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通过核DNA片段化的特异性标记原位鉴定程序性细胞死亡。

Identification of programmed cell death in situ via specific labeling of nuclear DNA fragmentation.

作者信息

Gavrieli Y, Sherman Y, Ben-Sasson S A

机构信息

Department of Experimental Medicine, Hebrew University-Hadassah Medical School, Jerusalem, Israel.

出版信息

J Cell Biol. 1992 Nov;119(3):493-501. doi: 10.1083/jcb.119.3.493.

Abstract

Programmed cell death (PCD) plays a key role in developmental biology and in maintenance of the steady state in continuously renewing tissues. Currently, its existence is inferred mainly from gel electrophoresis of a pooled DNA extract as PCD was shown to be associated with DNA fragmentation. Based on this observation, we describe here the development of a method for the in situ visualization of PCD at the single-cell level, while preserving tissue architecture. Conventional histological sections, pretreated with protease, were nick end labeled with biotinylated poly dU, introduced by terminal deoxy-transferase, and then stained using avidin-conjugated peroxidase. The reaction is specific, only nuclei located at positions where PCD is expected are stained. The initial screening includes: small and large intestine, epidermis, lymphoid tissues, ovary, and other organs. A detailed analysis revealed that the process is initiated at the nuclear periphery, it is relatively short (1-3 h from initiation to cell elimination) and that PCD appears in tissues in clusters. The extent of tissue-PCD revealed by this method is considerably greater than apoptosis detected by nuclear morphology, and thus opens the way for a variety of studies.

摘要

程序性细胞死亡(PCD)在发育生物学以及维持不断更新组织的稳态中起着关键作用。目前,其存在主要是通过对汇集的DNA提取物进行凝胶电泳推断出来的,因为PCD已被证明与DNA片段化有关。基于这一观察结果,我们在此描述一种在单细胞水平原位可视化PCD的方法的开发,同时保留组织结构。用蛋白酶预处理的传统组织学切片,用末端脱氧转移酶引入的生物素化聚dU进行缺口末端标记,然后用抗生物素蛋白偶联过氧化物酶染色。该反应具有特异性,只有预期发生PCD的位置的细胞核被染色。初步筛选包括:小肠、大肠、表皮、淋巴组织、卵巢和其他器官。详细分析表明,该过程始于核周边,相对较短(从开始到细胞清除为1 - 3小时),并且PCD以簇状出现在组织中。通过这种方法揭示的组织PCD程度明显大于通过核形态学检测到的凋亡,从而为各种研究开辟了道路。

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