McColl S R, Hachicha M, Levasseur S, Neote K, Schall T J
Centre de Recherche en Inflammation, Immunologie et Rhumatologie, Université Laval, Sainte-Foy, Québec, Canada.
J Immunol. 1993 May 15;150(10):4550-60.
Macrophage inflammatory proteins-1 (MIP-1) alpha and beta are members of the C-C branch of the platelet factor 4 superfamily of cytokines, recently designated the "chemokine" superfamily. It has been suggested that the major cellular targets for the biologic activities of the C-C chemokines are the mononuclear leukocytes. However, the original designation of murine MIP-1 proteins as inflammatory mediators was based on suggestions that they activated neutrophil functions such as chemotaxis, the respiratory burst, and degranulation. In this study, we have evaluated the ability of human (Hu) MIP-1 alpha and beta to affect purified human neutrophil function. Although both rHuMIP-1 alpha and -1 beta stimulated significant calcium mobilization in human monocytes, only HuMIP-1 alpha exerted a detectable effect on neutrophils. HuMIP-1 alpha stimulated a small, dose-dependent increase in intracellular calcium, which was accompanied by a simultaneous change in right-angle light scatter, the latter indicating induction of shape change. While the effect of HuMIP-1 alpha on calcium mobilization in neutrophils was small when compared with that elicited by IL-8 or Gro alpha, it had similar characteristics to that by other receptor-dependent neutrophil agonists in that it was dependent on pertussis toxin-sensitive G proteins and on both mobilization of calcium from intracellular sources as well as influx from the extracellular environment. In addition, stimulation of neutrophils with HuMIP-1 alpha led to desensitization to subsequent additions of HuMIP-1 alpha. The stimulatory effect of HuMIP-1 alpha on neutrophil calcium mobilization and shape change was not coupled to other standard measures of neutrophil effector function. For instance, neither HuMIP-1 alpha nor -1 beta had any detectable stimulatory effect on the Na+/H+ antiport, degranulation, actin polymerization, or chemotaxis. Moreover, although HuMIP-1 alpha binding could easily be measured on monocytes or monocytic cell lines, the number of sites were too few to characterize on neutrophils by the same technique. Taken together, these results show that neither HuMIP-1 alpha nor -1 beta stimulate significant neutrophil activation and support the concept that the biologic effects of members of the C-C branch of the platelet factor 4 superfamily are not primarily directed toward neutrophils.
巨噬细胞炎性蛋白-1(MIP-1)α和β是细胞因子血小板因子4超家族C-C分支的成员,该超家族最近被命名为“趋化因子”超家族。有人提出,C-C趋化因子生物学活性的主要细胞靶点是单核白细胞。然而,鼠MIP-1蛋白最初被指定为炎性介质是基于它们激活中性粒细胞功能(如趋化性、呼吸爆发和脱颗粒)的推测。在本研究中,我们评估了人(Hu)MIP-1α和β影响纯化的人中性粒细胞功能的能力。虽然重组人MIP-1α和-1β均能刺激人单核细胞中显著的钙动员,但只有HuMIP-1α对中性粒细胞产生了可检测到的影响。HuMIP-1α刺激细胞内钙有小幅度的剂量依赖性增加,同时伴有直角光散射的同步变化,后者表明诱导了形态改变。虽然与IL-8或Groα相比,HuMIP-1α对中性粒细胞钙动员的影响较小,但它与其他依赖受体的中性粒细胞激动剂具有相似的特征,即它依赖百日咳毒素敏感的G蛋白,以及细胞内钙的动员和细胞外环境的钙内流。此外,用HuMIP-1α刺激中性粒细胞会导致对随后添加的HuMIP-1α脱敏。HuMIP-1α对中性粒细胞钙动员和形态改变的刺激作用与中性粒细胞效应功能的其他标准指标无关。例如,HuMIP-1α和-1β对Na+/H+反向转运、脱颗粒、肌动蛋白聚合或趋化性均无任何可检测到的刺激作用。此外,虽然可以很容易地在单核细胞或单核细胞系上检测到HuMIP-1α的结合,但用相同技术在中性粒细胞上可表征的结合位点数量太少。综上所述,这些结果表明,HuMIP-1α和-1β均不能刺激显著的中性粒细胞活化,并支持血小板因子4超家族C-C分支成员的生物学效应并非主要针对中性粒细胞的观点。
