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端粒在体外和体内的DNA拓扑异构酶II切割

DNA topoisomerase II cleavage of telomeres in vitro and in vivo.

作者信息

Yoon H J, Choi I Y, Kang M R, Kim S S, Muller M T, Spitzner J R, Chung I K

机构信息

Department of Biology, Yonsei University, Seoul, South Korea.

出版信息

Biochim Biophys Acta. 1998 Jan 7;1395(1):110-20. doi: 10.1016/s0167-4781(97)00139-5.

Abstract

In this work, we have analyzed the reactivity of DNA topoisomerase II with telomeric DNA both in vitro and in vivo. Topoisomerase II cleavage reactions were performed on the tandem repeats of telomeric DNA. Analysis of this DNA on sequencing gels revealed that DNA topoisomerase II is catalytically active in cleaving the telomere DNA repeat. The topoisomerase II cleavage site is 5'TTAGG*G3' (cleavage site marked by the asterisk) and since telomere DNA is a tandem array of the above sequence, topoisomerase cleavage sites could exist every six base pairs. Detection of topoisomerase II cleavages was strongly dependent upon one specific topoisomerase II poison, etoposide (VP-16). A number of other topoisomerase II poisons were tested but did not stimulate cleavage activity at the telomere repeat. We have also analyzed the association of endogenous topoisomerase II with chromosomal telomeric DNA in HeLa cells. The in vivo complex of enzyme (ICE) bioassay was used to isolate topoisomerase II-DNA covalent complexes. In consistence with in vitro cleavage data, endogenous topoisomerase II-telomeric DNA complexes were detected in only etoposide-treated HeLa cells.

摘要

在这项工作中,我们分析了DNA拓扑异构酶II在体外和体内与端粒DNA的反应活性。对端粒DNA串联重复序列进行了拓扑异构酶II切割反应。在测序凝胶上对该DNA进行分析,结果显示DNA拓扑异构酶II在切割端粒DNA重复序列方面具有催化活性。拓扑异构酶II的切割位点为5'TTAGG*G3'(切割位点用星号标记),由于端粒DNA是上述序列的串联阵列,因此拓扑异构酶的切割位点可能每六个碱基对就存在一个。拓扑异构酶II切割的检测强烈依赖于一种特定的拓扑异构酶II抑制剂,依托泊苷(VP - 16)。测试了许多其他拓扑异构酶II抑制剂,但它们均未刺激端粒重复序列处的切割活性。我们还分析了HeLa细胞中内源性拓扑异构酶II与染色体端粒DNA的关联。利用体内酶复合物(ICE)生物测定法分离拓扑异构酶II - DNA共价复合物。与体外切割数据一致,仅在经依托泊苷处理的HeLa细胞中检测到内源性拓扑异构酶II - 端粒DNA复合物。

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