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通过扫描电子显微镜观察重新封闭过程中的细胞表面事件。

Cell surface events during resealing visualized by scanning-electron microscopy.

作者信息

McNeil P L, Baker M M

机构信息

Department of Cellular Biology and Anatomy, and Institute of Molecular Medicine and Genetics, Medical College of Georgia, Augusta 30912, USA.

出版信息

Cell Tissue Res. 2001 Apr;304(1):141-6. doi: 10.1007/s004410000286.

Abstract

The function of exocytosis during plasma membrane resealing might be to facilitate the flow of surface lipid over the disruption site and/or to add defect-spanning "patches" of internal membrane across it. Scanning-electron-microscopic visualization of large plasma membrane disruptions in sea urchin eggs is here used to distinguish between these two possibilities. Disruptions were induced by shear stress in the presence and absence of resealing-permissive levels of external Ca2+, and the eggs were fixed at various intervals thereafter for microscopic processing. In eggs fixed immediately (<1 s) after shearing in the absence of Ca2+, a condition which prevents resealing, disruption sites were filled with a uniform population of spherical vesicles (approximately 1 microm in diameter). In eggs fixed immediately after shearing at a resealing-permissive level of Ca2+, disruption sites were filled with a highly heterogeneous population of enlarged vesicles, some being more than 10 microm in diameter and many having irregular profiles and/or appearing to be joined to one another. In eggs fixed 2 s or 5 s post-shearing, the continuity of these large vesicles with one another and the surface membrane began to obscure individual vesicle identities. Single "apertures" of discontinuity over disruption sites, the predicted morphology of a flow-based resealing mechanism, were not observed at any time point (1-5 s) during the interval required for completion of resealing. These observations provide strong confirmation that "patching" of large disruptions mediates their resealing.

摘要

在质膜重新封闭过程中,胞吐作用的功能可能是促进表面脂质在破裂部位的流动和/或在内膜上添加跨越缺陷的“补丁”。本文利用扫描电子显微镜观察海胆卵中大型质膜破裂情况,以区分这两种可能性。在存在和不存在允许重新封闭的外部Ca2+水平的情况下,通过剪切应力诱导破裂,然后在不同时间间隔固定卵以便进行显微镜处理。在无Ca2+剪切后立即固定(<1秒)的卵中,这种情况会阻止重新封闭,破裂部位充满了均匀的球形囊泡群体(直径约1微米)。在允许重新封闭的Ca2+水平下剪切后立即固定的卵中,破裂部位充满了高度异质的扩大囊泡群体,一些直径超过10微米,许多具有不规则轮廓和/或似乎相互连接。在剪切后2秒或5秒固定的卵中,这些大囊泡彼此之间以及与表面膜的连续性开始模糊单个囊泡的特征。在重新封闭所需的时间间隔内(1-5秒)的任何时间点都未观察到破裂部位上基于流动的重新封闭机制所预测的单个“不连续孔”。这些观察结果有力地证实了大型破裂的“补丁”介导了它们的重新封闭。

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