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使用地高辛标记的聚(A)寡核苷酸探针通过原位杂交在组织切片中检测富含胸腺嘧啶的DNA序列,以显示凋亡细胞。

Demonstration of apoptotic cells in tissue sections by in situ hybridization using digoxigenin-labeled poly(A) oligonucleotide probes to detect thymidine-rich DNA sequences.

作者信息

Hilton D A, Love S, Barber R

机构信息

Department of Neuropathology, Frenchay Hospital, Bristol, United Kingdom.

出版信息

J Histochem Cytochem. 1997 Jan;45(1):13-20. doi: 10.1177/002215549704500103.

DOI:10.1177/002215549704500103
PMID:9010464
Abstract

The recognition of apoptotic cells by morphological appearance alone may be difficult. We have investigated the use of in situ hybridization (ISH) with digoxigenin-labeled poly(A) probes to detect apoptotic cells in tissue sections. This method was compared to conventional morphologic assessment and in situ end-labelling (ISEL) in a range of tissues in which apoptosis is known to occur. ISH with poly(A) probes detected apoptotic nuclei in all tissues in which there was evidence of apoptosis as judged by conventional histology. ISH and, to a lesser extent, ISEL preferentially labeled shrunken but still intact nuclei with margination of chromatin, presumably at an early stage of apoptosis. The poly(A) hybridization was abolished by pretreatment of tissue sections with DNAse. After denaturation of DNA, poly(A) hybridized to nuclei in all cells. No convincing hybridization signal was detected in alcohol-fixed or fresh-frozen sections. Both ISEL and ISH labeled some of the nuclei in ischemic tissues. ISH with poly(A) oligonucleotide probes offers a simple alternative to ISEL for detection of cells in early stages of apoptosis. These probes hybridize to thymidine-rich sequences of DNA in the highly repeated Alu sequences within the nuclear genome. These sequences are believed to become available for hybridization after formalin fixation and paraffin embedding as a result of the apoptosis-related increase in the susceptibility of nuclear DNA to denaturation.

摘要

仅通过形态外观来识别凋亡细胞可能会很困难。我们研究了使用地高辛配体标记的聚(A)探针进行原位杂交(ISH)来检测组织切片中的凋亡细胞。在一系列已知会发生凋亡的组织中,将该方法与传统形态学评估和原位末端标记(ISEL)进行了比较。根据传统组织学判断,聚(A)探针原位杂交在所有有凋亡证据的组织中都检测到了凋亡细胞核。ISH以及在较小程度上ISEL优先标记了染色质边缘化的皱缩但仍完整的细胞核,推测处于凋亡的早期阶段。用DNA酶预处理组织切片可消除聚(A)杂交。DNA变性后,聚(A)与所有细胞中的细胞核杂交。在酒精固定或新鲜冷冻切片中未检测到令人信服的杂交信号。ISEL和ISH都标记了缺血组织中的一些细胞核。用聚(A)寡核苷酸探针进行ISH为ISEL提供了一种简单的替代方法,用于检测凋亡早期阶段的细胞。这些探针与核基因组中高度重复的Alu序列内富含胸腺嘧啶的DNA序列杂交。由于凋亡相关的核DNA变性敏感性增加,这些序列在福尔马林固定和石蜡包埋后被认为可用于杂交。

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