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在经历凋亡而非坏死的细胞中存在具有单碱基3'端突出的双链断裂。

Presence of double-strand breaks with single-base 3' overhangs in cells undergoing apoptosis but not necrosis.

作者信息

Didenko V V, Hornsby P J

机构信息

Huffington Center on Aging, Baylor College of Medicine, Houston, Texas 77030, USA.

出版信息

J Cell Biol. 1996 Dec;135(5):1369-76. doi: 10.1083/jcb.135.5.1369.

Abstract

Apoptotic cells in rat thymus were labeled in situ in paraffin-embedded and frozen tissue sections by ligation of double-stranded DNA fragments containing digoxigenin or Texas red. Two forms of double-stranded DNA fragments were prepared using the polymerase chain reaction: one was synthesized using Taq polymerase, which yields products with single-base 3' overhangs, and one using Pfu polymerase, which produces blunt-ended products. Both types of fragment could be ligated to apoptotic nuclei in thymus, indicating the presence in such nuclei of DNA double-strand breaks with single-base 3' overhangs as well as blunt ends. However, in nuclei with DNA damage resulting from a variety of nonapoptotic processes (necrosis, in vitro autolysis, peroxide damage, and heating) single-base 3' overhangs were either nondetectable or present at much lower concentrations than in apoptotic cells. Blunt DNA ends were present in such tissues, but at lower concentrations than in apoptotic cells. In contrast, in all of these forms of DNA damage, nuclei contained abundant 3'-hydroxyls accessible to labeling with terminal deoxynucleotidyl transferase. Thus, although single-base 3' overhangs and blunt ends are present in apoptotic nuclei, the specificity of the in situ ligation of 3'-overhang fragments to apoptotic nuclei indicates that apoptotic cells labeled in this way can readily be distinguished from cells with nonapoptotic DNA damage. These data are consistent with the involvement of an endonuclease similar to DNase I in apoptosis, which is predicted to leave short 3' overhangs as well as blunt ends in digestion of chromatin.

摘要

通过连接含有地高辛或德克萨斯红的双链DNA片段,对石蜡包埋和冷冻组织切片中的大鼠胸腺凋亡细胞进行原位标记。使用聚合酶链反应制备了两种形式的双链DNA片段:一种是使用Taq聚合酶合成的,其产生具有单碱基3'突出端的产物;另一种是使用Pfu聚合酶合成的,其产生平端产物。两种类型的片段都可以连接到胸腺中的凋亡细胞核上,表明在这些细胞核中存在具有单碱基3'突出端以及平端的DNA双链断裂。然而,在由多种非凋亡过程(坏死、体外自溶、过氧化物损伤和加热)导致DNA损伤的细胞核中,单碱基3'突出端要么检测不到,要么其浓度比凋亡细胞中的低得多。平端DNA在这些组织中存在,但浓度低于凋亡细胞。相比之下,在所有这些形式的DNA损伤中,细胞核含有丰富的可被末端脱氧核苷酸转移酶标记的3'-羟基。因此,尽管凋亡细胞核中存在单碱基3'突出端和平端,但3'突出端片段与凋亡细胞核原位连接的特异性表明,以这种方式标记的凋亡细胞可以很容易地与具有非凋亡DNA损伤的细胞区分开来。这些数据与一种类似于DNase I的内切核酸酶参与凋亡过程一致,预计该酶在染色质消化过程中会留下短的3'突出端和平端。

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