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HeLa细胞中EGFP构建体的自发及MNNG诱导的回复突变:一种通过荧光显微镜观察活细胞中突变的检测方法。

Spontaneous and MNNG-induced reversion of an EGFP construct in HeLa cells: an assay for observing mutations in living cells by fluorescent microscopy.

作者信息

Gemignani F, Landi S, DeMarini D M, Kole R

机构信息

Lineberger Comprehensive Cancer Center and Department of Pharmacology, University of North Carolina, Chapel Hill, North Carolina, USA.

出版信息

Hum Mutat. 2001 Dec;18(6):526-34. doi: 10.1002/humu.1229.

Abstract

A HeLa cell line stably expressing the enhanced green fluorescence protein (EGFP) gene, interrupted by the HBB IVS2-654 intron, was studied without treatment and after treatment with a single standard dose of 15 microM of N-methyl-N'-nitro-N-nitrosoguanidine (MNNG). This assay was done in order to prove that such a construct can revert by a variety of mechanisms and that it produces a visible phenotype, i.e., green fluorescence. The system permits visual detection of living mutant cells among a background of non-mutant cells and does not require a selective medium. The results show that the construct reverts by large deletions (-62, -100, and -162 bp), small insertions (+4 bp), small rearrangements (19 bp duplication), base substitutions at purines (G652, G653, A655, G579), and a pyrimidine (T654) between nucleotide positions 579 and 837. Splice-site mutations were recovered, and some of the mechanisms underlying these mutations are discussed. Because of the ease of detection of revertant cells under fluorescent light and the wide variety of mutations that can be recovered, further development of this system could make it a useful new mammalian cell mutagenicity assay.

摘要

对一种稳定表达增强型绿色荧光蛋白(EGFP)基因的HeLa细胞系进行了研究,该基因被HBB IVS2 - 654内含子中断,研究内容包括未处理时以及用15微摩尔的N - 甲基 - N'- 硝基 - N - 亚硝基胍(MNNG)单标准剂量处理后。进行该试验是为了证明这样的构建体可以通过多种机制回复突变,并且它会产生可见的表型,即绿色荧光。该系统允许在非突变细胞背景中目视检测存活的突变细胞,并且不需要选择性培养基。结果表明,构建体通过大的缺失(-62、-100和-162碱基对)、小的插入(+4碱基对)、小的重排(19碱基对重复)、嘌呤(G652、G653、A655、G579)和嘧啶(T654)在核苷酸位置579和837之间的碱基替换回复突变。恢复了剪接位点突变,并讨论了这些突变背后的一些机制。由于在荧光灯下易于检测回复细胞以及可以恢复的多种突变类型,该系统的进一步开发可能使其成为一种有用的新型哺乳动物细胞致突变性试验。

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