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苯并[a]芘二醇环氧化物诱导二倍体人成纤维细胞的锚定非依赖性。细胞原癌基因分析。

Benzo[a]pyrene-diol-epoxide-induced anchorage-independence in diploid human fibroblasts. Analysis of cellular protooncogenes.

作者信息

Stevens C W, Brondyk W H, Fahl W E

机构信息

McArdle Laboratory for Cancer Research, University of Wisconsin, Madison 53706.

出版信息

J Cancer Res Clin Oncol. 1989;115(2):118-28. doi: 10.1007/BF00397911.

Abstract

Treatment of diploid human fibroblasts with stereoisomeric benzo[alpha]pyrene anti and syn diol epoxides has been shown to induce anchorage-independent clones of cells with a dose dependence and frequency [(0.5-12) X 10(-4)] not significantly different from mutations at the hypoxanthine-guanine phosphoribosyltransferase locus [(1-8) X 10(-4)] in these cells. The majority of the anchorage-independent clones that were picked retained their mutagen-induced, anchorage-independent phenotype through at least 20 generations of expansion in monolayer culture. No variant cells showing extended life-span were detected among survivors in any of the mutagen treatment groups (less than 1.6 X 10(-7) frequency). Extensive analysis of a pool of 15 cellular protooncogenes (Ha-ras, Ki-ras, N-ras, mos, fos, fes, myc, abl, sis, myb, erbA, erbB, src, raf, N-myc), using Southern and northern blot analysis, was done to determine whether mutagen-induced rearrangement, amplification or overexpression of any of these genes was responsible for the mutagen-induced, anchorage-independent phenotype. We found no evidence that the genomic arrangement or expression level of any of these genes had been altered, thus indicating that an alternative form of mutation, or an alternative gene not included in this screening was responsible for the mutagen-induced, anchorage-independent phenotype.

摘要

用立体异构的苯并[a]芘反式和顺式二醇环氧化物处理二倍体人成纤维细胞,已显示可诱导出不依赖贴壁的细胞克隆,其剂量依赖性和频率[(0.5 - 12)×10⁻⁴]与这些细胞次黄嘌呤 - 鸟嘌呤磷酸核糖基转移酶位点的突变频率[(1 - 8)×10⁻⁴]无显著差异。挑选出的大多数不依赖贴壁的克隆在单层培养中至少经过20代扩增后仍保留其诱变诱导的不依赖贴壁表型。在任何诱变处理组的存活细胞中均未检测到显示寿命延长的变异细胞(频率小于1.6×10⁻⁷)。使用Southern和Northern印迹分析对15个细胞原癌基因(Ha - ras、Ki - ras、N - ras、mos、fos、fes、myc、abl、sis、myb、erbA、erbB、src、raf、N - myc)进行了广泛分析,以确定这些基因中的任何一个的诱变诱导重排、扩增或过表达是否导致了诱变诱导的不依赖贴壁表型。我们没有发现证据表明这些基因中的任何一个的基因组排列或表达水平发生了改变,因此表明是另一种突变形式或该筛选中未包括的另一个基因导致了诱变诱导的不依赖贴壁表型。

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