Both reactions were independent of extracellular Ca(2+) and Mg(2+) and were unaffected by rendering mononuclear cells cytotoxically inactive by brief heat shock. These findings indicate that the adhesion step in ADCC directed against virus-infected or uninfected tissue culture cells is only modestly dependent on effector cell energy generation, that centrifugation greatly reduces this dependence, and that microfilaments but not microtubules are necessary. The modest ambient temperature and energy requirements, independence of extracellular divalent cations, lack of sensitivity to colchicine, and relative resistance to supraphysiological temperature serve to distinguish the adhesion step from the lytic step in ADCC.

摘要

通过抗体依赖性细胞毒性(ADCC)对单纯疱疹病毒感染的组织培养细胞进行裂解需要一个初步步骤,即效应细胞粘附于免疫球蛋白G抗体包被的靶细胞。为了研究粘附步骤,我们利用了两个观察结果:(i)人血液中的一些单核细胞与抗体包被的靶细胞形成玫瑰花结,以及(ii)通过使单核细胞粘附于抗体致敏的组织培养细胞单层,可以去除大多数ADCC效应细胞。在单位重力和离心后的ADCC培养物中评估了各种实验条件对粘附步骤的影响。在单位重力下,与37℃相比,4℃时玫瑰花结形成和单层粘附均部分降低。在含有叠氮化钠和2-脱氧葡萄糖的无葡萄糖培养基中,两者也均受到部分抑制,但在仅含有这些能量抑制剂之一的无葡萄糖培养基中则不受影响。相比之下,离心后,在4℃或含有叠氮化钠和2-脱氧葡萄糖的无葡萄糖培养基中,两种反应均未受到抑制。细胞松弛素B而非秋水仙碱抑制了两种反应。细胞松弛素B的抑制作用不能通过离心逆转。两种反应均独立于细胞外Ca(2+)和Mg(2+),并且短暂热休克使单核细胞细胞毒性失活对其无影响。这些发现表明,针对病毒感染或未感染的组织培养细胞的ADCC中的粘附步骤仅适度依赖于效应细胞的能量产生,离心大大降低了这种依赖性,并且微丝而非微管是必需的。适度的环境温度和能量需求、对细胞外二价阳离子的独立性、对秋水仙碱不敏感以及对超生理温度的相对抗性,使得粘附步骤与ADCC中的裂解步骤得以区分。

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