Internalization pathway of C3b receptors in human neutrophils and its transmodulation by chemoattractant receptors stimulation.

Cell regulation Pub Date : 1991-01-01 DOI:10.1091/mbc.2.1.41
J L Carpentier, D P Lew, J P Paccaud, R Gil, B Iacopetta, M Kazatchkine, O Stendahl, T Pozzan
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引用次数: 52

Abstract

On the surface of phagocytes, C3b receptors (CR1) bind C3b-coated particles and promote their ingestion after activation by appropriate stimuli such as lymphokines or the chemoattractant formyl methionyl leucyl phenylalanine (fMLP) and fibronectin. The aims of the present study were 1) to define at the electron microscopic level the nature of the process responsible for CR1 internalization and 2) to dissect the mechanism by which a physiological activator (fMLP) stimulates this process. CR1 was visualized either by the immunogold technique or by quantitative electron microscopic autoradiography using a monoclonal anti-CR1 antibody. Both techniques revealed that after anti-CR1 binding, CR1 cluster on the neutrophil surface in a time-, temperature-, and antibody-dependent fashion, but do not concentrate in coated pits. CR1 internalization requires receptor cross-linking (does not occur in the presence of Fab fragments of anti-CR1) and intact microfilaments. It results in the association of the internalized material with large flattened vacuoles, organized in stacks. Together with the surface localization of CR1 close to cytoplasmic projections (ruffles), these observations suggest that uptake of CR1 occurs through a macropinocytotic process. Eventually, CR1 concentrate in lysosomal structures. fMLP markedly stimulates this pattern of CR1 internalization without affecting their clustering or their lack of association with coated pits. Stimulation by fMLP is inhibited by pertussis toxin, unaffected by preventing receptor-triggered cytosolic free calcium [Ca2+]i elevations, and mimicked by phorbol myristate acetate. Taken together our data demonstrate 1) that, in neutrophils, CR1 is internalized via a coated pit independent macropinocytotic process, dependent on intact microfilaments and receptor cross-linking; 2) that, in the same cells, fMLP is internalized via the classical coated pits pathway; and 3) that fMLP amplifies CR1 uptake possibly via protein kinase C stimulation.

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人中性粒细胞C3b受体的内化途径及其在化学引诱剂受体刺激下的转调。
在吞噬细胞表面,C3b受体(CR1)结合C3b包被颗粒,并在适当的刺激(如淋巴因子或化学引诱剂甲酰基甲硫基亮基苯丙氨酸(fMLP)和纤维连接蛋白)激活后促进其摄入。本研究的目的是1)在电子显微镜水平上定义负责CR1内化过程的性质,2)剖析生理激活剂(fMLP)刺激这一过程的机制。通过免疫金技术或使用单克隆抗CR1抗体的定量电镜放射自显影技术可见CR1。两种技术都显示,在抗CR1结合后,CR1以时间、温度和抗体依赖的方式聚集在中性粒细胞表面,但不集中在涂覆的凹坑中。CR1内化需要受体交联(在抗CR1的Fab片段存在时不会发生)和完整的微丝。它导致内化的物质与大的扁平液泡相关联,排列成堆栈。再加上CR1在细胞质突起(皱褶)附近的表面定位,这些观察结果表明,CR1的摄取是通过巨噬细胞过程发生的。最终,CR1集中在溶酶体结构中。fMLP显著刺激CR1内化的这种模式,而不影响它们的聚类或它们与被涂层凹坑的缺乏关联。fMLP的刺激被百日咳毒素抑制,不受防止受体触发的胞质游离钙[Ca2+]i升高的影响,并被肉豆蔻酸酯所模拟。综上所述,我们的数据表明:1)在中性粒细胞中,CR1通过一个独立于包被坑的巨噬细胞过程内化,依赖于完整的微丝和受体交联;2)在相同的细胞中,fMLP通过经典的包被凹坑途径内化;3) fMLP可能通过蛋白激酶C刺激而放大CR1摄取。
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