首页> 美国卫生研究院文献>Journal of Anatomy and Physiology >Morphometric studies of secretory granule formation in mouse pancreatic acinar cells. Dissecting the early structural changes following pilocarpine injection
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Morphometric studies of secretory granule formation in mouse pancreatic acinar cells. Dissecting the early structural changes following pilocarpine injection

机译:小鼠胰腺腺泡细胞分泌颗粒形成的形态计量学研究。剖析毛果芸香碱注射后的早期结构变化

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摘要

Secretory granule formation in pancreatic acinar cells is known to involve massive membrane flow. In previous studies we have undertaken morphometry of the regranulation mechanism in these cells and in mast cells as a model for cellular membrane movement. In our current work, electron micrographs of pancreatic acinar cells from ICR mice were taken at several time points after extensive degranulation induced by pilocarpine injection in order to investigate the volume changes of rough endoplasmic reticulum (RER), nucleus, mitochondria and autophagosomes. At 2–4 h after stimulation, when the pancreatic cells demonstrated a complete loss of granules, this was accompanied by an increased proportion of autophagosomal activity. This change primarily reflected a greatly increased proportion of profiles retaining autophagic vacuoles containing recognisable cytoplasmic structures such as mitochondria, granule profiles and fragments of RER. The mitochondrial structures reached a significant maximal size 4 h following injection (before degranulation 0.178±0.028 μm3; at 4 h peak value, 0.535±0.109 μm3). Nucleus size showed an early volume increase approaching a maximum value 2 h following degranulation. The regranulation span was thus divided into 3 stages. The first was the membrane remodelling stage (0–2 h). During this period the volume of the RER and secretory granules was greatly decreased. At the intermediate stage (2–4 h) a significant increase of the synthesis zone was observed within the nucleus. The volume of the mitochondria was increasing. At the last step, the major finding was a significant granule accumulation in parallel with an active Golgi zone.
机译:已知胰腺腺泡细胞中分泌颗粒的形成涉及大量的膜流动。在以前的研究中,我们对这些细胞和肥大细胞中的再形成机制进行了形态测量,以此作为细胞膜运动的模型。在我们目前的工作中,从毛果芸香碱注射液引起的广泛脱粒后,在几个时间点拍摄了ICR小鼠胰腺腺泡细胞的电子显微照片,以研究粗糙内质网(RER),细胞核,线粒体和自噬体的体积变化。在刺激后2-4小时,当胰腺细胞显示出颗粒完全丧失时,这伴随着自噬体活性比例的增加。这种变化主要反映了保留自噬液泡的轮廓比例大大增加,其中自噬液泡包含可识别的细胞质结构,例如线粒体,颗粒轮廓和RER片段。注射后4 h(脱粒前0.178±0.028μm 3 ;在4 h峰值为0.535±0.109μm 3 ),线粒体结构达到最大尺寸。脱核后2小时,核大小显示出早期体积增加,接近最大值。因此,重新调节跨度分为三个阶段。第一个是膜重塑阶段(0–2小时)。在此期间,RER和分泌颗粒的体积大大减少。在中间阶段(2-4小时),观察到细胞核内合成区的显着增加。线粒体的体积在增加。在最后一步,主要发现是与活跃的高尔基体区域平行的大量颗粒堆积。

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