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转基因大蓝鼠2和大蓝鼠胚胎成纤维细胞系的细胞遗传学特征分析。

Cytogenetic characterization of the transgenic Big Blue Rat2 and Big Blue mouse embryonic fibroblast cell lines.

作者信息

Erexson G L, Cunningham M L, Tindall K R

机构信息

Molecular Mutagenesis Group, Laboratory of Environmental Carcinogenesis and Mutagenesis, National Institute of Environmental Health Sciences, Research Triangle Park, NC 27709, USA.

出版信息

Mutagenesis. 1998 Nov;13(6):649-53. doi: 10.1093/mutage/13.6.649.

Abstract

The transgenic Big Blue Rat2 and Big Blue mouse embryonic fibroblast cell lines have been used to complement the transgenic Big Blue rat and mouse in vivo mutagenesis assays. However, limited information is available regarding the karyology of these cell lines. Therefore, we have characterized the ploidy, mitotic index, spontaneous frequencies of chromosome and chromatid aberrations and rate of micronucleus (MN) formation in both cell lines. We have also characterized the frequency of sister chromatid exchange (SCE) in transgenic Big Blue mouse cells. Big Blue Rat2 cells are hyperploid and have extremely high baseline frequencies of cytogenetic damage. In addition, Big Blue Rat2 cells are BrdU-resistant, therefore, SCE frequencies cannot be assessed in these cells. We conclude that Big Blue Rat2 cells are not useful for routine cytogenetic toxicology studies. The transgenic Big Blue mouse cell line is polyploid and consistently yields a low mitotic index (approximately 1%) in untreated cells. These mouse cells also exhibited moderately high baseline frequencies of chromosome and chromatid aberrations, however, baseline frequencies of SCE and of MN were not elevated. Transgenic Big Blue mouse embryonic fibroblasts were further studied for MN induction following treatment with N-ethyl-N-nitrosourea (ENU) for 0.5 h at concentrations of 0.425, 0.85 and 1.7 mM. Concentration-dependent increases in MN were observed in these cells. Thus, while an ENU-induced cytogenetic response using transgenic Big Blue mouse cells demonstrates that this cellular model could be used to cytogenetically complement the mutagenesis assays, the low mitotic index and the high spontaneous frequency of chromosome damage confounds its use for routine genetic toxicology studies.

摘要

转基因大蓝鼠2和大蓝鼠胚胎成纤维细胞系已用于补充转基因大蓝鼠和大蓝鼠体内诱变试验。然而,关于这些细胞系的核型的信息有限。因此,我们已经对这两种细胞系的倍性、有丝分裂指数、染色体和染色单体畸变的自发频率以及微核(MN)形成率进行了表征。我们还对转基因大蓝鼠细胞中的姐妹染色单体交换(SCE)频率进行了表征。大蓝鼠2细胞是超倍体,具有极高的细胞遗传学损伤基线频率。此外,大蓝鼠2细胞对溴脱氧尿苷(BrdU)具有抗性,因此,无法在这些细胞中评估SCE频率。我们得出结论,大蓝鼠2细胞对于常规细胞遗传学毒理学研究没有用处。转基因大蓝鼠细胞系是多倍体,在未处理的细胞中始终产生较低的有丝分裂指数(约1%)。这些小鼠细胞还表现出中等程度的高染色体和染色单体畸变基线频率,然而,SCE和MN的基线频率并未升高。在用0.425、0.85和1.7 mM的浓度的N-乙基-N-亚硝基脲(ENU)处理0.5小时后,对转基因大蓝鼠胚胎成纤维细胞进行了MN诱导的进一步研究。在这些细胞中观察到MN呈浓度依赖性增加。因此,虽然使用转基因大蓝鼠细胞的ENU诱导的细胞遗传学反应表明这种细胞模型可用于细胞遗传学上补充诱变试验,但低有丝分裂指数和高染色体损伤自发频率使其难以用于常规遗传毒理学研究。

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