首页> 美国卫生研究院文献>Journal of the Boston Society of Medical Sciences >Immune complex receptors on cell surfaces. II. Cytochemical evaluation of their abundance on different immune cells: distribution uptake and regeneration.
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Immune complex receptors on cell surfaces. II. Cytochemical evaluation of their abundance on different immune cells: distribution uptake and regeneration.

机译:免疫细胞表面的复杂受体。二。对不同免疫细胞上它们的丰度进行细胞化学评估:分布摄取和再生。

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摘要

A recently developed method for ultrastructural demonstration of cell surface receptors for immune complexes is applied to evaluation of these receptors on various cell types. The method entailing incubation with a complex of horesradish peroxidase (HRP) and antibody to HRP (anti-HRP) disclosed dense foci indicative of immune complex receptors distributed at 30- to 120-mmu intervals over macrophage surfaces. Invaginations, loop-like evaginations, and pinocytotic vasicles stained prominently. The number of stained immune complex receptors averaged 200,000 per oil-induced macrophage and 120,000 per noninduced macrophage, as determined from counts of focal deposits in electron micrographs. Receptor periodicity on giant cells present in oil-induced exudates resembled that on macrophages, but the larger giant cells contained an estimated 1.5 million sites. Although receptor periodicity on eosinophils and neutrophils equaled that on macrophages, the staining was lighter and was interrupted by intervals of unstained membrane. Neutrophils averaged 28,000 and eosinophils 35,000 receptors per cell, whereas those lymphocytes with receptors averaged 3,500 per cell. Viable cells incubated with anti-HRP sequentially exhibited about half as many reactive sites as did cells incubated with immune complex. When warmed to 37 C, viable macrophages and eosinophils pinocytosed soluble immune complexes almost completely within 30 minutes and phagocytosed insoluble complexes more slowly. The endocytosed soluble immune complexes were sequestered within tubulovesicular structures in addition to the expected phagocytic vacuoles. Receptors appeared fully active on macrophages that were restained with soluble, cold immune complex after they had endocytosed immune complex in the course of a 30-minute warming interval.
机译:最近开发的用于免疫复合物的细胞表面受体超微结构展示的方法被用于评估各种细胞类型上的这些受体。该方法需要与辣根过氧化物酶(HRP)和抗HRP抗体(抗HRP)的复合物进行孵育,该方法公开了致密的病灶,表明免疫复合物受体以30至120 mmu的间隔分布在巨噬细胞表面。内陷,环状外陷和胞吞性血管明显染色。根据电子显微照片中的沉积物计数,染色的免疫复合受体的数量平均每个油诱导的巨噬细胞为200,000,每个非诱导的巨噬细胞为120,000。油诱导的渗出液中巨细胞的受体周期性与巨噬细胞相似,但是较大的巨细胞估计有150万个位点。尽管嗜酸性粒细胞和嗜中性粒细胞的受体周期性与巨噬细胞相同,但染色较浅并且被未染色的膜间隔中断。中性粒细胞平均每个细胞28,000个受体,嗜酸性粒细胞35,000个受体,而那些带有受体的淋巴细胞平均每个细胞3,500个。与抗HRP孵育的活细胞依次显示的反应位点是与免疫复合物孵育的细胞的反应位的一半。当升温至37°C时,有活力的巨噬细胞和嗜酸性粒细胞在30分钟内几乎完全吞噬了可溶性免疫复合物,而吞噬了不溶性复合物的速度则更慢。除了预期的吞噬液泡之外,将内吞的可溶性免疫复合物隔离在微管小体结构内。受体在30分钟的升温间隔内被内吞的免疫复合物吞噬后,对保留有可溶性冷免疫复合物的巨噬细胞表现出完全的活性。

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