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Ku70/80基因表达和DNA依赖性蛋白激酶(DNA-PK)活性与正常人成纤维细胞中的双链断裂(dsb)修复能力及细胞放射敏感性不相关。

Ku70/80 gene expression and DNA-dependent protein kinase (DNA-PK) activity do not correlate with double-strand break (dsb) repair capacity and cellular radiosensitivity in normal human fibroblasts.

作者信息

Kasten U, Plottner N, Johansen J, Overgaard J, Dikomey E

机构信息

Institute of Biophysics and Radiobiology, University of Hamburg, Germany.

出版信息

Br J Cancer. 1999 Mar;79(7-8):1037-41. doi: 10.1038/sj.bjc.6690166.

Abstract

The expression of the Ku70 and Ku80 genes as well as the activity of the DNA-dependent protein kinase (DNA-PK) were studied in 11 normal human fibroblast lines. The proteins studied are known to be part of a double-strand break (dsb) repair complex involved in non-homologous recombination, as was demonstrated for the radiosensitive rodent mutant cell lines of the complementation groups 5-7. The 11 fibroblast lines used in this study represent a typical spectrum of normal human radiosensitivity with the surviving fraction measured for a dose of 3.5 Gy, SF3.5 GY, ranging from 0.03 to 0.28. These differences in cell survival were previously shown to correlate with the number of non-repaired dsbs. We found that the mRNA signal intensities of both Ku70 and Ku80 genes were fairly similar for the 11 cell lines investigated. In addition, the DNA-PK activity determined by the pulldown assay was fairly constant in these fibroblast lines. Despite the correlation between cell survival and dsb repair capacity, there was no correlation between dsb repair capacity and DNA-PK activity in the tested normal human fibroblast lines. Obviously, in this respect, other proteins/pathways appear to be more relevant.

摘要

在11种正常人成纤维细胞系中研究了Ku70和Ku80基因的表达以及DNA依赖性蛋白激酶(DNA-PK)的活性。所研究的蛋白质已知是参与非同源重组的双链断裂(dsb)修复复合物的一部分,这在互补组5-7的放射敏感啮齿动物突变细胞系中得到了证实。本研究中使用的11种成纤维细胞系代表了正常人放射敏感性的典型范围,剂量为3.5 Gy时的存活分数SF3.5 GY在0.03至0.28之间。先前已表明细胞存活的这些差异与未修复的dsb数量相关。我们发现,在所研究的11种细胞系中,Ku70和Ku80基因的mRNA信号强度相当相似。此外,通过下拉试验测定的DNA-PK活性在这些成纤维细胞系中相当恒定。尽管细胞存活与dsb修复能力之间存在相关性,但在所测试的正常人成纤维细胞系中,dsb修复能力与DNA-PK活性之间没有相关性。显然,在这方面,其他蛋白质/途径似乎更相关。

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