人中性粒细胞膜形貌:使用凝集素作为探针检测识别位点的分布、运动和再生。

D L Weinbaum, J A Sullivan, G L Mandell
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引用次数: 0

摘要

我们使用荧光素和罗丹明标记的凝集素作为探针,研究了极化和非极化人中性粒细胞中膜结合位点的重新分布、运动和再现的模式。悬浮中,多形核白细胞(PMN)呈球形,对所有探针显示随机的识别位点阵列。PMN在悬浮液中被10(-6)M n -甲酰基- l-甲硫基- l-苯丙氨酸(f-Met-Phe)极化,附着在底物上的PMN在尾足上积累了结合的凝集素识别位点复合物(Con A;92.0 +/- 0.2%细胞和91.3 +/- 9.8%细胞)。在加入凝集素之前,以趋化梯度定向的中性粒细胞戊二醛固定揭示了先天的非结合识别位点阵列。未结合的Con A识别位点以“前灯”模式聚集在74.7 +/- 0.8%的细胞前部,但其他凝集素的结合位点随机分布在极化细胞周围。当结合的Con A复合物被扫到极化活PMN的尾部时,“新的”未结合的Con A结合位点出现在细胞的前部。环己亚胺、KCN和秋水仙碱均未干扰新结合位点的出现。细胞松弛素B和碘乙酸钠抑制PMN极化,干扰新受体的出现。这表明这些新位点是被发现的,以前是隐藏的结合位点,而不是新合成的结构。凝集素结合位点的形貌和运动与PMN的功能状态有关。由于Con A和某些细菌都与甘露糖衍生物结合,我们假设“前灯模式”和新结合位点的发现有助于PMN在吞噬细胞向前移动时吞噬生物体。
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Human neutrophil membrane topography: examination of distribution, movement, and regeneration of recognition sites using lectins as probes.

We have studied the pattern of membrane binding site redistribution, movement, and reappearance in polarized and nonpolarized human neutrophils using fluorescein and rhodamine-labeled lectins as probes. In suspension, polymorphonuclear leukocytes (PMN) were spherical and displayed a random array of recognition sites for all of the probes. PMN polarized in suspension by 10(-6) M N-formyl-L-methionyl-L-phenylalanine (f-Met-Phe), and PMN attached to substrate accumulated the bound lectin recognition site complex at the uropod (for Con A; 92.0 +/- 0.2% of cells and 91.3 +/- 9.8% of cells, respectively). Glutaraldehyde fixation of neutrophils oriented in a chemotactic gradient prior to lectin addition revealed the innate unbound recognition site array. Unbound Con A recognition sites were clustered at the front of 74.7 +/- 0.8% of cells in a "headlight" pattern, but binding sites for other lectins were distributed randomly around the polarized cell. When bound Con A complexes are swept to the tail of the polarized living PMN, "new" unbound Con A binding sites appear at the front of the cell. Neither cycloheximide nor KCN nor colchicine interferred with new binding site appearance. Cytochalasin B and sodium iodacetate prevented PMN polarization and interfered with appearance of new receptors. This suggests that these fresh sites are uncovered, previously cryptic binding sites rather than newly synthesized structures. Lectin binding site topography and movement are related to the functional state of the PMN. Since both Con A and certain bacteria bind to mannose derivatives, we postulate that the "headlight pattern" and uncovering of fresh binding sites aid the PMN in engulfing organisms as the phagocyte moves forward.

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