Processing of concanavalin A-receptor complexes by rat osteoclasts in vitro.

S N Popoff, G B Schneider
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引用次数: 5

Abstract

The osteoclast is a large multinucleate cell that is widely accepted as the primary effector cell responsible for normal bone resorption. In a previous study, we demonstrated that concanavalin A (con A) has a dose-dependent biphasic effect on the bone-resorbing capacity of osteoclasts, using a 45Ca bone-organ culture system; bone resorption was stimulated at low concentrations and inhibited at high concentrations. The mitogenic property of con A in lymphocyte cultures is well documented; therefore con A has been used extensively to study the manner in which lymphocytes and other mononuclear cells process the cell-bound lectin. In this study, we have investigated the processing of con A-receptor complexes by osteoclasts in culture, using con A-FITC to evaluate the redistribution of cell-bound con A via epifluorescence microscopy and using con A-ferritin to determine whether the lectin receptor complexes are internalized. The osteoclasts were obtained from the long bones of newborn rats and allowed to attach to glass coverslips at 37 degrees C. Following attachment, the nonadherent cells were removed by rinsing. The adherent osteoclasts were preincubated in 50 micrograms/ml con A-FITC or con A-ferritin at 4 degrees C for 10 min, washed to remove unbound con A, and incubated at 37 degrees C for 15 or 30 min in the absence of con A. Positive controls were fixed immediately after preincubation at 4 degrees C; negative controls were preincubated in con A-FITC and alpha-methyl mannoside, the haptenic inhibitor of con A binding. The results demonstrate that redistribution and endocytosis of con A-receptor complexes occurs within 30 min. These findings confirm the hypothesis that cell-bound con A can alter the structure and activity of osteoclast membrane components in a manner similar to that observed in mononuclear cell cultures. The internalization of con A may be important in altering osteoclastic activity by mediating intracellular mechanisms involved in the bone-resorbing process.

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大鼠破骨细胞体外加工刀豆蛋白a受体复合物的实验研究。
破骨细胞是一种大的多核细胞,被广泛认为是正常骨吸收的主要效应细胞。在之前的一项研究中,我们使用45Ca骨器官培养系统证明了刀豆蛋白a (con a)对破骨细胞的骨吸收能力具有剂量依赖性的双相效应;低浓度刺激骨吸收,高浓度抑制骨吸收。con A在淋巴细胞培养中的有丝分裂特性已得到充分证明;因此,con A已被广泛用于研究淋巴细胞和其他单核细胞处理细胞结合凝集素的方式。在本研究中,我们研究了破骨细胞在培养过程中对con A受体复合物的加工,使用con A- fitc通过荧光显微镜评估细胞结合的con A的重新分配,并使用con A-铁蛋白来确定凝集素受体复合物是否被内化。从新生大鼠的长骨中获得破骨细胞,并将其附着在37℃的玻璃罩上。附着后,通过冲洗去除非粘附细胞。将粘附的破骨细胞在50微克/毫升的con A- fitc或con A-铁蛋白中4℃预孵育10分钟,洗涤去除未结合的con A,在无con A的情况下37℃孵育15或30分钟,4℃预孵育后立即固定阳性对照;阴性对照在con A- fitc和α -甲基甘露糖苷(con A结合的半抗原抑制剂)中预孵育。结果表明,con - A受体复合物的重新分配和内吞作用在30分钟内发生。这些发现证实了细胞结合的con - A可以改变破骨细胞膜成分的结构和活性的假设,其方式类似于在单核细胞培养中观察到的。con A的内化可能通过介导参与骨吸收过程的细胞内机制,在改变破骨细胞活性方面发挥重要作用。
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