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Apoptosis and necrosis: Detection, discrimination and phagocytosis.

机译:凋亡和坏死:检测,鉴别和吞噬作用。

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Three major morphologies of cell death have been described: apoptosis (type I), cell death associated with autophagy (type II) and necrosis (type III). Apoptosis and cell death associated with autophagy can be distinguished by certain biochemical events. However, necrosis is characterized mostly in negative terms by the absence of caspase activation, cytochrome c release and DNA oligonucleosomal fragmentation. A particular difficulty in defining necrosis is that in the absence of phagocytosis apoptotic cells become secondary necrotic cells with many morphological features of primary necrosis. In this review, we present a selection of techniques that can be used to identify necrosis and to discriminate it from apoptosis. These techniques rely on the following cell death parameters: (1) morphology (time-lapse and transmission electron microscopy and flow fluorocytometry); (2) cell surface markers (phosphatidylserine exposure versus membrane permeability by flow fluorocytometry); (3) intracellular markers(oligonucleosomal DNA fragmentation by flow fluorocytometry, caspase activation, Bid cleavage and cytochrome c release by western blotting); (4) release of extracellular markers in the supernatant (caspases, HMGB-1 and cytokeratin 18). Finally, we report on methods that can be used to examine interactions between dying cells and phagocytes. We illustrate a quantitative method for detecting phagocytosis of dying cells by flow fluorocytometry. We also describe a recently developed approach based on the use of fluid phase tracers and different kind of microscopy, transmission electron and fluorescence microscopy, to characterize the mechanisms used by phagocytes to internalize dying cells.
机译:已经描述了细胞死亡的三种主要形态:细胞凋亡(I型),与自噬相关的细胞死亡(II型)和坏死(III型)。与自噬相关的细胞凋亡和细胞死亡可以通过某些生化事件来区分。然而,坏死的主要特征是缺乏胱天蛋白酶激活,细胞色素c释放和DNA寡核小体片段化。定义坏死的一个特殊困难是,在没有吞噬作用的情况下,凋亡细胞会变成具有许多原发性坏死形态特征的继发性坏死细胞。在这篇综述中,我们提出了一些可用于鉴定坏死并将其与凋亡区分开的技术。这些技术依赖于以下细胞死亡参数:(1)形态(延时和透射电子显微镜以及流式细胞术); (2)细胞表面标志物(通过流式细胞术检测磷脂酰丝氨酸暴露与膜通透性); (3)细胞内标记(通过流式细胞术检测寡核小体DNA片段,半胱天冬酶激活,Bid裂解和Western blot释放细胞色素c); (4)释放上清液中的细胞外标记(胱天蛋白酶,HMGB-1和细胞角蛋白18)。最后,我们报告了可用于检查垂死细胞与吞噬细胞之间相互作用的方法。我们说明了一种定量方法,用于通过流式细胞术检测垂死细胞的吞噬作用。我们还描述了一种最新发展的方法,该方法基于使用液相示踪剂和不同种类的显微镜,透射电子和荧光显微镜来表征吞噬细胞内在化垂死细胞的机制。

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