首页> 美国卫生研究院文献>The Journal of Biophysical and Biochemical Cytology >ELECTRON MICROSCOPE OBSERVATIONS ON COMPOUND 48/80-INDUCED DEGRANULATION IN RAT MAST CELLS
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ELECTRON MICROSCOPE OBSERVATIONS ON COMPOUND 48/80-INDUCED DEGRANULATION IN RAT MAST CELLS

机译:复方大鼠肥大细胞中48/80诱导的脱粒的电子显微镜观察

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摘要

In vitro degranulation of rat mast cells was studied at different intervals ranging from 10 to 60 sec after adding the histamine liberator, compound 48/80 (0.4 µg/ml, 17°C). The ultrastructural changes were followed by electron microscopy, and parallel assays were made to determine the histamine released. In addition, the extracellular tracers lanthanum and hemoglobin (demonstrated by its peroxidative activity) were applied to mast cells to follow communication of the extracellular space with the cavities formed during degranulation. After a lag period of 10 sec, degranulation started in the most peripherally located granules. The perigranular membrane fused with the plasma membrane, resulting in a pore bridged by a thin diaphragm. This was followed by rupture of the diaphragm and extrusion of the granule matrix (exocytosis). The process advanced towards the cell interior by fusion and opening of the deeper situated granules to the formerly opened granule cavities. At the end of the process, the cell was filled by a system of complicated cavities containing a number of altered granules. Extracellular tracers have shown that these intracellular cavities were in unbroken communication with the extracellular space from the very beginning of their formation. Both lanthanum and hemoglobin were found to be adsorbed to the limiting membrane of the cavities and bound to altered mast cell granules. In contrast, no tracer substance was present in nondegranulating mast cells. Degranulation of mast cells by compound 48/80 is regarded as a sequential exocytosis, a process similar to that described for some exocrine gland cells. All the "intracellular" cavities, formed by degranulation, were shown to communicate with the extracellular space; consequently, granules lying in these cavities must be considered as biologically extracellular. The present findings support the view that histamine is released from the granule matrix by the extracellular ionic milieu.
机译:加入组胺释放剂化合物48/80(0.4 µg / ml,17°C)后,在10至60秒的不同间隔研究大鼠肥大细胞的体外脱粒作用。通过电子显微镜观察超微结构的变化,并进行平行测定以确定释放的组胺。另外,将细胞外示踪剂镧和血红蛋白(通过其过氧化活性证明)应用于肥大细胞,以追踪细胞外空间与脱粒过程中形成的腔的连通。 10秒钟的滞后时间后,位于最外围的颗粒开始脱粒。周质膜与质膜融合,形成由薄隔膜桥接的孔。随后隔膜破裂和颗粒基质挤出(胞吐作用)。通过将较深位置的颗粒融合并向先前打开的颗粒腔开放,该过程向细胞内部发展。在该过程结束时,将细胞填充到一个复杂的空腔系统中,该系统包含许多改变的颗粒。细胞外示踪剂表明,这些细胞内腔从形成之初就一直与细胞外空间保持不间断的通讯。发现镧和血红蛋白都被吸附到腔的极限膜上,并与改变的肥大细胞颗粒结合。相反,在非脱颗粒肥大细胞中不存在示踪物质。化合物48/80对肥大细胞的脱粒被认为是顺序性胞吐作用,该过程类似于某些外分泌腺细胞所描述的过程。通过脱粒形成的所有“细胞内”腔均显示与细胞外空间连通;因此,位于这些腔内的颗粒必须被视为生物学上的细胞外。本发现支持以下观点:组胺通过细胞外离子环境从颗粒基质释放。

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